TY  - JOUR
A1  - Al-Kassab, Jasser
A1  - Thiesse, Frederic
A1  - Buckel, Thomas
T1  - RFID Data Analytics in Retail Logistics: A Case Example
JF  - Journal of Theoretical and Applied E-Commerce Research
N2  - The growing interest in Radio Frequency Identification (RFID) technology in recent years has sparked an intensive debate on the benefits to be expected. With the growth of RFID implementations in size and scope comes a shift away from infrastructural aspects to the question of how to draw value from the large amounts of collected data. However, the necessary procedures for the handling of massive RFID data sets are still an under-researched issue. Against this background, the study presents results from a real-world trial conducted by a large apparel retailer. The objective of the trial was to explore the opportunities for generating novel performance indicators and reports on the reality of store processes and customer behavior on the sales floor. We give an overview of the algorithms used for RFID data processing and the interpretation of the resulting insights from a practitioner’s point of view. The case example thus provides an overview of the potential of RFID as a powerful tool for assortment optimization, customer research, store layout design, and other management tasks in retail.
KW  - RFID
KW  - apparel retail
KW  - store logistics
KW  - data management
KW  - business analytics
Y1  - 2013
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-129500
VL  - 8
IS  - 2
ER  - 
TY  - JOUR
A1  - Al-Janabi, Omar
A1  - Taubert, Helge
A1  - Lohse-Fischer, Andrea
A1  - Fröhner, Michael
A1  - Wach, Sven
A1  - Stöhr, Robert
A1  - Keck, Bastian
A1  - Burger, Max
A1  - Wieland, Wolf
A1  - Erdmann, Kati
A1  - Wirth, Manfred P.
A1  - Wullich, Bernd
A1  - Baretton, Gustavo
A1  - Magdolen, Viktor
A1  - Kotzsch, Mathias
A1  - Füssel, Susanne
T1  - Association of Tissue mRNA and Serum Antigen Levels of Members of the Urokinase-Type Plasminogen Activator System with Clinical and Prognostic Parameters in Prostate Cancer
JF  - Biomed Research International
N2  - The objective was to determine the mRNA expression and protein levels of uPA system components in tissue specimens and serum samples, respectively, from prostate cancer (PCa) patients and to assess their association with clinicopathological parameters and overall survival (OS). The mRNA expression levels of uPA, its receptor (uPAR), and its inhibitor type 1 (PAI-1) were analyzed in corresponding malignant and adjacent nonmalignant tissue specimens from 132 PCa patients by quantitative PCR. Preoperative serum samples from 81 PCa patients were analyzed for antigen levels of uPA system members by ELISA. RNA levels of uPA system components displayed significant correlations with each other in the tumor tissues. A significantly decreased uP AmRNA expression in PCa compared to the corresponding nonmalignant tissue was detected. High uPA mRNA level was significantly associated with a high Gleason score. Elevated concentration of soluble uPAR (suPAR) in serum was significantly associated with a poor OS of PCa patients (P = 0.022). PCa patients with high suPAR levels have a significantly higher risk of death (multivariate Cox's regression analysis; IIR - 7.12, P - 0.027). The association of high suPAR levels with poor survival of PCa patients suggests a prognostic impact of suPAR levels in serum of cancer patients.
KW  - receptor splice variant
KW  - primary breast cancer
KW  - radical prostatectomy
KW  - tumor tissue
KW  - progression
KW  - potential marker
KW  - inhibitor PAI-1
KW  - gastric cancer
KW  - biomarkers UPA
KW  - expression
Y1  - 2014
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-117967
SN  - 2314-6141
IS  - 972587
ER  - 
TY  - THES
A1  - AL-Hijailan, Reem Saud
T1  - Establishment of endothelialized cardiac tissue using human induced pluripotent stem cells generated cardiomyocytes
T1  - Etablierung eines endothelialisierten kardialen Gewebes mittels Kardiomyozyten, differenziert aus induzierten pluripotenten Stammzellen
N2  - Cardiovascular diseases are considered the leading cause of death worldwide according to the World Health Organization. Heart failure is the last stage of most of these diseases, where loss of myocardium leads to architectural and functional decline. 
The definitive treatment option for patients with CVDs is organ or tissue transplantation, which relies on donor availability. Therefore, generating an autologous bioengineered myocardium or heart could overcome this limitation. In addition, generating cardiac patches will provide ventricular wall support and enable reparative stem cells delivery to damaged areas.  Although many hurdles still exist, a good number of researches have attempted to create an engineered cardiac tissue which can induce endogenous cardiac repair by replacing damaged myocardium. 
The present study provided cardiac patches in two models, one by a detergent coronary perfusion decellularization protocol that was optimized, and the other that resulted in a 3D cell-free extracellular matrix with intact architecture and preserved s-glycosaminoglycan and vasculature conduits.  Perfusion with 1% Sodium dodecyle sulfate (SDS) under constant pressure resulted in cell-free porcine scaffold within two and cell-free rat scaffold in 7 days, whereas scaffold perfused with 4% sodium deoxycholate (SDO) was not able to remove cells completely.  Re-reendothelialization of tissue vasculature was obtained by injecting human microvascular endothelial cell and human fibroblast in 2:1 ratio in a dynamic culture. One-week later, CD31 positive cells and endothelium markers were observed, indicating new blood lining. Moreover, functionality test of re-endothelialized tissue revealed improvement in clotting seen in decellularized tissues.  When the tissue was ready to be repopulated, porcine induced pluripotent stem cells (PiPSc) were generated by transfected reprogramming of porcine skin fibroblast and then differentiated to cardiac cells following a robust protocol, for an autologous cardiac tissue model. However, due to the limitation in the PiPSc cell number, alternatively, human induced pluripotent stem cells generated cardiac cells were used. 
For reseeding a coculture of human iPSc generated cardiac cells, human mesenchymal stem cells and human fibroblast in 2:1:1 ratio respectively were used in a dynamic culture for 6-8 weeks. Contractions at different areas of the tissue were recorded at an average beating rate of 67 beats/min.  In addition, positive cardiac markers (Troponin T), Fibroblast (vemintin), and mesenchymal stem cells (CD90) were detected.  Not only that, but by week 3, MSC started differentiating to cardiac cells progressively until few CD90 positive cells were very few by week 6 with increasing troponin t positive cells in parallel.  Electrophysiological and drug studies were difficult to obtain due to tissue thickness and limited assessment sources. However, the same construct was established using small intestine submucosa (SISer) scaffold, which recorded a spontaneous beating rate between 0.88 and 1.2 Hz, a conduction velocity of 23.9 ± 0.74 cm s−1, and a maximal contraction force of 0.453 ± 0.015 mN. Moreover, electrophysiological studies demonstrated a drug-dependent response on beating rate; a higher adrenalin frequency was revealed in comparison to the untreated tissue and isoproterenol administration, whereas a decrease in beating rate was observed with propranolol and untreated tissue. 
The present study demonstrated the establishment of vascularized cardiac tissue, which can be used for human clinical application.
N2  - Etablierung eines endothelialisierten kardialen Gewebes mittels Kardiomyozyten, differenziert aus induzierten pluripotenten Stammzellen
KW  - cardiac tissue
KW  - biological scaffolds
KW  - decellularization
KW  - induced pluripotent stem cells
Y1  - 2019
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-173979
ER  - 
TY  - JOUR
A1  - Al-Hejailan, Reem
A1  - Weigel, Tobias
A1  - Schürlein, Sebastian
A1  - Berger, Constantin
A1  - Al-Mohanna, Futwan
A1  - Hansmann, Jan
T1  - Decellularization of full heart — optimizing the classical sodium-dodecyl-sulfate-based decellularization protocol
JF  - Bioengineering
N2  - Compared to cell therapy, where cells are injected into a defect region, the treatment of heart infarction with cells seeded in a vascularized scaffold bears advantages, such as an immediate nutrient supply or a controllable and persistent localization of cells. For this purpose, decellularized native tissues are a preferable choice as they provide an in vivo-like microenvironment. However, the quality of such scaffolds strongly depends on the decellularization process. Therefore, two protocols based on sodium dodecyl sulfate or sodium deoxycholate were tailored and optimized for the decellularization of a porcine heart. The obtained scaffolds were tested for their applicability to generate vascularized cardiac patches. Decellularization with sodium dodecyl sulfate was found to be more suitable and resulted in scaffolds with a low amount of DNA, a highly preserved extracellular matrix composition, and structure shown by GAG quantification and immunohistochemistry. After seeding human endothelial cells into the vasculature, a coagulation assay demonstrated the functionality of the endothelial cells to minimize the clotting of blood. Human-induced pluripotent-stem-cell-derived cardiomyocytes in co-culture with fibroblasts and mesenchymal stem cells transferred the scaffold into a vascularized cardiac patch spontaneously contracting with a frequency of 25.61 ± 5.99 beats/min for over 16 weeks. The customized decellularization protocol based on sodium dodecyl sulfate renders a step towards a preclinical evaluation of the scaffolds.
KW  - tissue engineering
KW  - decellularization
KW  - vascularized scaffold
KW  - cardiac patch
KW  - dynamic culture
Y1  - 2022
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-270781
SN  - 2306-5354
VL  - 9
IS  - 4
ER  - 
TY  - THES
A1  - Al-Farajat, Mohammad
T1  - Hydrogeo-Eco-Systems in Aquaba/Jordan - Coasts and Region
T1  - Hydrogeo-Ökosysteme an der Küste und in der Region Aquaba/Jordanien
N2  - The coast of Aqaba and the Aqaba region (Jordan) were investigated on their hydrogeo-ecosystem. The results of the research were translated into digits to build a geo-spatial data base. The fillings of the graben aquifer receive indirect type of recharge through the side wadis which drain the highlands. Surface water balance was modeled for a period of 20 years of daily climate records using MODBIL program which attributes direct recharge to wet years only. The hydrodynamic fresh water/seawater interface in the coastal zones was investigated by applying vertical geoelectric surveys and models of several methods to confirm its coincidence with the aquifer’s flow amounts, where human impacts in terms of over-pumping allowed more encroachment of seawater into land, and unintended recharge which led to seaward interface migration. A groundwater balance and solute transport were approached by developing a flow model from the hydrogeological and hydrochemical data. The nature of soil cover and aquifer whose physical properties enhance human impacts indicated the vulnerability of groundwater to pollution. This certainly threatens the marine ecology which forms the sink where the in-excess flow ends. The constructed digital background was exported into GIS to sub-zone the study area in terms of the aquifer’s vulnerability to pollution risks using DRASTIC index. However, it was unable to meet all geo-spatial factors that proved to have significant impacts on the vulnerability. Consequently, a comprehensive index -SALUFT- was developed. This suggests the suitable land use units for each zone in the light of vulnerability grades aiming at protecting the available groundwater resources.
N2  - Die Küste und die Region von Aqaba (Jordanien) wurde im Hinblick auf ihre Hydrogeo-ökosysteme untersucht. Die Ergebnisse dieser Forschungsarbeiten wurden in eine digitale Form überführt, um bezüglich der Geofaktoren ein realitätsnahes Abbild der Umgebung zu erzeugen. Der Graben-Aquifer erhält seine Grundwasserneubildung meist indirekt von den Seiten, von denen Wadis ihr Wasser abführen. Die Bilanzierung des Oberflächenwassers wurde aus Tagesklimawerten der letzten 20 Jahre unter Benutzung des Programms MODBIL errechnet. Daraus ergab sich eine Neubildung des Grundwassers nur in feuchten Jahren. Die hydrodynamische Süßwasser-Salzwasser-Mischungsfront im Küstenbereich wurde durch geoelektrische Tiefensondierungen untersucht. Durch Modellierungen mit verschiedenen Methoden wurden Fließgeschwindigkeit und Wassermenge dort mit der des Aquifers in Einklang gebracht, wo durch Überpumpen das Salzwasser weiter ins Landesinnere vordringt. Durch die Entwicklung eines Fließmodells aus den hydrogeologischen und hydrochemischen Daten konnte die Grundwasserbilanzierung und der Stofftransport ermittelt werden. Die Natur des Bodens und des Aquifers, deren physikalische Eigenschaften die Einflüsse durch menschliche Aktivitäten steigern, führt zu einer Anfälligkeit gegenüber Verschmutzung, die die Qualität des Grundwassers verschlechtert. Dies beeinflusst die Ökologie des Meeres, das an den Stellen als Schadstoffsenke dient, an denen die Grundwasserströme enden. Die im Computer erstellte digitale Umgebung wurde dazu genutzt, den Aquifer im Untersuchungsgebiet mit Hilfe von GIS in Zonen unterschiedlicher Verschmutzungs-empfindlichkeit zu unterteilen. Dazu wurde der DRASTIC-Index benutzt. Im Laufe der Untersuchungen zeigte sich allerdings, dass es nicht möglich war, alle Faktoren, die einen signifikanten Einfluss auf das System haben, mit Hilfe dieses Index zu erfassen. Aus diesem Grund wurde der SALUFT-Index entwickelt. Damit wurde es möglich, bezüglich der Verschmutzungsempfindlichkeit für jede Zone die günstigste Art der Landnutzung zu ermitteln, um die verfügbaren Grundwasserressourcen zu schützen.
KW  - Golf von Akaba
KW  - Akaba
KW  - Hydrogeologie
KW  - Hydrologie
KW  - Ökosystem
KW  - farajat
KW  - aqaba
KW  - umwelt
KW  - grundwasser
KW  - verschmutzung
KW  - boden
KW  - geophysik
KW  - jordanien
KW  - wasser
KW  - farajat
KW  - aqaba
KW  - environment
KW  - groundwater
KW  - pollution
KW  - soil
KW  - geophysics
KW  - jordan
KW  - water
Y1  - 2001
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-1182066
ER  - 
TY  - THES
A1  - Al-Baidhani, Mohammed
T1  - Spectroscopy as a tool to investigate the high energy optical properties of nanostructured magnetically doped topological insulator
T1  - Spektroskopie als Methode zur Untersuchung der optischen Eigenschaften nanostrukturierter, magnetisch dotierter Topologischer Isolatoren bei hohen Energien
N2  - In this dissertation the electronic and high-energy optical properties of thin nanoscale
films of the magnetic topological insulator (MTI) (V,Cr)y(BixSb1-x)2-yTe3 are studied
by means of X-ray photoelectron spectroscopy (XPS) and electron energy-loss
spectroscopy (EELS). Magnetic topological insulators are presently of broad interest
as the combination of ferromagnetism and spin-orbit coupling in these materials
leads to a new topological phase, the quantum anomalous Hall state (QAHS), with
dissipation less conduction channels. Determining and controlling the physical
properties of these complex materials is therefore desirable for a fundamental understanding
of the QAHS and for their possible application in spintronics. EELS can
directly probe the electron energy-loss function of a material from which one can
obtain the complex dynamic dielectric function by means of the Kramers-Kronig
transformation and the Drude-Lindhard model of plasmon oscillations.
The XPS core-level spectra in (V,Cr)y(BixSb1-x)2-yTe3 are analyzed in detail with
regards to inelastic background contributions. It is shown that the spectra can be
accurately described based on the electron energy-loss function obtained from an
independent EELS measurement. This allows for a comprehensive and quantitative
analysis of the XPS data, which will facilitate future core-level spectroscopy studies
in this class of topological materials. From the EELS data, furthermore, the bulk and
surface optical properties were estimated, and compared to ab initio calculations
based on density functional theory (DFT) performed in the GW approximation
for Sb2Te3. The experimental results show a good agreement with the calculated
complex dielectric function and the calculated energy-loss function. The positions of
the main plasmon modes reported here are expected to be generally similar in other
materials in this class of nanoscale TI films. Hence, the present work introduces
EELS as a powerful method to access the high-energy optical properties of TI
thin films. Based on the presented results it will be interesting to explore more
systematically the effects of stoichiometry, magnetic doping, film thickness and
surface morphology on the electron-loss function, potentially leading to a better
understanding of the complex interplay of structural, electronic, magnetic and
optical properties in MTI nanostructures.
N2  - Die vorliegende Dissertation beschäftigt sich mit den elektronischen und hochen- ergetischen optischen Eigenschaften von auf der Nanoskala dünnen Filmen des magnetischen topologischen Isolators (MTI) (V,Cr)y(BixSb1−x)2−yTe3 mithilfe von Röntgenphotoelektronenspektroskopie (engl.: X-ray photoelectron spectroscopy, XPS), sowie Elektronenenergieverlustspektroskopie (engl.: electron energy-loss spectroscopy, EELS). Magnetische topologische Isolatoren sind gegenwärtig von großem Interesse, da die Kombination von Ferromagnetismus und Spin-Bahn- Kopplung in diesen Materialien zu einer neuen topologischen Phase führt, der Quanten-Anomalen-Hall-Phase (engl.: quantum anomalous Hall state, QAHS), die sich durch verlustfreie Leitungskanäle auszeichnet. Bestimmung und Kontrolle der physikalischen Eigenschaften dieser komplexen Materialien ist somit erstrebenswert für ein fundamentales Verständnis des QAHS sowie für Anwendungen in der Spin- tronik. EELS erlaubt die direkte Untersuchung der Elektronenenergieverlustfunk- tion eines Materials, aus der man, mithilfe der Kramers-Kronig-Transformation und des Drude-Lindhard-Modells von Plasmonenoszillationen, die komplexe dynamis- che dielektrische Funktion des Materials erhält.
In den XPS-Spektren der Rumpfniveaus in (V,Cr)y(BixSb1−x)2−yTe3 wird detail- liert insbesondere der Beitrag des inelastischen Untergrunds analysiert. Es kann gezeigt werden, dass, basierend auf der in einem unabhängigen EELS-Experiment gewonnenen Elektronenenergieverlustfunktion, die Rumpfniveauspektren präzise beschrieben werden können. Dies erlaubt eine umfangreiche und quantitative Anal- yse der Daten, was zukünftige Rumpfniveaustudien dieser Klasse topologischer Materialien erleichtern wird. Die mit EELS gewonnenen Daten ermöglichen weiter- hin eine Abschätzung der optischen Eigenschaften von Volumen und Oberfläche der Materialien, die in der vorliegenden Arbeit mit ab initio Berechnungen aus der Literatur für Sb2Te3 verglichen werden, welche auf Basis der Dichtefunktionaltheo- rie (DFT) in GW-näherung durchgeführt wurden. Die experimentellen Ergebnisse zeigen gute Übereinstimmungen mit der berechneten komplexen dielektrischen Funktion, sowie mit der Energieverlustfunktion. Es wird erwartet, dass die hier beschriebenen Positionen der Hauptplasmonenmoden im Allgemeinen ähnlich zu denen anderer Materialien dieser Klasse auf der Nanoskala dünner topologischer Isolatoren sind. Somit stellt die vorliegende Arbeit das EELS Experiment als eine mächtige Methode vor, die einen Zugang zu den hochenergetischen optischen Eigen- schaften dünner TIs schafft. Basierend auf den hier vorgestellten Ergebnissen bleibt es interessant sein die Auswirkungen von Stöchiometrie, magnetischer Dotierung, Filmdicke, sowie Oberflächenmorphologie auf die Energieverlustfunktion system- atischer zu untersuchen, um damit ein besseres Verständnis für das komplexe Zusammenspiel aus strukturellen, elektronischen und optischen Eigenschaften in MTI-Nanostrukturen zu erlangen.
KW  - spectroscopy
KW  - XPS
KW  - REELS
KW  - topological insulator
KW  - QAHE
KW  - Topologischer Isolator
KW  - Optische Eigenschaft
KW  - Elektronenspektroskopie
Y1  - 2018
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-157221
ER  - 
TY  - JOUR
A1  - Aktas, Bertal H.
A1  - Upcin, Berin
A1  - Henke, Erik
A1  - Padmasekar, Manju
A1  - Qin, Xuebin
A1  - Ergün, Süleyman
T1  - The Best for the Most Important: Maintaining a Pristine Proteome in Stem and Progenitor Cells
JF  - Stem Cells International
N2  - Pluripotent stem cells give rise to reproductively enabled offsprings by generating progressively lineage-restricted multipotent stem cells that would differentiate into lineage-committed stem and progenitor cells. These lineage-committed stem and progenitor cells give rise to all adult tissues and organs. Adult stem and progenitor cells are generated as part of the developmental program and play critical roles in tissue and organ maintenance and/or regeneration. The ability of pluripotent stem cells to self-renew, maintain pluripotency, and differentiate into a multicellular organism is highly dependent on sensing and integrating extracellular and extraorganismal cues. Proteins perform and integrate almost all cellular functions including signal transduction, regulation of gene expression, metabolism, and cell division and death. Therefore, maintenance of an appropriate mix of correctly folded proteins, a pristine proteome, is essential for proper stem cell function. The stem cells' proteome must be pristine because unfolded, misfolded, or otherwise damaged proteins would interfere with unlimited self-renewal, maintenance of pluripotency, differentiation into downstream lineages, and consequently with the development of properly functioning tissue and organs. Understanding how various stem cells generate and maintain a pristine proteome is therefore essential for exploiting their potential in regenerative medicine and possibly for the discovery of novel approaches for maintaining, propagating, and differentiating pluripotent, multipotent, and adult stem cells as well as induced pluripotent stem cells. In this review, we will summarize cellular networks used by various stem cells for generation and maintenance of a pristine proteome. We will also explore the coordination of these networks with one another and their integration with the gene regulatory and signaling networks.
KW  - Endoplasmic-Reticulum Stress
KW  - Heme-regulated inhibitor
KW  - Human Muse Cells
KW  - Transcription factor NRF1
KW  - ER-Stress
KW  - Hematopoietic Stem
KW  - Quality-control
KW  - Messenger-RNAs
KW  - Neural Differentiation
KW  - Translation Initiation
Y1  - 2019
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-227769
ER  - 
TY  - JOUR
A1  - Akshat, Puri
A1  - Aaboud, M.
A1  - Aad, G.
A1  - Abbott, B.
A1  - Abdinov, O.
A1  - Abeloos, B.
A1  - Abhayasinghe, D. K.
A1  - Abidi, S. H.
A1  - Abou Zeid, O. S.
A1  - Abraham, N. L.
A1  - Abramowicz, H.
A1  - Abreu, H.
A1  - Abulaiti, Y.
A1  - Acharya, B. S.
A1  - Adachi, S.
A1  - Adam, L.
A1  - Adamczyk, L.
A1  - Adelman, J.
A1  - Adersberger, M.
A1  - Adiguzel, A.
A1  - Adye, T.
A1  - Affolder, A. A.
A1  - Afik, Y.
A1  - Agheorghiesei, C.
A1  - Aguilar-Saavedra, J. A.
A1  - Ahmadov, F.
A1  - Aiellil, G.
A1  - Akatsuka, S.
A1  - Akesson, T. P. A.
A1  - Akilli, E.
A1  - Akimov, A. V.
A1  - Alberghi, G. L.
A1  - Albert, J.
A1  - Albicocco, P.
A1  - Alconada Verzini, M. J.
A1  - Alderweireld, S.
A1  - Aleksa, M.
A1  - Aleksandrov, I. N.
A1  - Alexa, C.
A1  - Alexopoulos, T.
A1  - Alhroob, M.
A1  - Ali, B.
A1  - Alimonti, G.
A1  - Alison, J.
A1  - Andre, S. P.
A1  - Allaire, C.
A1  - Allbrooke, B. M. M.
A1  - Allen, B. W.
A1  - Allport, P. P.
A1  - Aloisio, A.
A1  - Alonso, A.
A1  - Alonso, F.
A1  - Alpigiani, C.
A1  - Alshehri, A. A.
A1  - Alstaty, M. I.
A1  - Alvarez, Gonzalez B.
A1  - Alvarez Piqueras, D.
A1  - Alviggi, M. G.
A1  - Amadio, B. T.
A1  - Amaral, Coutinho, Y.
A1  - Ambler, A.
A1  - Ambroz, L.
A1  - Amelung, C.
A1  - Amidei, D.
A1  - Amor Dos Santos, S. P.
A1  - Amoroso, S.
A1  - Amrouche, C. S.
A1  - Anastopoulos, C.
A1  - Ancu, L. S.
A1  - Andari, N.
A1  - Andeen, T.
A1  - Anders, C. F.
A1  - Anders, J. K.
A1  - Anderson, K. J.
A1  - Andreazza, A.
A1  - Andrei, V.
A1  - et al, 
T1  - Measurement of angular and momentum distributions of charged particles within and around jets in Pb plus Pb and pp collisions at root s(NN)=5.02 TeV with ATLAS at the LHC : XXVIIth International Conference on Ultrarelativistic Nucleus-Nucleus Collisions
(Quark Matter 2018)
JF  - Nuclear Physics A
N2  - Studies of the fragmentation of jets into charged particles in heavy-ion collisions can help in understanding the mechanism of jet quenching by the hot and dense QCD matter created in such collisions, the quark-gluon plasma. These proceedings present a measurement of the angular distribution of charged particles around the jet axis in root s(NN) = 5.02 TeV Pb+Pb and pp collisions, done using the ATLAS detector at the LHC. The measurement is performed inside jets reconstructed with the anti-k(t) algorithm with radius parameter R = 0.4, and is extended to regions outside the jet cone. Results are presented as a function of Pb+Pb collision centrality, and both jet and charged-particle transverse momenta.
KW  - jets
KW  - fragmentation functions
KW  - jet shapes
Y1  - 2019
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-224703
VL  - 982
IS  - 2
ER  - 
TY  - THES
A1  - Akindeinde, Saheed Ojo
T1  - Numerical Verification of Optimality Conditions in Optimal Control Problems
T1  - Numerischen Verifizierung von Optimalitätsbedingungen für Optimalsteurungsprobleme
N2  - This thesis is devoted to numerical verification of optimality conditions for non-convex optimal control problems. In the first part, we are concerned with a-posteriori verification of sufficient optimality conditions. It is a common knowledge that verification of such conditions for general non-convex PDE-constrained optimization problems is very challenging. We propose a method to verify second-order sufficient conditions for a general class of optimal control problem. If the proposed verification method confirms the fulfillment of the sufficient condition then a-posteriori error estimates can be computed. A special ingredient of our method is an error analysis for the Hessian of the underlying optimization problem. We derive conditions under which positive definiteness of the Hessian of the discrete problem implies positive definiteness of the Hessian of the continuous problem. The results are complemented with numerical experiments. In the second part, we investigate adaptive methods for optimal control problems with finitely many control parameters. We analyze a-posteriori error estimates based on verification of second-order sufficient optimality conditions using the method developed in the first part. Reliability and efficiency of the error estimator are shown. We illustrate through numerical experiments, the use of the estimator in guiding adaptive mesh refinement.
N2  - Diese Arbeit widmet sich der numerischen Verifizierung von Optimalitaetsbedingungen fuer nicht konvexe Optimalsteuerungsprobleme. Im ersten Teil beschaeftigen wir uns mit der a-posteriori Ueberpruefung von hinreichenden Optimalitaetskriterien. Es ist bekannt, dass der Nachweis solcher Bedingungen fuer allgemeine nicht konvexe Optimierungsproblemem mit Nebenbedingungen in Form von partiellen Differentialgleichungen sehr schwierig ist. Wir stellen eine Methode vor, um die hinreichenden Bedingungen zweiter Ordnung fuer eine allgemeine Problemklasse zu testen. Falls die vorgeschlagene Strategie bestaetigt, dass diese Bedingungen erfuellt sind, koennen a-posteriori Fehlerschaetzungen berechnet werden. Ein wesentlicher Bestandteil unserer Methode ist eine Fehleranalyse fuer die Hessematrix des zugrunde liegenden Optimierungsproblems. Es werden Bedingungen hergeleitet, unter denen die positive Definitheit der Hessematrix des diskreten Problems die positive Definitheit der Hessematrix fuer das kontinuierliche Problem nach sich zieht. Diese Ergebnisse werden durch numerische Experimente ergaenzt. Im zweiten Teil untersuchen wir adaptive (Diskretisierungs-)methoden fuer Optimalsteuerungsprobleme mit endlich vielen Kontrollparametern. Basierend auf dem Nachweis hinreichender Optimalitaetsbedingungen zweiter Ordnung analysieren wir a posteriori Fehlerschaetzungen. Dies geschieht unter der Nutzung der Resultate des ersten Teils der Arbeit. Es wird die Zuverlaessigkeit und Effizienz des Fehlerschaetzers bewiesen. Mittels weiterer numerischer Experimente illustrieren wir, wie der Fehlerschaetzer zur Steuerung adaptiver Gitterverfeinerung eingesetzt werden kann.
KW  - Optimale Kontrolle
KW  - Nichtkonvexe Optimierung
KW  - Numerisches Verfahren
KW  - non-convex optimal control problems
KW  - sufficient optimality conditions
KW  - a-posteriori error estimates
KW  - numerical approximations
KW  - adaptive refinement
Y1  - 2012
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-76065
ER  - 
TY  - THES
A1  - Akimzhanov, Askar M.
T1  - Epigenetic repression of the NFATc1 transcription factor in human lymphomas
T1  - Epigenetische Repression des NFATc1 Transkriptionsfakors in menschlichen Lymphomen
N2  - We examined the regulation of NFATc1 in different lymphomas and observed an inversed correlation between the methylation status and expression of NFATc1. Our data demonstrate that aberrant DNA methylation associated with chromatin remodeling within nfatc1 locus is a major mechanism for the repression of NFATc1 expression, suggesting that the DNA methylation-mediated transcriptional silencing of NFATc1 may be a critical event in the tumorogenesis of ALCLs and cHLs. Furthermore, the DNA methylation of human nfatc1 promoter region could be used as a novel biomarker of tumor progression. Our results indicate a close link between the loss of immunoreceptor signaling and NFATc1 expression in human lymphomas. For both ALCLs and cHLs, defects in immunoreceptor signaling have been described which result in a loss of receptor-mediated gene expression programs (Schwering et al., 2003; Bonzheim et al., 2004; Marafioti et al., 2004). In T cells, one indicator gene of these programs appears to be the nfatc1 gene whose expression is controlled by TCR signals (Chuvpilo et al., 2002a). In contrast, in T cells NFATc1 expression is unaffected by TCR signals, and NFATc2 was found to be expressed at normal levels in ALCLs and cHLs (L.K., unpubl. data). Moreover, the activity of NF-kappaB factors which can bind to certain NFAT binding sites and share a distantly-related DNA binding domain with NFATs is strongly elevated in cHL cells (Bargou et al., 1997; Hinz et al., 2001; Hinz et al., 2002) suggesting that NFATs and NF-kappaBs exert very different effects on generation and maintenance of Hodgkin’s lymhomas. However, it should be mentioned that in Burkitt’s and further B cell lymphomas in which NFATc1 proteins are strongly expressed and controlled by receptor signals (Kondo et al., 2003), they could exert a promoting function in tumor development. The genes of p53 family members p63 and p73 are prominent examples for mammalian genes whose products can act both as oncoproteins and tumor suppressor genes (Hibi et al., 2000; Stiewe and Putzer, 2002), and it is likely that more genes exist which encode both tumor suppressors and oncoproteins. It remains to be shown whether the nfatc1 gene is one of them.
N2  - Wir haben die Regulation von NFATc1 in verschiedenen Lymphomen untersucht und beobachteten eine umgekehrte Korrelation zwischen dem Ausmaß an Methylierung und der Expression von NFATc1. Unsere Daten demonstrieren, dass eine aberrante DNA-Methylierung, die mit veränderter Chromatinstruktur innerhalb des nfatc1 Lokus assoziiert ist, der Hauptmechanismus für die Repression der NFATc1-Expression ist. Es wäre zu vermuten, dass die durch DNA-Methylierung verursachte transkriptionelle Abschaltung von NFATc1 der kritische Schritt bei der Tumorgenese von ALCLs und cHLs ist. Des weiteren könnte das Ausmaß der DNA-Methylierung in der humanen nfatc1-Promotorregion als neuer Biomarker für Tumorprogression genutzt werden. Unsere Daten indizieren eine enge Verbindung zwischen dem Verlust von Immunrezeptorsignalen und der NFATc1-Expression in humanen Lymphomen. Für sowohl ALCLs als auch cHLs wurden Defekte in der Immunrezeptorsignalgebung beschrieben, welche sich im Verlust des Rezeptor vermittelten Genexpressionsprogramms niederschlagen (Schwering et al., 2003; Bonzheim et al., 2004; Marafioti et al., 2004). In T-Zellen scheint das nfatc1-Gen eins der Indikatorgene dieses Programms zu sein, dessen Expression durch TCR-Signale kontrolliert wird (Chuvpilo et al., 2002a). Im Gegensatz dazu bleibt die NFATc2-Expression in T-Zellen unbeeinflusst von TCR-Signalen, weshalb NFATc2 in ALCLs und cHLs auch in normalem Ausmaß exprimiert wird (L.K., unpubl. data). Andererseits ist die Aktivität der NF-kappaB-Faktoren, die auch an bestimmte NFAT-Bindungsstellen binden können und deren DNA-Bindungsdomäne entfernt mit der der NFATs verwandt ist, in cHL-Zellen stark erhöht (Bargou et al., 1997; Hinz et al., 2001; Hinz et al., 2002). Das lässt vermuten, dass NFATc1 und die NF-kappa-Faktoren eine sehr unterschiedliche Rolle bei der Entstehung und dem Erhalt der Hodgkinlymphome spielen. Es sollte aber erwähnt werden, dass in Burkitts und anderen B-Zelllymphomen, in denen NFATc1-Proteine stark exprimiert und darüber hinaus durch Rezeptorsignale kontrolliert sind (Kondo et al., 2003), diese eine Tumor fördernde Funktion ausüben könnten. Die Gene der p53-Familienmitglieder p63 und p73 sind prominente Beispiele für Säugergene, deren Produkte sowohl als Onkoproteine als auch als Tumorsuppressoren fungieren können (Hibi et al., 2000; Stiewe and Putzer, 2002), und es ist wahrscheinlich, dass es noch weitere Gene gibt, die beide Funktionen ausüben. Es wird zu zeigen sein, ob das nfatc1-Gen eins von ihnen ist.
KW  - Lymphom
KW  - T-Lymphozyt
KW  - Transkriptionsfaktor
KW  - Methylierung
KW  - Epigenese
KW  - NFATc1
KW  - Lymphome
KW  - Epigenetik
KW  - Methylierung
KW  - NFATc1
KW  - Lymphoma
KW  - Epigenetics
KW  - Methylation
Y1  - 2005
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-12921
ER  - 
TY  - JOUR
A1  - Akhundzadah, Noor Ahmad
A1  - Soltani, Salim
A1  - Aich, Valentin
T1  - Impacts of climate change on the water resources of the Kunduz River Basin, Afghanistan
JF  - Climate
N2  - The Kunduz River is one of the main tributaries of the Amu Darya Basin in North Afghanistan. Many communities live in the Kunduz River Basin (KRB), and its water resources have been the basis of their livelihoods for many generations. This study investigates climate change impacts on the KRB catchment. Rare station data are, for the first time, used to analyze systematic trends in temperature, precipitation, and river discharge over the past few decades, while using Mann–Kendall and Theil–Sen trend statistics. The trends show that the hydrology of the basin changed significantly over the last decades. A comparison of landcover data of the river basin from 1992 and 2019 shows significant changes that have additional impact on the basin hydrology, which are used to interpret the trend analysis. There is considerable uncertainty due to the data scarcity and gaps in the data, but all results indicate a strong tendency towards drier conditions. An extreme warming trend, partly above 2 °C since the 1960s in combination with a dramatic precipitation decrease by more than −30% lead to a strong decrease in river discharge. The increasing glacier melt compensates the decreases and leads to an increase in runoff only in the highland parts of the upper catchment. The reduction of water availability and the additional stress on the land leads to a strong increase of barren land and a reduction of vegetation cover. The detected trends and changes in the basin hydrology demand an active management of the already scarce water resources in order to sustain water supply for agriculture and ecosystems in the KRB.
KW  - climate change
KW  - Kunduz River Basin
KW  - trend analysis
KW  - river discharge
KW  - landcover changes
Y1  - 2020
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-213199
SN  - 2225-1154
VL  - 8
IS  - 10
ER  - 
TY  - JOUR
A1  - Akhrif, Atae
A1  - Romanos, Marcel
A1  - Domschke, Katharina
A1  - Schmitt-Boehrer, Angelika
A1  - Neufang, Susanne
T1  - Fractal Analysis of BOLD Time Series in a Network Associated With Waiting Impulsivity
JF  - Frontiers in Physiology
N2  - Fractal phenomena can be found in numerous scientific areas including neuroscience. Fractals are structures, in which the whole has the same shape as its parts. A specific structure known as pink noise (also called fractal or 1/f noise) is one key fractal manifestation, exhibits both stability and adaptability, and can be addressed via the Hurst exponent (H). FMRI studies using H on regional fMRI time courses used fractality as an important characteristic to unravel neural networks from artificial noise. In this fMRI-study, we examined 103 healthy male students at rest and while performing the 5-choice serial reaction time task. We addressed fractality in a network associated with waiting impulsivity using the adaptive fractal analysis (AFA) approach to determine H. We revealed the fractal nature of the impulsivity network. Furthermore, fractality was influenced by individual impulsivity in terms of decreasing fractality with higher impulsivity in regions of top-down control (left middle frontal gyrus) as well as reward processing (nucleus accumbens and anterior cingulate cortex). We conclude that fractality as determined via H is a promising marker to quantify deviations in network functions at an early stage and, thus, to be able to inform preventive interventions before the manifestation of a disorder.
KW  - fMRI
KW  - Hurst Exponent
KW  - frontal cortex
KW  - nucleus accumbens
KW  - biomarker
KW  - impulse control disorders
Y1  - 2018
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-189191
SN  - 1664-042X
VL  - 9
ER  - 
TY  - THES
A1  - Akhrif, Atae
T1  - The BOLD Signal is more than a Brain Activation Index
T1  - Das BOLD Signal ist mehr als ein Maß für Hirnaktivierung
N2  - In the recent years, translational studies comparing imaging data of animals and humans have gained increasing scientific interests with crucial findings stemming from both, human and animal work. In order to harmonize statistical analyses of data from different species and to optimize the transfer of knowledge between them, shared data acquisition protocols and combined statistical approaches have to be identified. Following this idea, methods of data analysis, which have until now mainly been used to model neural responses of electrophysiological recordings from rodent data, were applied on human hemodynamic responses (i.e. Blood-Oxygen-Level-Dependent BOLD signal) as measured via functional magnetic resonance imaging (fMRI).
At the example of two attention and impulsivity networks, timing dynamics and amplitude of the fMRI signal were determined (study 1). Study 2 described the same parameters frequency-specifically, and in study 3, the complexity of neural processing was quantified in terms of fractality. Determined parameters were compared with regard to the subjects’ task performance / impulsivity to validate findings with regard to reports of the current scientific debate. 
In a general discussion, overlapping as well as additional information of methodological approaches were discussed with regard to its potential for biomarkers in the context of neuropsychiatric disorders.
N2  - In den letzten Jahren haben translationale Studien, in denen Befunde von Tieren und Menschen direkt verglichen werden, zunehmend an wissenschaftlichem Interesse gewonnen. Um statistische Analysen von Daten verschiedener Spezies zu harmonisieren und somit den Wissenstransfer zu optimieren, müssen gemeinsame Datenerfassungsprotokolle sowie kombinierte statistische Ansätze identifiziert werden. Diesem Gedanken folgend werden in dieser Arbeit Methoden der Datenanalyse, die bisher hauptsächlich zur Modellierung neuronaler Antworten aus elektrophysiologischer Aufzeichnungen bei Nagetierdaten verwendet wurden, auf hämodynamische Antworten (d.h. Blood-Oxygen-Level-Dependent BOLD-Signal), welche mittels funktionaler Magnetresonanztomo-graphie (fMRT) gemessen werden, im Menschen angewendet. 
Am Beispiel zweier Aufmerksamkeits- und Impulsivitätsnetzwerke wurden der zeitliche Verlauf und Amplitude des fMRI-Signals bestimmt (Studie 1). In Studie 2 wurden die gleichen Parameter frequenzspezifisch ausgewertet, und in Studie 3 wurde die Komplexität neuronaler Verarbeitung anhand von Fraktalität quantifiziert. Die ermittelten Parameter wurden hinsichtlich der Task Performance / Impulsivität der Probanden verglichen, um die Ergebnisse im Kontext von Befunden aus der aktuellen wissenschaftlichen Debatte zu validieren. 
In einer allgemeinen Diskussion wurden sowohl überlappende als auch zusätzliche Informationen zu methodischen Ansätzen hinsichtlich ihres Potenzials für Biomarker im Zusammenhang mit neuropsychiatrischen Erkrankungen diskutiert.
KW  - funktionelle Kernspintomographie
KW  - BOLD signal
KW  - fMRI time series
Y1  - 2020
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-207299
N1  - Aus datenschutzrechtlichen Gründen wurde der Zugriff auf den Volltext zu diesem Dokument gesperrt. Eine inhaltlich identische neue Version ist erhältlich unter:
https://doi.org/10.25972/OPUS-32287
ER  - 
TY  - THES
A1  - Akhrif, Atae
T1  - The BOLD Signal is more than a Brain Activation Index
T1  - Das BOLD Signal ist mehr als ein Maß für Hirnaktivierung
N2  - In the recent years, translational studies comparing imaging data of animals and humans have gained increasing
scientific interests with crucial findings stemming from both, human and animal work. In order to harmonize
statistical analyses of data from different species and to optimize the transfer of knowledge between them, shared
data acquisition protocols and combined statistical approaches have to be identified. Following this idea, methods
of data analysis, which have until now mainly been used to model neural responses of electrophysiological
recordings from rodent data, were applied on human hemodynamic responses (i.e. Blood-Oxygen-Level-
Dependent BOLD signal) as measured via functional magnetic resonance imaging (fMRI).
At the example of two attention and impulsivity networks, timing dynamics and amplitude of the fMRI signal were
determined (study 1). Study 2 described the same parameters frequency-specifically, and in study 3, the
complexity of neural processing was quantified in terms of fractality. Determined parameters were compared with
regard to the subjects’ task performance / impulsivity to validate findings with regard to reports of the current
scientific debate.
In a general discussion, overlapping as well as additional information of methodological approaches were
discussed with regard to its potential for biomarkers in the context of neuropsychiatric disorders.
N2  - In den letzten Jahren haben translationale Studien, in denen Befunde von Tieren und Menschen direkt verglichen
werden, zunehmend an wissenschaftlichem Interesse gewonnen. Um statistische Analysen von Daten
verschiedener Spezies zu harmonisieren und somit den Wissenstransfer zu optimieren, müssen gemeinsame
Datenerfassungsprotokolle sowie kombinierte statistische Ansätze identifiziert werden. Diesem Gedanken folgend
werden in dieser Arbeit Methoden der Datenanalyse, die bisher hauptsächlich zur Modellierung neuronaler
Antworten aus elektrophysiologischer Aufzeichnungen bei Nagetierdaten verwendet wurden, auf
hämodynamische Antworten (d.h. Blood-Oxygen-Level-Dependent BOLD-Signal), welche mittels funktionaler
Magnetresonanztomo-graphie (fMRT) gemessen werden, im Menschen angewendet.
Am Beispiel zweier Aufmerksamkeits- und Impulsivitätsnetzwerke wurden der zeitliche Verlauf und Amplitude des
fMRI-Signals bestimmt (Studie 1). In Studie 2 wurden die gleichen Parameter frequenzspezifisch ausgewertet, und
in Studie 3 wurde die Komplexität neuronaler Verarbeitung anhand von Fraktalität quantifiziert. Die ermittelten
Parameter wurden hinsichtlich der Task Performance / Impulsivität der Probanden verglichen, um die Ergebnisse
im Kontext von Befunden aus der aktuellen wissenschaftlichen Debatte zu validieren.
In einer allgemeinen Diskussion wurden sowohl überlappende als auch zusätzliche Informationen zu
methodischen Ansätzen hinsichtlich ihres Potenzials für Biomarker im Zusammenhang mit neuropsychiatrischen
Erkrankungen diskutiert.
KW  - BOLD signal
KW  - functional neuroimaging
KW  - fMRI time series
KW  - funktionelle Kernspintomographie
Y1  - 2023
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-322879
N1  - Dieses Dokument wurde aus Datenschutzgründen - ohne inhaltliche Änderungen - erneut veröffentlicht.
Die ursprüngliche Veröffentlichung war am 08.07.2020
ER  - 
TY  - JOUR
A1  - Akhoon, Bashir A.
A1  - Singh, Krishna P.
A1  - Varshney, Megha
A1  - Gupta, Shishir K.
A1  - Shukla, Yogeshwar
A1  - Gupta, Shailendra K.
T1  - Understanding the Mechanism of Atovaquone Drug Resistance in Plasmodium falciparum Cytochrome b Mutation Y268S Using Computational Methods
JF  - PLOS ONE
N2  - The rapid appearance of resistant malarial parasites after introduction of atovaquone (ATQ) drug has prompted the search for new drugs as even single point mutations in the active site of Cytochrome b protein can rapidly render ATQ ineffective. The presence of Y268 mutations in the Cytochrome b (Cyt b) protein is previously suggested to be responsible for the ATQ resistance in Plasmodium falciparum (P. falciparum). In this study, we examined the resistance mechanism against ATQ in P. falciparum through computational methods. Here, we reported a reliable protein model of Cyt bc1 complex containing Cyt b and the Iron-Sulphur Protein (ISP) of P. falciparum using composite modeling method by combining threading, ab initio modeling and atomic-level structure refinement approaches. The molecular dynamics simulations suggest that Y268S mutation causes ATQ resistance by reducing hydrophobic interactions between Cyt bc1 protein complex and ATQ. Moreover, the important histidine contact of ATQ with the ISP chain is also lost due to Y268S mutation. We noticed the induced mutation alters the arrangement of active site residues in a fashion that enforces ATQ to find its new stable binding site far away from the wild-type binding pocket. The MM-PBSA calculations also shows that the binding affinity of ATQ with Cyt bc1 complex is enough to hold it at this new site that ultimately leads to the ATQ resistance.
KW  - molecular-dynamics simulations
KW  - HIV-1 protease
KW  - structure prediction
KW  - saccharomyces cerevisiae
KW  - I-tasser
KW  - inhibitors
KW  - binding
KW  - malaria
KW  - complex
KW  - protein-protein interactions
Y1  - 2014
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-114882
VL  - 9
IS  - 10
ER  - 
TY  - JOUR
A1  - Akhoon, Bashir A.
A1  - Gupta, Shishir K.
A1  - Tiwari, Sudeep
A1  - Rathor, Laxmi
A1  - Pant, Aakanksha
A1  - Singh, Nivedita
A1  - Gupta, Shailendra K.
A1  - Dandekar, Thomas
A1  - Pandey, Rakesh
T1  - C. elegans protein interaction network analysis probes RNAi validated pro-longevity effect of nhr-6, a human homolog of tumor suppressor Nr4a1
JF  - Scientific Reports
N2  - Protein-protein interaction (PPI) studies are gaining momentum these days due to the plethora of various high-throughput experimental methods available for detecting PPIs. Proteins create complexes and networks by functioning in harmony with other proteins and here in silico network biology hold the promise to reveal new functionality of genes as it is very difficult and laborious to carry out experimental high-throughput genetic screens in living organisms. We demonstrate this approach by computationally screening C. elegans conserved homologs of already reported human tumor suppressor and aging associated genes. We select by this nhr-6, vab-3 and gst-23 as predicted longevity genes for RNAi screen. The RNAi results demonstrated the pro-longevity effect of these genes. Nuclear hormone receptor nhr-6 RNAi inhibition resulted in a C. elegans phenotype of 23.46% lifespan reduction. Moreover, we show that nhr-6 regulates oxidative stress resistance in worms and does not affect the feeding behavior of worms. These findings imply the potential of nhr-6 as a common therapeutic target for aging and cancer ailments, stressing the power of in silico PPI network analysis coupled with RNAi screens to describe gene function.
KW  - Computer modelling
KW  - Embryonic induction
KW  - RNAi
Y1  - 2019
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-202666
VL  - 9
ER  - 
TY  - THES
A1  - Akakpo, Martin Gameli
T1  - The influence of learner characteristics on interactions to seek and share information in e-learning: A media psychology perspective
T1  - Der Einfluss von Lernendenmerkmale auf die Interaktionen zur Suche und zum Austausch von Informationen im E-Learning: Eine medienpsychologische Perspektive
N2  - Research on the deployment and use of technology to assist learning has seen a significant
rise over the last decades (Aparicio et al., 2017). The focus on course quality, technology,
learning outcome and learner satisfaction in e-learning has led to insufficient attention by
researchers to individual characteristics of learners (Cidral et al., 2017 ; Hsu et al., 2013). The current work aims to bridge this gap by investigating characteristics identified by previous works and backed by theory as influential individual differences in e-learning. These learner characteristics have been suggested as motivational factors (Edmunds et al., 2012) in decisions by learners to interact and exchange information (Luo et al., 2017).
In this work e-learning is defined as interaction dependent information seeking and sharing enabled by technology. This is primarily approached from a media psychology perspective. The role of learner characteristics namely, beliefs about the source of knowledge (Schommer, 1990), learning styles (Felder & Silverman, 1988), need for affect (Maio & Esses, 2001), need for cognition (Cacioppo & Petty, 1982) and power distance (Hofstede, 1980) on interactions to seek and share information in e-learning are investigated. These investigations were shaped by theory and empirical lessons as briefly mentioned in the next paragraphs. Theoretical support for investigations is derived from the technology acceptance model(TAM) by psychologist Davis (1989) and the hyper-personal model by communication scientist Walther (1996). The TAM was used to describe the influence of learner characteristics on decisions to use e-learning systems (Stantchev et al., 2014). The hyper-personal model described why computer-mediated communication thrives in e-learning (Kaye et al., 2016) and how learners interpret messages exchanged online (Hansen et al., 2015). This theoretical framework was followed by empirical reviews which justified the use of interaction and information seeking-sharing as key components of e-learning as well as the selection of learner characteristics. The reviews provided suggestions for the measurement of variables (Kühl et al., 2014) and the investigation design (Dascalau et al., 2015). Investigations were designed and implemented through surveys and quasi experiments which were used for three preliminary studies and two main studies. Samples were selected from Germany and Ghana with same variables tested in both countries. Hypotheses were tested with interaction and information seeking-sharing as dependent variables while beliefs about the source of knowledge, learning styles, need for affect, need for cognition and power distance were independent variables. Firstly, using analyses of variance, the influence of beliefs about the source of knowledge on interaction choices of learners was supported. Secondly, the role of need for cognition on interaction choices of learners was supported by results from a logistic regression. Thirdly, results from multiple linear regressions backed the influence of need for cognition and power distance on information seeking-sharing behaviour of learners. Fourthly, the relationship between need for affect and need for cognition
was supported. The findings may have implications for media psychology research, theories used in this work, research on e-learning, measurement of learner characteristics and the design of e-learning platforms. The findings suggest that, the beliefs learners have about the source of knowledge, their need for cognition and their power distance can influence decisions to interact and seek or share information. The outlook from reviews and findings in this work predicts more research on learner characteristics and a corresponding intensity in the use of e-learning by individuals. It is suggested that future studies investigate the relationship between learner autonomy and power distance. Studies on inter-cultural similarities amongst e-learners in different populations are also
suggested.
N2  - Forschungsbemühungen zur Bereitstellung und die Nutzung von Technologien zur Unterstützung des Lernens nahm in den letzten Jahrzehnten erheblich zu (Aparicio et al., 2017). Der Fokus auf Kursqualität, Technologie, Lernergebnisse und Zufriedenheit der Lernenden im E-Learning führte dazu, dass die Forschenden den individuellen Eigenschaften der Lernenden nicht genügend Aufmerksamkeit schenkten (Cidral et al., 2017; Hsu et al., 2013). Die vorliegende Arbeit ist bestrebt, diese Lücke zu schließen. Sie untersucht Lernendenmerkmale, die in früheren Arbeiten identifiziert und theoretisch als einflussreiche individuelle Unterschiede beim E-Learning unterstrichen wurden. Diese Eigenschaften des Lernenden wurden als Motivationsfaktoren (Edmunds et al., 2012) in Entscheidungen des Lernenden bei Interaktion mit und zum Austausch von Informationen vorgeschlagen (Luo et al., 2017). 
In der vorliegenden Arbeit wird E-Learning definiert als Informationssuche und -austausch, der durch Technologie ermöglicht wird und auf Interaktionen basiert. Diese Ideen werden vor allem aus medienpsychologischer Sicht angegangen. Die Rolle der Merkmale des Lernenden, nämlich seine jeweiligen Überzeugungen über die Quelle des Wissens (Schommer, 1990), Lernstile (Felder & Silverman, 1988), Bedürfnis nach Zuwendung (Maio & Esses, 2001), Erkenntnisdrang (Cacioppo & Petty, 1982) und Machtdistanz (Hofstede, 1980) werden bzgl. der Interaktionen, die zur Suche und zum Austausch von Informationen dienen, untersucht. Diese Untersuchungen berücksichtigen theoretische Annahmen und empirische Erkenntnisse, die hier kurz skizziert werden.
Das ‚Technology Acceptance Model‘ (TAM) des Psychologen Davis (1989) und das ‚Hyper-Personal Model‘ des Kommunikationswissenschaftlers Walther (1996) liegen den durchgeführten Untersuchungen zugrunde. Mit dem TAM wurde der Einfluss der Eigenschaften eines Lernenden auf Entscheidungen zur Verwendung von E-Learning-Systemen erklärt (Stantchev et al., 2014). Das ‚Hyper-Personal Model‘ skizzierte Ursachen, warum computervermittelte Kommunikation im E-Learning gelingt (Kaye et al., 2016) und wie Lernende online ausgetauschte Nachrichten interpretieren (Hansen et al., 2015). Diesem theoretischen Rahmen folgend, werden empirische Arbeiten umrissen, die die Verwendung von Interaktion, zur Suche und zum Austausch von Informationen als Schlüsselkomponenten des E-Learning beschreiben sowie die Auswahl der zu untersuchenden Eigenschaften der Lernenden rechtfertigten. Aus diesen Arbeiten wurden Ideen für die Messung der Variablen (Kühl et al., 2014) und das Untersuchungsdesign (Dascalau et al., 2015) abgeleitet. Umfragen und Quasi-Experimente wurden hierzu durchgeführt. Diese Instrumente wurden für drei Vorstudien und zwei Hauptstudien verwendet. Probanden wurden aus Deutschland und Ghana ausgewählt, wobei in beiden Ländern die gleichen Variablen getestet wurden.
	Die Hypothesentestung berücksichtigte Interaktion und Informationssuche und -austausch als abhängige Variablen, während die Überzeugungen bzgl. der  Quellen des Wissens, Lernstile, Bedürfnis nach Zuwendung, Erkenntnisdrang und Machtdistanz als unabhängige Variablen dienten. Durchgeführte Varianzanalysen (1.) belegen die Annahme, dass Überzeugungen über die Wissensquelle Einfluss auf die Interaktionswahl der Lernenden haben. Zudem konnte ein Effekt (2.) des Erkenntnisdrangs auf die Wahlentscheidung der Lernenden durch die Ergebnisse einer logistischen Regression unterstützt werden. Des Weiteren (3.) unterstützten die Ergebnisse mehrerer linearer Regressionen den Einfluss des Erkenntnisdrangs und der Machtdistanz auf das Verhalten der Lernenden bezüglich Informationssuche und -austausch. Schließlich (4.) wurde die Wechselbeziehung zwischen Bedürfnis nach Zuwendung und Erkenntnisdrang unterstützt.
Die Ergebnisse sind relevant für die medienpsychologische Forschung, Theorien, die in dieser Arbeit verwendet werden, die Untersuchung von E-Learning, die Messung der Merkmale der Lernenden, sowie für die Gestaltung von E-Learning-Plattformen. Die Ergebnisse deuten darauf hin, dass die Überzeugungen der Lernenden über die Wissensquelle, ihr Erkenntnisdrang (NfC) und ihre Machtdistanz, die Entscheidungen, wie sie interagieren und Informationen suchen oder sie auszutauschen, beeinflussen können. Schlußfolgerungen aus der erarbeiteten Theorie und Empirie sowie aus dieser Arbeit befürworten eine stärkere Erforschung der Eigenschaften der Lernenden. Es erscheint darüber hinaus ratsam, dass zukünftige Studien den Zusammenhang zwischen der Autonomie der Lernenden und der Machtdistanz untersuchen. Es werden außerdem weitere Studien zu interkulturellen Ähnlichkeiten zwischen E-Learning-Lernenden in verschiedenen Bevölkerungsgruppen vorgeschlagen.
KW  - e-learning
KW  - Individualität
KW  - E-Learning
KW  - Media Psychology
KW  - Interactions
KW  - Information seeking and sharing
KW  - information sharing
KW  - learner characteristics
Y1  - 2019
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-185934
ER  - 
TY  - JOUR
A1  - Aistleitner, Karin
A1  - Heinz, Christian
A1  - Hoermann, Alexandra
A1  - Heinz, Eva
A1  - Montanaro, Jacqueline
A1  - Schulz, Frederik
A1  - Maier, Elke
A1  - Pichler, Peter
A1  - Benz, Roland
A1  - Horn, Matthias
T1  - Identification and Characterization of a Novel Porin Family Highlights a Major Difference in the Outer Membrane of Chlamydial Symbionts and Pathogens
JF  - PLoS ONE
N2  - The Chlamydiae constitute an evolutionary well separated group of intracellular bacteria comprising important pathogens of humans as well as symbionts of protozoa. The amoeba symbiont Protochlamydia amoebophila lacks a homologue of the most abundant outer membrane protein of the Chlamydiaceae, the major outer membrane protein MOMP, highlighting a major difference between environmental chlamydiae and their pathogenic counterparts. We recently identified a novel family of putative porins encoded in the genome of P. amoebophila by in silico analysis. Two of these Protochlamydia outer membrane proteins, PomS (pc1489) and PomT (pc1077), are highly abundant in outer membrane preparations of this organism. Here we show that all four members of this putative porin family are toxic when expressed in the heterologous host Escherichia coli. Immunofluorescence analysis using antibodies against heterologously expressed PomT and PomS purified directly from elementary bodies, respectively, demonstrated the location of both proteins in the outer membrane of P. amoebophila. The location of the most abundant protein PomS was further confirmed by immuno-transmission electron microscopy. We could show that pomS is transcribed, and the corresponding protein is present in the outer membrane throughout the complete developmental cycle, suggesting an essential role for P. amoebophila. Lipid bilayer measurements demonstrated that PomS functions as a porin with anion-selectivity and a pore size similar to the Chlamydiaceae MOMP. Taken together, our results suggest that PomS, possibly in concert with PomT and other members of this porin family, is the functional equivalent of MOMP in P. amoebophila. This work contributes to our understanding of the adaptations of symbiotic and pathogenic chlamydiae to their different eukaryotic hosts.
KW  - cell wall
KW  - protochlamydia amoebophila
KW  - escherichia coli
KW  - matrix protein porin
KW  - gram negative bacteria
KW  - single channel analysis
KW  - developmental cycle
KW  - mycobacterium smegmatis
KW  - monoclonal antibodies
KW  - signal peptides
Y1  - 2013
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-131176
VL  - 8
IS  - 1
ER  - 
TY  - JOUR
A1  - Aintablian, Arpa
A1  - Strozniak, Sandra
A1  - Heuer, Marion
A1  - Lutz, Manfred B.
T1  - M-MDSC in vitro generation from mouse bone marrow with IL-3 reveals high expression and functional activity of arginase 1
JF  - Frontiers in Immunology
N2  - Myeloid-derived suppressor cells (MDSC) represent major regulators of immune responses, which can control T cells via their inducible nitric oxide synthase (iNOS)- and arginase 1 (Arg1)-mediated effector functions. While GM-CSF is well documented to promote MDSC development, little is known about this potential of IL-3, an established growth factor for mast cells. Here, we show that IL-3, similar to GM-CSF, generates monocytic MDSC (M-MDSC) from murine bone marrow (BM) cells after 3 days of in vitro culture. At this time point, predominantly CD11b+ CD49a+ monocytic and CD11b+ CD49a- FcεR I- neutrophilic cells were detectable, while CD11blow/neg FcεR I+ mast cells accumulated only after extended culture periods. Both growth factors were equivalent in generating M-MDSC with respect to phenotype, cell yield and typical surface markers. However, IL-3 generated M-MDSC produced less TNF, IL-1β and IL-10 after activation with LPS + IFN-γ but showed higher Arg1 expression compared to GM-CSF generated M-MDSC. Arg1 was further induced together with iNOS after MDSC activation. Accordingly, an increased Arg1-dependent suppressor activity by the IL-3 generated M-MDSC was observed using respective iNOS and Arg1 inhibitors. Together, these data indicate that M-MDSC can be generated in vitro by IL-3, similar to GM-CSF, but with increased Arg1 expression and Arg1-mediated suppression capacity. This protocol now allows further in vitro studies on the role of IL-3 for MDSC biology.
KW  - myeloid-derived suppressor cells (MDSC)
KW  - bone marrow
KW  - IL-3
KW  - GM-CSF
KW  - in vitro culture
KW  - protocol
Y1  - 2023
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-317769
VL  - 14
ER  - 
TY  - THES
A1  - Aigner, Max
T1  - Establishing successful protocols and imaging pipelines for Expansion Microscopy in murine blood platelets
T1  - Etablierung erfolgreicher Protokolle zur Probenpräparation und Bildgebung für die ‚Expansion Microscopy‘ in murinen Thrombozyten
N2  - Platelets play an important role in the body, since they are part of the hemostasis
system, preventing and stopping blood loss. Nevertheless, when platelet or
coagulation system function are impaired, uncontrolled bleedings but also irreversible
vessel occlusion followed by ischemic tissue damage can occur. Therefore,
understanding platelet function and activation, mechanisms which are controlled by a
variety of platelet membrane receptors and other factors is important to advance out
knowledge of hemostasis and platelet malfunction. For a complete picture of platelet
function and their modulating behavior it is desired to be able to quantify receptor
distributions and interactions of these densely packed molecular ensembles in the
membrane. This challenges scientists for several reasons. Most importantly, platelets
are microscopically small objects, challenging the spatial resolution of conventional
light microscopy. Moreover, platelet receptors are highly abundant on the membrane
so even super-resolution microscopy struggles with quantitative receptor imaging on
platelets.
With Expansion microscopy (ExM), a new super-resolution technique was introduced,
allowing resolutions to achieve super-resolution without using a super-resolution
microscope, but by combining a conventional confocal microscopy with a highly
processed sample that has been expanded physically. In this doctoral thesis, I
evaluated the potential of this technique for super-resolution platelet imaging by
optimizing the sample preparation process and establishing an imaging and image
processing pipeline for dual-color 3D images of different membrane receptors. The
analysis of receptor colocalization using ExM demonstrated a clear superiority
compared to conventional microscopy. Furthermore, I identified a library of
fluorescently labeled antibodies against different platelet receptors compatible with
ExM and showed the possibility of staining membrane receptors and parts of the
cytoskeleton at the same time.
N2  - Thrombozyten spielen eine wichtige Rolle im Körper, denn als Teil des
Gerinnungssystems, sind sie daran beteiligt Blutverlust vorzubeugen und zu stoppen.
Gleichwohl können sie bei Störungen des Gerinnungssystems zu unkontrollierbaren
Blutungen und auch durch Aggregation zu kardiovaskulären Ereignissen, wie
Herzinfarkt und Schlaganfällen führen. Für ein besseres Verständnis von Hämostase
und Gerinnungsstörungen ist es deshalb nötig die Funktion und Aktivierung von
Thrombozyten zu verstehen, welche durch eine Vielzahl von Membranrezeptoren und
anderen Faktoren gesteuert wird. Eine Methode, um weitere Einblicke in diese
Prozesse zu bekommen ist die mikroskopische Darstellung von Rezeptorverteilungen
auf der Zellmembran und deren Interaktionen. Dies zu realisieren ist aus
verschiedenen Gründen anspruchsvoll. Der mikroskopisch kleine Durchmesser der
Thrombozyten macht es konventioneller Lichtmikroskopie schwer, einzelne
Rezeptoren auf der Membran darzustellen. Außerdem befinden sich sehr viele
Rezeptoren dicht gepackt auf der Membran, sodass sogar superhochauflösende
Mikroskope Schwierigkeiten haben, die Rezeptoren quantitativ zu beurteilen.
Mit ‚Expansion microscopy‘ (ExM) wurde eine relativ junge superhochaufösende
Technik auf Thrombozyten angewendet. Diese Technik erreicht Auflösungen
vergleichbar mit sogenannten ‚super-resolution‘ Mikroskopen, ohne die Benutzung
selbiger, sondern durch die Kombination von konfokaler Mikroskopie mit einer
physikalisch expandierten Probe. In dieser Arbeit evaluierte ich das Potential dieser
Technik für superhochauflösende Bilder von Thrombozytenrezeptoren und optimierte
die Probenvorbereitung, sodass zweifarbige 3D Bilder von verschiedenen
Membranrezeptoren möglich waren. Die Ergebnisse der Kolokationsanalyse zeigten
einen deutlich vergrößerten Dynamikumfang durch ExM. Außerdem katalogisierte ich
fluoreszenzmarkierte Antikörper gegen verschiedene Thrombozyten Rezeptoren
bezüglich ihrer Tauglichkeit mit ExM und zeigte, dass es möglich ist
Membranrezeptoren und Bestandteile des Zytoskeletts gleichzeitig zu färben.
KW  - Expansion Microscopy
KW  - platelets
KW  - Mikroskopie
KW  - Microscopy
Y1  - 2023
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-309003
ER  - 
TY  - JOUR
A1  - Aido, Ahmed
A1  - Zaitseva, Olena
A1  - Wajant, Harald
A1  - Buzgo, Matej
A1  - Simaite, Aiva
T1  - Anti-Fn14 antibody-conjugated nanoparticles display membrane TWEAK-like agonism
JF  - Pharmaceutics
N2  - Conventional bivalent IgG antibodies targeting a subgroup of receptors of the TNF superfamily (TNFSF) including fibroblast growth factor-inducible 14 (anti-Fn14) typically display no or only very limited agonistic activity on their own and can only trigger receptor signaling by crosslinking or when bound to Fcγ receptors (FcγR). Both result in proximity of multiple antibody-bound TNFRSF receptor (TNFR) molecules, which enables engagement of TNFR-associated signaling pathways. Here, we have linked anti-Fn14 antibodies to gold nanoparticles to mimic the “activating” effect of plasma membrane-presented FcγR-anchored anti-Fn14 antibodies. We functionalized gold nanoparticles with poly-ethylene glycol (PEG) linkers and then coupled antibodies to the PEG surface of the nanoparticles. We found that Fn14 binding of the anti-Fn14 antibodies PDL192 and 5B6 is preserved upon attachment to the nanoparticles. More importantly, the gold nanoparticle-presented anti-Fn14 antibody molecules displayed strong agonistic activity. Our results suggest that conjugation of monoclonal anti-TNFR antibodies to gold nanoparticles can be exploited to uncover their latent agonism, e.g., for immunotherapeutic applications.
KW  - Fn14
KW  - nanoparticles
KW  - surface modification
KW  - drug-delivery
KW  - anti-TNFRSF receptor (TNFR) antibodies
Y1  - 2021
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-242710
SN  - 1999-4923
VL  - 13
IS  - 7
ER  - 
TY  - THES
A1  - Aido, Ahmed
T1  - Development of anti-TNF antibody-gold nanoparticles (anti-TNF-AuNPs)
T1  - Entwicklung von Anti-TNF-Antikörper-Gold-Nanopartikeln
N2  - Gold nanoparticles of diameter ca. 60 nm have been synthesized based on Turkevich and Frens protocols. We have demonstrated that the carboxyl-modified gold nanoparticles can be coupled covalently with antibodies (Ab) of interest using the EDC/NHS coupling procedure. Binding studies with Ab-grafted AuNPs and GpL fusion proteins proved that conjugation of AuNPs with antibodies enables immobilization of antibodies with preservation of a significant antigen binding capacity. More importantly, our findings showed that the conjugation of types of anti-TNF receptors antibodies such as anti-Fn14 antibodies (PDL192 and 5B6) (Aido et al., 2021), anti-CD40, anti-4-1BB and anti-TNFR2 with gold nanoparticles confers them with potent agonism. Thus, our results suggest that AuNPs can be utilized as a platform to immobilize anti-TNFR antibodies which, on the one hand, helps to enhance their agonistic activity in comparison to “free” inactive antibodies by mimicking the effect of cell-anchored antibodies or membrane-bound TNF ligands and, on the other hand, allows to develop new generations of drug delivery systems. These constructs are characterized with their biocompatibility and their tunable synthesis process.
In a further work part, we combined the benefits of the established system of Ab-AuNPs with materials used widely in the modern biofabrication approaches such as the photo-crosslinked hydrogels, methacrylate-modified gelatin (GelMA), combined with embedded variants of human cell lines. The acquired results demonstrated clearly that the attaching of proteins like antibodies to gold nanoparticles might reduce their release rate from the crosslinked hydrogels upon the very low diffusion of gold nanoparticles from the solid constructs to the surrounding medium yielding long-term local functioning proteins-attached particles. Moreover, our finding suggests that hydrogel-embedded AuNP-immobilized antibodies, e.g. anti-TNFα-AuNPs or anti-IL1-AuNPs enable local inhibitory functions,
To sum up, our results demonstrate that AuNPs can act as a platform to attach anti-TNFR antibodies to enhance their agonistic activity by resembling the output of cell-anchoring or membrane bounding. Gold nanoparticles are considered, thus, as promising tool to develop the next generation of drug delivery systems, which may contribute to cancer therapy. On top of that, the embedding of anti-inflammatory-AuNPs in the biofabricated hydrogel presents new innovative strategy of the treatment of autoinflammatory diseases.
N2  - Gold-Nanopartikel mit einem Durchmesser von ca. 60 nm wurden auf Basis der Turkevich- und Frens-Protokolle synthetisiert. Bindungsstudien mit Ab-verankerten AuNPs und GpL-Fusionsproteinen haben gezeigt, dass die Konjugation von AuNPs mit Antikörpern die Immobilisierung von Antikörpern mit Erhaltung einer signifikanten Antigenbindungs-Kapazität ermöglicht. Noch wichtiger ist, dass unsere Ergebnisse zeigen, dass die Konjugation von Typen von Antikörpern gegen TNFRs wie anti-Fn14-Antikörper (PDL192 und 5B6), anti-CD40, anti-4-1BB und anti-TNFR2 mit Gold-Nanopartikeln ihnen eine starke agonistische Wirkung verleiht. Unsere Ergebnisse legen nahe, dass AuNPs als Plattform genutzt werden können, um Antikörper gegen TNFR zu immobilisieren, was einerseits dazu beiträgt, ihre agonistische Aktivität im Vergleich zu "freien" inaktiven Antikörpern zu erhöhen, indem sie die Wirkung von zellgebundenen Antikörpern oder membranverankerten TNF-Liganden nachahmen und andererseits die Entwicklung neuer Generationen von Wirkstoffabgabe Systemen ermöglicht. Diese Konstrukte zeichnen sich durch ihre Biokompatibilität und ihren einstellbaren Syntheseprozess aus.
In einem weiteren Teil der Arbeit haben wir die Vorteile des etablierten Systems von Ab-AuNPs mit Materialien kombiniert, die in modernen Biofabrikationsansätzen weit verbreitet sind, nämlich Hydrogele, z.b. methacrylatmodifiziertes Gelatine (GelMA), kombiniert mit eingebetteten Varianten von menschlichen Zelllinien. Die erzielten Ergebnisse zeigten deutlich, dass die Anbindung von Proteinen wie Antikörpern an Gold-Nanopartikel ihre Freisetzung aus den vernetzten Hydrogelen reduzieren könnte, da die Diffusion von Gold-Nanopartikeln aus den festen Konstrukten in das umgebende Medium sehr gering ist und so langfristig Konstrukte mit lokalem Proteine load - erzeugt werden können. Darüber hinaus legt unser Befund nahe, dass in das Hydrogel eingebettete AuNP-immobilisierte Antikörper wie Anti-TNFα-AuNPs oder Anti-IL1-AuNPs eine lokal Immunsuppression erlauben. Diese können als vielversprechende Ansätze betrachtet werden, um verschiedene Arten von Autoimmunerkrankungen zu behandeln.
Zusammenfassend zeigen unsere Ergebnisse, dass AuNPs als Plattform dienen können, um Anti-TNFR-Antikörper anzubinden und ihre agonistische Aktivität zu erhöhen. Goldnanopartikel werden daher als vielversprechendes Werkzeug zur Entwicklung der nächsten Generation von Wirkstofftransportsystemen angesehen, die zur Krebstherapie beitragen können. Darüber hinaus stellt die Einbettung von entzündungshemmenden-AuNPs in das biofabrizierte Hydrogel eine neue innovative Strategie für die Behandlung von autoinflammatorischen Erkrankungen dar.
KW  - AuNPs
KW  - TNF
KW  - Nanoparticles
KW  - Antibody
KW  - Gold Nanoparticles
KW  - Drug delivery system (DDS)
KW  - Nanopartikel
Y1  - 2024
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-349212
ER  - 
TY  - JOUR
A1  - Aich, Valentin
A1  - Akhundzadah, Noor Ahmad
A1  - Knuerr, Alec
A1  - Khoshbeen, Ahmad Jamshed
A1  - Hattermann, Fred
A1  - Paeth, Heiko
A1  - Scanlon, Andrew
A1  - Paton, Eva Nora
T1  - Climate change in Afghanistan deduced from reanalysis and coordinated regional climate downscaling experiment (CORDEX)—South Asia Simulations
JF  - Climate
N2  - Past and the projected future climate change in Afghanistan has been analyzed systematically and differentiated with respect to its different climate regions to gain some first quantitative insights into Afghanistan’s vulnerability to ongoing and future climate changes. For this purpose, temperature, precipitation and five additional climate indices for extremes and agriculture assessments (heavy precipitation; spring precipitation; growing season length (GSL), the Heat Wave Magnitude Index (HWMI); and the Standardized Precipitation Evapotranspiration Index (SPEI)) from the reanalysis data were examined for their consistency to identify changes in the past (data since 1950). For future changes (up to the year 2100), the same parameters were extracted from an ensemble of 12 downscaled regional climate models (RCM) of the Coordinated Regional Climate Downscaling Experiment (CORDEX)-South Asia simulations for low and high emission scenarios (Representative Concentration Pathways 4.5 and 8.5). In the past, the climatic changes were mainly characterized by a mean temperature increase above global level of 1.8 °C from 1950 to 2010; uncertainty with regard to reanalyzed rainfall data limited a thorough analysis of past changes. Climate models projected the temperature trend to accelerate in the future, depending strongly on the global carbon emissions (2006–2050 Representative Concentration Pathways 4.5/8.5: 1.7/2.3 °C; 2006–2099: 2.7/6.4 °C, respectively). Despite the high uncertainty with regard to precipitation projections, it became apparent that the increasing evapotranspiration is likely to exacerbate Afghanistan’s already existing water stress, including a very strong increase of frequency and magnitude of heat waves. Overall, the results show that in addition to the already extensive deficiency in adaptation to current climate conditions, the situation will be aggravated in the future, particularly in regard to water management and agriculture. Thus, the results of this study underline the importance of adequate adaptation to climate change in Afghanistan. This is even truer taking into account that GSL is projected to increase substantially by around 20 days on average until 2050, which might open the opportunity for extended agricultural husbandry or even additional harvests when water resources are properly managed.
KW  - climate change
KW  - Afghanistan
KW  - Coordinated Regional Climate Downscaling Experiment (CORDEX)-South Asia
KW  - trend analysis
KW  - Heat Wave Magnitude Index (HWMI)
KW  - Standardized Precipitation Evapotranspiration Index (SPEI)
KW  - growing season length (GSL)
Y1  - 2017
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-198024
SN  - 2225-1154
VL  - 5
IS  - 2
ER  - 
TY  - THES
A1  - Ahrens, Lea Marlen
T1  - The Role of Attentional Control and Fear Acquisition and Generalization in Social Anxiety Disorder
T1  - Die Rolle von Aufmerksamkeitskontrolle und Furchtlernen und Generalisierung bei Sozialer Angststörung
N2  - Although Social Anxiety Disorder (SAD) is one of the most prevalent mental disorders, still little is known about its development and maintenance. Cognitive models assume that deviations in attentional as well as associative learning processes play a role in the etiology of SAD. Amongst others, deficits in inhibitory attentional control as well as aberrations during fear generalization, which have already been observed in other anxiety disorders, are two candidate mechanisms that might contribute to the onset and retention of SAD. However, a review of the literature shows that there is a lack of research relating to these topics. Thus, the aim of the present thesis was to examine in which way individuals with SAD differ from healthy controls regarding attentional control and generalization of acquired fear during the processing of social stimuli.
Study 1 tested whether impairment in the inhibitory control of attention is a feature of SAD, and how it might be influenced by emotional expression and gaze direction of an interactional partner. For this purpose, individuals with SAD and healthy controls (HC) participated in an antisaccade task with faces displaying different emotional expressions (angry, neutral and happy) and gaze directions (direct and averted) serving as target stimuli. While the participants performed either pro- or antisaccades in response to the peripherally presented faces, their gaze behavior was recorded via eye-tracking, and ratings of valence and arousal were obtained. Results revealed that both groups showed prolonged latencies and increased error rates in trials with correct anti- compared to prosaccades. However, there were no differences between groups with regard to response latency or error rates, indicating that SAD patients did not exhibit impairment on inhibitory attentional control in comparison to HC during eye-tracking. Possible explanations for this finding could be that reduced inhibitory attentional control in SAD only occurs under certain circumstances, for example, when these individuals currently run the risk of being negatively evaluated by others and not in the mere presence of phobic stimuli, or when the cognitive load of a task is so high that it cannot be unwound by compensatory strategies, such as putting more effort into a task. 
As not only deviations in attentional, but also associative learning processes might be pathogenic markers of SAD, these mechanisms were further addressed in the following experiments. Study 2 is the first that attempted to investigate the generalization of conditioned fear in patients with SAD. To this end, patients with SAD and HC were conditioned to two neutral female faces serving as conditioned stimuli (CS+: reinforced; CS-: non-reinforced) and a fearful face paired with a loud scream serving as unconditioned stimulus (US). Fear generalization was tested by presenting morphs of the two faces (GS: generalization stimuli), which varied in their similarity to the original faces. During the whole experiment, self-report ratings, heart rate (HR) and skin conductance responses (SCR) were recorded. Results demonstrated that SAD patients rated all stimuli as less pleasant and more arousing, and overestimated the occurrence of the US compared to HC, indicating a general hyperarousal in individuals with SAD. In addition, ratings and SCR indicated that both groups generalized their acquired fear from the CS+ to intermediate GSs as a function of their similarity to the CS+. However, except for the HR data, which indicated that only SAD patients but not HC displayed a generalization response in this measure, most of the results did not support the hypothesis that SAD is characterized by overgeneralization. A plausible reason for this finding could be that overgeneralization is just a key characteristic of some anxiety disorders and SAD is not one of them. Still, other factors, such as comorbidities in the individuals with SAD, could also have had an influence on the results, which is why overgeneralization was further examined in study 3.
The aim of study 3 was to investigate fear generalization on a neuronal level. Hence, high (HSA) and low socially anxious participants (LSA) underwent a conditioning paradigm, which was an adaption of the experimental design used study 2 for EEG. During the experiment, steady-state visually evoked potentials (ssVEPs) and ratings of valence and arousal were recorded. Analyses revealed significant generalization gradients in all ratings with highest fear responses to the CS+ and a progressive decline of these reactions with increasing similarity to the CS-. In contrast, the generalization gradient on a neuronal level showed highest amplitudes for the CS+ and a reduction in amplitude to the most proximal, but not distal GSs in the ssVEP signal, which might be interpreted as lateral inhibition in the visual cortex. The observed dissociation among explicit and implicit measures points to different functions of behavioral and sensory cortical processes during fear generalization: While the ratings might reflect an individual’s consciously increased readiness to react to threat, the lateral inhibition pattern in the occipital cortex might serve to maximize the contrast among stimuli with and without affective value and thereby improve adaptive behavior. As no group differences could be observed, the finding of study 2 that overgeneralization does not seem to be a marker of SAD is further consolidated. 
In sum, the conducted experiments suggest that individuals with SAD are characterized by a general hyperarousal during the exposition to disorder-relevant stimuli as indicated by enhanced arousal and reduced valence ratings of the stimuli compared to HC. However, the hypotheses that reduced inhibitory attentional control and overgeneralization of conditioned fear are markers of SAD were mostly not confirmed. Further research is required to elucidate whether they only occur under certain circumstances, such as high cognitive load (e.g. handling two tasks simultaneously) or social stress (e.g. before giving a speech), or whether they are not characteristics of SAD at all. With the help of these findings, new interventions for the treatment of SAD can be developed, such as attentional bias modification or discrimination learning.
N2  - Obwohl die Soziale Angststörung (SAS) eine der häufigsten psychischen Erkrankungen ist, ist über ihre Entstehung und Aufrechterhaltung noch wenig bekannt. Kognitive Modelle nehmen an, dass Abweichungen sowohl in Aufmerksamkeits- als auch assoziativen Lernprozessen eine Rolle bei ihrer Entwicklung spielen. Unter anderem werden Defizite in der Aufmerksamkeitskontrolle sowie Abweichungen während der Generalisierung von konditionierter Furcht als für die Ätiologie potentiell bedeutsame Faktoren gehandelt, da diese Auffälligkeiten bereits bei anderen Angststörungen beobachtet wurden.  Eine Literaturübersicht zeigt jedoch, dass zu dieser Thematik ein Mangel an Forschung besteht. Das Ziel der vorliegenden Doktorarbeit war es daher zu untersuchen, auf welche Weise sich Individuen mit Sozialer Angststörung bei der Verarbeitung sozialer Stimuli von gesunden Kontrollprobanden in Hinblick auf ihre Aufmerksamkeitskontrolle und die Generalisierung gelernter Furchtreaktionen unterscheiden.
Studie 1 testete, ob das Vorliegen einer Beeinträchtigung der inhibitorischen Aufmerksamkeitskontrolle ein Merkmal der SAS ist, und auf welche Weise diese vom emotionalen Gesichtsausdruck sowie der Blickrichtung von Interaktionspartnern beeinflusst werden kann. Zu diesem Zweck nahmen Patienten mit SAS und eine gesunde Kontrollgruppe (KG) an einer Antisakkaden-Aufgabe teil, bei welcher Gesichter mit unterschiedlichem emotionalen Ausdruck (wütend, neutral und fröhlich) und unterschiedlicher Blickrichtung (direkter und abgewandter Blick) als Stimuli dienten. Während die Probanden in Abhängigkeit eines Hinweisreizes entweder Pro- oder Antisakkaden in Reaktion auf die peripher präsentierten Gesichter ausübten, wurde ihr Blickverhalten mittels Eye-Tracking aufgezeichnet. Außerdem wurden anschließend Valenz- und Arousal-Ratings der Stimuli erfasst. Die Ergebnisse zeigten, dass beide Gruppen erhöhte Latenzzeiten sowie Fehlerraten in Durchgängen mit korrekt ausgeführten Antisakkaden im Vergleich zu Prosakkaden aufwiesen. Jedoch gab es keinen Gruppenunterschied in Bezug auf die Antwortlatenz und Fehlerrate, was darauf hindeutet, dass Patienten mit SAS im Vergleich zur KG kein Defizit der inhibitorischen Aufmerksamkeitskontrolle während des Eye-Trackings erkennen ließen. Eine mögliche Ursache für diesen Befund könnte sein, dass eine reduzierte inhibitorische Aufmerksamkeitskontrolle bei SAS nur unter bestimmten Umständen auftritt, beispielsweise, wenn betroffene Individuen akut Gefahr laufen von anderen negativ bewertet zu werden, und nicht bloß phobischen Stimuli ausgesetzt sind, oder wenn die kognitive Belastung durch eine Aufgabe so groß ist, dass sie nicht durch kompensatorische Strategien, wie beispielsweise mehr Anstrengung, ausgeglichen werden kann. 
Da nicht nur abweichende Aufmerksamkeitsprozesse, sondern auch abweichende assoziative Lernprozesse pathogene Marker von SAS sein könnten, wurden letztere in den folgenden Experimenten genauer untersucht. Studie 2 stellt den ersten Versuch dar die Generalisierung konditionierter Furcht in Patienten mit SAS zu erforschen. Hierfür wurden sowohl SAS Patienten als auch eine KG auf zwei neutrale, weibliche Gesichter konditioniert, welche als Konditionierungsstimuli (conditioned stimuli [CS]: CS+: verstärkt; CS-: unverstärkt) dienten. Bei dem unkonditionierten Stimulus (unconditioned stimulus [US]) handelte es sich um die bereits bekannten Gesichter mit ängstlichem Ausdruck, die mit einem lauten Schrei gepaart wurden. Die Furchtgeneralisierung wurde mittels der Präsentation von Gesichtern, welche aus den beiden Ursprungsgesichtern gemorpht worden waren und als Generalisierungsstimuli (generalization stimuli [GS]) dienten, getestet. Während des Experiments wurden Selbstauskunftsratings sowie Herzrate (heart rate [HR]) und Hautleitfähigkeit (skin conductance response [SCR]) aufgezeichnet. Die Ergebnisse zeigten, dass Patienten mit SAS im Vergleich zur KG alle Stimuli als unangenehmer und aufregender bewerteten sowie die Auftretenswahrscheinlichkeit des US überschätzten, was auf eine generelle Übererregung in Individuen mit SAS hinweist. Darüber hinaus ergaben die Ergebnisse, dass beide Gruppen ihre erworbene Furcht vom CS+ in Abhängigkeit ihrer Ähnlichkeit mit dem CS+ auf intermediäre GSs übertrugen. Allerdings stützen abgesehen von den Daten der Herzrate, in denen nur SAS Patienten und nicht die KG eine Generalisierungsreaktion zeigten, die meisten Befunde nicht die Hypothese, dass Übergeneralisierung ein Merkmal von SAS ist. Eine mögliche Ursache dieses Ergebnisses könnte sein, dass Übergeneralisierung nur ein wichtiges Merkmal einiger bestimmter Angststörungen ist und SAS nicht zu ihnen gehört. Dennoch könnten auch andere Faktoren, wie beispielsweise die Komorbiditäten der untersuchten SAS Patienten, einen Einfluss auf die Ergebnisse gehabt haben. Aus diesem Grund wurde Übergeneralisierung in Studie 3 näher untersucht. 
Das Ziel von Studie 3 war es Furchtgeneralisierung auf neuronaler Ebene zu untersuchen. Folglich wurde das Paradigma der zweiten Studie an einen Versuchsplan, der für die Messung von neuronaler Aktivität mittels EEG geeignet war, angepasst und auf eine hoch (high socially anxious [HSA])- sowie eine niedrig sozialängstliche Gruppe (low socially anxious [LSA]) angewandt. Während des Experiments wurden sowohl steady-state visually evoked potentials (ssVEPs) als auch Valenz- und Arousal-Ratings erfasst. Die Analyse ergab signifikante Generalisierungsgradienten in allen Ratings mit der höchsten Furchtreaktion auf den CS+ und einem fortschreitenden Abfall der Reaktion auf die GSs mit zunehmender Ähnlichkeit zum CS-. Im Gegensatz dazu zeigte sich in der ssVEP-Amplitude ein anderes Muster: hier erreichte der Generalisierungsgradient zwar auch die höchste Amplitude in Reaktion auf den CS+, jedoch eine anschließende Reduktion der Amplitude auf den nächst proximalen, nicht jedoch distale GS, was ein Hinweis auf laterale Hemmungsprozesse im visuellen Kortex sein könnte. Die beobachtete Dissoziation zwischen expliziten und impliziten Maßen könnte auf unterschiedliche Funktionen von behavioralen und sensorischen kortikalen Prozessen während der Generalisierung von Furcht hinweisen: Während die Ratings möglicherweise die bewusste Bereitschaft eines Individuums auf Bedrohung zu reagieren widerspiegeln, könnte das Muster lateraler Hemmung im okzipitalen Kortex dazu dienen den Kontrast zwischen Stimuli mit und ohne affektivem Wert zu maximieren und somit adaptives Verhalten verbessern. Da zwischen beiden Gruppen keine signifikanten Unterschiede gefunden wurden, untermauerte Studie 3 das Ergebnis von Studie 2, welches bereits eher dagegen sprach, dass Übergeneralisierung von Furcht ein Merkmal von Individuen mit SAS sei. 
Insgesamt suggerieren die Ergebnisse der durchgeführten Studien, dass Individuen mit SAS während der Exposition von störungsspezifischen Reizen im Vergleich zu Kontrollprobanden durch eine generelle Übererregung gekennzeichnet sind, was an erhöhten Arousal- und verringerten Valenz-Ratings erkennbar war. Jedoch konnten die Hypothesen, dass reduzierte Aufmerksamkeitskontrolle sowie Übergeneralisierung Merkmale von Individuen mit SAS sind, zum größten Teil nicht bestätigt werden. Weitere Forschung ist nötig um herauszufinden, ob diese Phänomene nur unter besonderen äußeren Umständen, wie beispielsweise hohen kognitiven Anforderungen (e.g. bei der Bearbeitung zweier Aufgaben gleichzeitig) oder sozialem Stress (e.g. vor dem Halten einer Rede), auftreten, oder ob sie gar kein Merkmal von SAS darstellen. Mit Hilfe der sich daraus ergebenden Befunde könnten neue Interventionen für die Behandlung von SAS entwickelt werden, wie beispielsweise Aufmerksamkeitsbias-Modifikations-Trainings oder Diskriminationslernen.
KW  - Sozialangst
KW  - Aufmerksamkeit
KW  - social anxiety
KW  - fear generalization
KW  - visual attention
KW  - Psychologie
KW  - Visuelle Aufmerksamkeit
KW  - Aversive Konditionierung
Y1  - 2020
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-171622
ER  - 
TY  - JOUR
A1  - Ahmed, Zeeshan
A1  - Zeeshan, Saman
A1  - Huber, Claudia
A1  - Hensel, Michael
A1  - Schomburg, Dietmar
A1  - Münch, Richard
A1  - Eylert, Eva
A1  - Eisenreich, Wolfgang
A1  - Dandekar, Thomas
T1  - ‘Isotopo’ a database application for facile analysis and management of mass isotopomer data
JF  - Database
N2  - The composition of stable-isotope labelled isotopologues/isotopomers in metabolic products can be measured by mass spectrometry and supports the analysis of pathways and fluxes. As a prerequisite, the original mass spectra have to be processed, managed and stored to rapidly calculate, analyse and compare isotopomer enrichments to study, for instance, bacterial metabolism in infection. For such applications, we provide here the database application ‘Isotopo’. This software package includes (i) a database to store and process isotopomer data, (ii) a parser to upload and translate different data formats for such data and (iii) an improved application to process and convert signal intensities from mass spectra of \(^{13}C\)-labelled metabolites such as tertbutyldimethylsilyl-derivatives of amino acids. Relative mass intensities and isotopomer distributions are calculated applying a partial least square method with iterative refinement for high precision data. The data output includes formats such as graphs for overall enrichments in amino acids. The package is user-friendly for easy and robust data management of multiple experiments.
KW  - stable-isotope
Y1  - 2014
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-120102
VL  - 2014
IS  - bau077
ER  - 
TY  - JOUR
A1  - Ahmed, Zeeshan
A1  - Zeeshan, Saman
A1  - Dandekar, Thomas
T1  - Mining biomedical images towards valuable information retrieval in biomedical and life sciences
JF  - Database - The Journal of Biological Databases and Curation
N2  - Biomedical images are helpful sources for the scientists and practitioners in drawing significant hypotheses, exemplifying approaches and describing experimental results in published biomedical literature. In last decades, there has been an enormous increase in the amount of heterogeneous biomedical image production and publication, which results in a need for bioimaging platforms for feature extraction and analysis of text and content in biomedical images to take advantage in implementing effective information retrieval systems. In this review, we summarize technologies related to data mining of figures. We describe and compare the potential of different approaches in terms of their developmental aspects, used methodologies, produced results, achieved accuracies and limitations. Our comparative conclusions include current challenges for bioimaging software with selective image mining, embedded text extraction and processing of complex natural language queries.
KW  - humans
KW  - software
KW  - image processing
KW  - animals
KW  - computer-assisted
KW  - data mining/methods
KW  - natural language processing
Y1  - 2016
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-162697
VL  - 2016
ER  - 
TY  - JOUR
A1  - Ahmed, Bilal
A1  - Ojha, Animesh K.
A1  - Hirsch, Florian
A1  - Fischer, Ingo
A1  - Patrice, Donfack
A1  - Materny, Arnulf
T1  - Tailoring of enhanced interfacial polarization in WO\(_3\) nanorods grown over reduced graphene oxide synthesized by a one-step hydrothermal method
JF  - RSC Advances
N2  - In the present report, well-defined WO3 nanorods (NRs) and a rGO–WO\(_3\) composite were successfully synthesized using a one-pot hydrothermal method. The crystal phase, structural morphology, shape, and size of the as-synthesized samples were studied using X-ray diffraction (XRD) and transmission electron microscopy (TEM) measurements. The optical properties of the synthesized samples were investigated by Raman, ultraviolet-visible (UV-Vis) and photoluminescence (PL) spectroscopy. Raman spectroscopy and TEM results validate the formation of WO\(_3\) (NRs) on the rGO sheet. The value of the dielectric constant (ε′) of WO3 NRs and rGO–WO\(_3\) composite is decreased with an increase in frequency. At low frequency (2.5 to 3.5 Hz), the value of ε′ for the rGO–WO3 composite is greater than that of pure WO\(_3\) NRs. This could be due to the fact that the induced charges follow the ac signal. However, at higher frequency (3.4 to 6.0), the value of ε′ for the rGO–WO\(_3\) composite is less compared to that of the pure WO3 NRs. The overall decrease in the value of ε′ could be due to the occurrence of a polarization process at the interface of the rGO sheet and WO3 NRs. Enhanced interfacial polarization in the rGO–WO\(_3\) composite is observed, which may be attributed to the presence of polar functional groups on the rGO sheet. These functional groups trap charge carriers at the interface, resulting in an enhancement of the interfacial polarization. The value of the dielectric modulus is also calculated to further confirm this enhancement. The values of the ac conductivity of the WO\(_3\) NRs and rGO–WO\(_3\) composite were calculated as a function of the frequency. The greater value of the ac conductivity in the rGO–WO\(_3\) composite compared to that of the WO\(_3\) NRs confirms the restoration of the sp:\(^{++}\) network during the in situ synthesis of the rGO–WO\(_3\) composite, which is well supported by the results obtained by Raman spectroscopy.
KW  - chemistry
Y1  - 2017
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-181829
VL  - 7
IS  - 23
ER  - 
TY  - THES
A1  - Ahmed, Arabe
T1  - Assessing particle deposition in a representative in vitro model of the rat respiratory tract
T1  - Entwicklung eines in vitro Modells (IVR) der Rattenlunge für die Untersuchung der Deposition von Wirkstoffpartikeln in den Atemwegen der Ratte
N2  - The aim of this thesis was to develop an in vitro model (IVR) of the rat lung for the purpose of investigating the deposition of drug particles in the rat airways. The model attempted to account for the affect of drug product characteristics and physiological parameters on deposition in the lungs. In addition, the model outputs were compared with in vivo lung deposition results from live rats and in silico predictions using published computer model of lung deposition in pre-clinical species.  

Initial work focussed on developing an aerosol exposure system capable of dosing small rodent to a range of airborne test materials. The system consists of two main parts; a fluidised bed aerosol generator and connection of the generator output to a nose only exposure chamber capable of accommodating 12 small animals in a single layer. In addition, an aerodynamic particle spectrometer (APS) was installed for continuously measuring the size distribution and airborne concentration of aerosol particles generated in the exposure chamber. System validation showed acceptable degree of variation of the test material tested, Fluorescent Microspheres (FMS) throughout the exposure chamber (CV < 15.0%). Particle size (MMAD ± GSD) using the APS was shown to be stable throughout the exposure periods.

The IVR model developed in this project was based on a number of euthanased (n=7), female Sprague-Dawley rats (weight: 372 ± 56 g), which underwent high-resolution micro-CT scans. The physical model consisted of five sub sections; Extra-Thoracic region containing the snout and nasophyarynx, trachea-bronchial region containing the trachea, bronchi, and bronchioles. All sections of the model were attached to one another in numerical order and housed within a containment unit. At the rear end of the cast, a flexible diaphragm was attached in order to collect the fraction of inhaled particles exiting the TB section and possibly reaching the lung, referred to as the Post-TB section. 

A study was conducted to assess the influence of inhalation parameters such as the breathing frequency and tidal volume on total and regional dose distribution using FMS as test material. The major finding of this study was the demonstration of the model sensitivity to changes in breathing parameters especially respiratory frequency, where the data showed increased deposition in the peripheral regions of the model with decreased respiratory frequency. Other studies assessed the effect of particle characteristics on deposition on the IVR model, such as particle size, dose increase and formulation changes. 
The results assessing particle size effect showed a slightly higher deposition levels for the 4µm sized particles versus 2µm sized particles in the head region; 90.8 ± 3.6% and 88.2 ± 6.6%. However, this difference did not reach statistical significance (P> 0.05) probably due to the polydispersity of aerosolised FMS particles. In addition, the regional deposition analysis showed an increased lung peripheral deposition with the smaller particles. In addition, the model was shown to be sensitive to changes in formulation composition mediated by inclusion of MgSt. 

The next stage of work was to validate the model in terms of comparison with lung deposition for in vivo rats.  For lung deposition comparison, the absolute amount deposited in the IVR lung model (expressed as µg/kg) was shown to have a reasonably strong correlation with in vivo lung concentration measures (µg/kg); R2= 0.66, P < 0.05. Compounds were predicted well and within 2-folds of the measured lung deposition values. However, knowing the variability in biological systems and the multiple components required to estimate lung doses, predictions within 2-fold of the measured values would seem reasonable

In terms of comparison with in silico model predictions using MPPD, similar deposition levels were noted between the two models, particularly when the data was expressed as percentage of total particles inhaled. The data showed the highest deposition levels were noted in the head region (> 80%) and less than 5.0% deposition for the peripheral lung fractions. 

With regards to using the IVR model to assess the relationship between dose, particle size and efficacy, an in vivo study using FP with different particle sizes (2.0 and 4.0 µm) but same doses ( 100 and 1000 µg/kg).  This study demonstrated that exposure of rat to FP powder resulted in a dose-dependent inhibition of neutrophils in BAL fluids. However, a clear difference in neutrophils suppression was demonstrated for equivalent doses but different particle sizes of FP, where the smaller FP particles (2.0 µm) induced a greater level of neutrophils suppression in comparison with larger FP particles (4.0 µm). In addition, a reasonably good correlation for the relationship between lung deposition in the IVR model and a neutrophils suppression level was demonstrated. Furthermore this data support the hypothesis that regional deposition is an important determinant in efficacy. Therefore, this suggests that the IVR model may be a useful as a tool to describe in vivo efficacy with in vitro data. However, further studies should be conducted to evaluate the validity of this model and relationship.

The IVR model has a number of important limitations. First, the model is based on scans up to generation four of the rat respiratory tract as this represented the limits of the micro-CT scanning technology at the time of this study. Therefore deposition in the deeper region of the lung may not be reflected precisely in the IVR model. Second, the regional deposition data generated using the model tended to show an overestimation of deposition in head region and an underestimation of deposition in the peripheral regions of the lung, in comparison with in vivo lung deposition data. Third, the current model does not take into account lung clearance. However, the amount of the drug present in the in vivo lungs is dependent on numerous physiological processes such as dissolution, passive or active absorption into the systemic circulation, binding to lung tissue and mucociliary clearance. Consequently, the results generated using this IVR model for drug molecules with high lung clearance rate should be treated with some caution. 

Future work extending this research could go in a number of directions. In this research, a representative model of the rat respiratory tract was constructed from analysis of imaging data from a number of euthanised Sprague-Dawley rats. This model represented the “average respiratory tract” in terms of dimensions of Sprague-Dawley rats. However, there is considerable variability in the airway dimensions between rats. This variability encompasses a number of factors such as the strains of rats, sex and age, and disease state. Thus, it may be possible to produce a small number of airway models to represent small and large rats and scaled to represent the extrathoracic and peripheral regions based on literature reports of their dimensions in different rat populations. This approach will then enable the effect of intersubject airway dimensions for different rat populations on aerosol deposition to be thoroughly examined.

In addition, due to the limitation of the micro-CT technology used to construct the physical IVR model, detailed morphology only up to generation 4 were captured. However, recent advances in MRI technology, such as the use of in situ-MRI based scanning technology have enabled rat airway morphometry to be extended to 16 airway generation. This coupled with improvements in the resolutions of rapid-prototyping process means it may be possible to construct a rat model that reflects the in vivo lung morphology more accurately, and thus enable greater understanding of the link between aerosol deposition and airway geometry.  

In conclusion, a model cast of the rat lung was developed and validated to allow the deposition of inhaled particles in the rat lung to be investigated. The model may be used to estimate the lung concentration in vivo rats in preference to exposure concentration measurements based on filter samples which have been shown to be a poor indicator of the lung concentration immediately after exposure. In addition, the model has the potential to be used along with live rats in an inhalation rig in pulmonary pharmaceutics research and may facilitate in development of inhaled formulations to target specific regions within the lung as well as screening of inhaled drugs in preclinical setting.
N2  - Das Ziel dieser Arbeit war es, ein in vitro Modell (IVR) der Rattenlunge für die Untersuchung der Deposition von Wirkstoffpartikeln in den Atemwegen der Ratte zu entwickeln. Das Modell sollte dabei den Einfluss der Arzneistoffeigenschaften und physiologischer Parameter auf die pulmonale Deposition berücksichtigen. Darüber hinaus wurden die Modellergebnisse mit in vivo Daten aus Versuchen mit Ratten und in silico Vorhersagen eines etablierten Computermodells der Partikeldeposition in präklinischen Spezies verglichen.

Erste Arbeiten konzentrierten sich auf die Entwicklung eines Aerosol-Expositionssystems, das in der Lage war, kleine Nagetiere einer Reihe von inhalativ verabreichten Testmaterialien auszusetzen. Das System bestand aus zwei Hauptteilen, einem Wirbelbett-Aerosolgenerator und einer Verabreichungskammer, die eine nasale Partikelexposition und –inhalation („Nose only Inhalation“) bei 12 Kleintieren auf einer Etage ermöglichte. Darüber hinaus wurde ein aerodynamisches Partikelspektrometer (APS) zur kontinuierlichen Messung der Größenverteilung und Konzentration der erzeugten Aerosolpartikel eingebaut. Die Systemvalidierung zeigte einen akzeptablen Grad der Variabilität des Testmaterials, Fluoreszenz-Mikrosphären (FMS), in der gesamten Expositionskammer (VK < 15,0%). Es konnte gezeigt werden, dass die aerodynamische Partikelgröße (MMAD ± GSD) der APS über die Expositionszeiten konstant blieb.

Das IVR-Modell, das in diesem Projekt entwickelt wurde, basierte auf einer Anzahl euthanasierter, weiblicher Sprague-Dawley-Ratten (Gewicht: 372 ± 56 g), die hochauf¬lösenden Mikro-CT-Scans unterzogen wurden. Das physikalische Modell gliederte sich in fünf Teilabschnitte, dem extrathorakalen Bereich bestehend aus der Schnauze und dem Nasopharynx, und dem tracheo-bronchialen Bereich (TB), der die Luftröhre, Bronchien und Bronchiolen umfasste. Alle Abschnitte des Modells wurden miteinander in numerische Reihenfolge gebracht und innerhalb einer Behältereinheit untergebracht. Am hinteren Ende des Gusses wurde eine flexible Membran angebracht, um den Anteil der inhalierten Partikel, der den TB-Abschnitt verlässt und möglicherweise die Lunge erreicht, zu sammeln. Dieses wurde als Post-TB-Anteil bezeichnet.

Eine Untersuchung sollte zeigen, welchen Einfluss Inhalationsparameter wie die Atem¬frequenz und –volumen auf die gesamte und regionale Dosisverteilung der FMS als Test¬material hatten. Das wichtigste Ergebnis dieser Studie war der Nachweis, dass das Modell empfindlich gegenüber Änderungen in der Respirationsparameter, vor allem der Atem¬frequenz, war. 

Die Daten zeigten, dass es unter verminderter Atemfrequenz zu einer verstärkten Partikeldeposition in den peripheren Modellbereichen kam. In weiteren Versuchsansätzen wurden die Wirkung von Partikeleigenschaften, wie Partikelgröße, Dosiserhöhung und Formulierungsänderungen auf die Deposition in dem IVR-Modell ermittelt.

Die Ergebnisse der Untersuchung des Partikelgrößeneffektes zeigten eine etwas höhere Deposition der 4 µm großen Partikel, verglichen mit den 2 µm Partikeln, im Kopfbereich, 90,8 ± 3,6% bzw. 88,2 ± 6,6%. Allerdings war dieser Unterschied statistisch nicht signifikant (P > 0,05), wahrscheinlich aufgrund der Polydispersität der FMS-Aerosolpartikel. Darüber hinaus zeigte die Analyse der regionalen Verteilung eine erhöhte periphere Lungendeposition bei kleineren Partikeln. Zudem war das Modell empfindlich gegenüber Veränderungen in der Formulierungszusammensetzung durch Zugabe von Magnesium¬stearat.

In nächsten Schritt sollte das Modell in Bezug auf den Vergleich mit der Lungendeposition bei Ratten in vivo validiert werden. Es zeigte sich, dass die absolut im IVR-Lungenmodell deponierte Menge (ausgedrückt in µg/kg) eine annehmbar starke Korrelation mit in vivo Daten (µg/kg) aufwies; R2 = 0,66, p < 0,05. Substanzen konnten gut innerhalb des 2-fachen Bereiches der gemessenen Lungendepositionsrate vorhergesagt werden. Angesichts der bekannt hohen Variabilität in biologischen Systemen und der Komplexität der Schätzung der Lungendeposition erscheinen Schwankungen der Vorhersagen innerhalb des 2-fachen Bereiches der tatsächlichen Werte akzeptabel.

Der Vergleich der in silico Vorhersagen mit den IVR-Resultaten zeigte ähnliche Depositions¬raten in beiden Modellen, insbesondere dann, wenn die Daten als Prozentsatz der insgesamt inhalierten Partikel ausgedrückt wurden. Die höchste Deposition fand im Kopfbereich (> 80%) statt und weniger als 5,0 % der Partikel erreichte den peripheren Lungenbereich.

Das IVR-Modell wurde nachfolgend auch in einer in vivo Studie mit Fluticasonpropionat (FP) eingesetzt, um die Beziehung zwischen der Dosis, Partikelgröße und Wirksamkeit unterschiedlicher Teilchengrößen (2,0 und 4,0 µm) bei gleichen Dosen (100 und 1000 µg/kg) zu beurteilen. Diese Studie zeigte eine dosisabhängige Hemmung der Neutrophilen in der bronchoalveolären Lavage. Es wurde jedoch ein deutlicher Unterschied in der Neutrophilensuppression unter äquivalenten Dosen unterschiedlicher Partikelgrößen beobachtet. Kleinere Partikel (2,0 µm) von FP hemmten die Neutrophilen stärker als die größeren FP-Partikel (4,0 µm). Darüber hinaus konnte eine recht gute Korrelation zwischen der Lungendepositionsrate im IVR-Modell und der Neutrophilensuppression gezeigt werden.
 Diese Daten unterstützen die Hypothese, dass die regionale Deposition eine wichtige Determinante der Wirksamkeit ist. Die Ergebnisse legen die mögliche Eignung des IVR-Modells als Hilfsmittel zur Beschreibung der in vivo Effektivität, ausgehend von in vitro Daten, nahe. Allerdings sollten weitere Studien durchgeführt werden, um die Valididtät dieses Modells und der gefundenen Beziehung zu bestätigen. Das IVR-Modell hat eine Reihe von wichtigen Einschränkungen. Erstens basiert das Modell auf Scans lediglich bis zu vierten Generation der Atemwege, was zum Zeitpunkt dieser Studie die Grenze der Mikro-CT-Scan-Technik darstellte. Daher wird in dem IVR-Modell eine Deposition in tieferen Bereichen der Lunge nicht präzise beschrieben. Zweitens zeigten die regionalen Depositionsdaten, die unter Verwendung des Modells ermittelt wurden, im Vergleich zu in vivo Ergebnissen eine Überschätzung der Deposition im Kopfbereich und eine Unterschätzung der Deposition in den peripheren Regionen der Lunge. Drittens berücksichtigt das Modell nicht die Clearance des Arzneistoffes.

Die Arzneistoffkonzentration in der Lunge hängt in vivo von zahlreichen physiologischen Prozessen ab, wie Auflösung, aktive und passive Absorption in den systemischen Kreislauf, die Bindung an das Lungengewebe und mukoziliäre Clearance. Daher sollten die Ergebnisse, die unter Verwendung dieses IVR-Modells gewonnen werden, für Wirkstoff¬moleküle mit hoher Clearance-Rate mit einer gewissen Vorsicht behandelt werden.

Zukünftige weiterführende Arbeiten könnten in eine Reihe von Richtungen gehen. In der vorliegenden Untersuchung wurde ein repräsentatives Modell des Rattenrespirationstraktes aus der Analyse der Bilddaten mehrerer anästhesierter Sprague-Dawley-Ratten erstellt. Dieses Modell repräsentiert die "durchschnittlichen Atemwege " in Bezug auf Abmessungen der Sprague-Dawley-Ratten. Es gibt jedoch eine beträchtliche Variabilität basierend auf einer Reihe von Faktoren wie den Rattenstamm, Geschlecht, Alter und Krankheitszustand. Es wäre möglich, mehrere verschiedene Atemwegsmodelle zu erstellen, um kleine und große Ratten zu repräsentieren. Es könnten, basierend auf Literaturangaben, die extra¬thorakalen und peripheren Regionen in ihren Abmessungen skaliert werden, um verschiedenen Rattenpopulationen zu repräsentieren. Dieser Ansatz würde dann die detaillierte Untersuchung des Einflusses interindividueller Unterschiede der Atemwegs¬dimensionen verschiedener Rattenpopulationen auf die Aerosoldeposition ermöglichen.






Aufgrund der Beschränkung der Mikro-CT-Technologie, die eingesetzt wurde, um das IVR-Modell zu erstellen, konnte eine detaillierte Morphologie nur bis zur vierten Atemwegs¬generation abgebildet werden. Jüngste Fortschritte in der MRI-Technologie, wie die in situ MRI-Scan-Technologie, ermöglichen die Erfassung der Atemwegsmorphometrie bis zu 16 Atemwegsgenerationen. Dieser Ansatz, in Verbindung mit Verbesserungen in den räumlichen Auflösungen der „Rapid-Prototyping“-Verfahren, könnte die Konstruktion eines Rattenmodells ermöglichen, das die in vivo Lungenmorphologie genauer widerspiegelt, und so zu einem besseren Verständnis für den Zusammenhang zwischen Aerosoldeposition und Atemwegsgeometrie führen.

Zusammenfassend lässt sich sagen, dass in der vorliegenden Arbeit ein Modellguss der Rattenlunge entwickelt und validiert wurde, um die Untersuchung der Deposition von inhalierten Partikel in der Rattenlunge zu ermöglichen. Das Modell kann verwendet werden, um die in vivo Lungenkonzentrationen von Arzneistoffen in Ratten abzuschätzen. Es bietet Vorteile gegenüber der Expositionsabschätzung auf der Basis von Filterproben, die ein schlechter Indikator der Lungenkonzentrationen unmittelbar nach der Exposition sind. Darüber hinaus hat das Modell das Potenzial, zusammen mit lebenden Ratten in einer Inhalationskammer in der Forschung verwendet zu werden und könnte in der Entwicklung von inhalativen Formulierungen erleichtern, die in bestimmten Regionen innerhalb der Lunge deponiert werden sollen. Darüber hinaus ermöglicht das Modell ein Screening inhalativ verabreichter Arzneistoffe in der präklinischen Phase.
KW  - In vitro rat
KW  - Ratte
KW  - in silico models
KW  - lung
KW  - deposition
KW  - Atemwege
KW  - In vitro
KW  - Wirkstoff
KW  - Inhalation
Y1  - 2014
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-104912
ER  - 
TY  - JOUR
A1  - Ahmad, Ruhel
A1  - Wolber, Wanja
A1  - Eckardt, Sigrid
A1  - Koch, Philipp
A1  - Schmitt, Jessica
A1  - Semechkin, Ruslan
A1  - Geis, Christian
A1  - Heckmann, Manfred
A1  - Brüstle, Oliver
A1  - McLaughlin, John K.
A1  - Sirén, Anna-Leena
A1  - Müller, Albrecht M.
T1  - Functional Neuronal Cells Generated by Human Parthenogenetic Stem Cells
JF  - PLoS One
N2  - Parent of origin imprints on the genome have been implicated in the regulation of neural cell type differentiation. The ability of human parthenogenetic (PG) embryonic stem cells (hpESCs) to undergo neural lineage and cell type-specific differentiation is undefined. We determined the potential of hpESCs to differentiate into various neural subtypes. Concurrently, we examined DNA methylation and expression status of imprinted genes. Under culture conditions promoting neural differentiation, hpESC-derived neural stem cells (hpNSCs) gave rise to glia and neuron-like cells that expressed subtype-specific markers and generated action potentials. Analysis of imprinting in hpESCs and in hpNSCs revealed that maternal-specific gene expression patterns and imprinting marks were generally maintained in PG cells upon differentiation. Our results demonstrate that despite the lack of a paternal genome, hpESCs generate proliferating NSCs that are capable of differentiation into physiologically functional neuron-like cells and maintain allele-specific expression of imprinted genes. Thus, hpESCs can serve as a model to study the role of maternal and paternal genomes in neural development and to better understand imprinting-associated brain diseases.
KW  - methylation
KW  - derivation
KW  - blastocysts
KW  - pluripotent
KW  - differentiation
KW  - lines
KW  - brain development
KW  - in-vitro
KW  - mice
KW  - specification
Y1  - 2012
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-130268
VL  - 7
IS  - 8
ER  - 
TY  - THES
A1  - Ahmad, Ruhel
T1  - Neurogenesis from parthenogenetic human embryonic stem cells
T1  - Neurogenese von parthenogenetischen humanen embryonalen Stammzellen
N2  - Imprinted genes play important roles in brain development. As the neural developmental capabilities of human parthenogenetic embryonic stem cells (hpESCs) with only a maternal genome were not assessed in great detail, hence here the potential of hpESCs to differentiate into various neural subtypes was determined. In addition DNA methylation and expression of imprinted genes upon neural differentiation was also investigated. The results demonstrated that hpESC-derived neural stem cells (hpNSCs) showed expression of NSC markers Sox1, Nestin, Pax6, and Musashi1 (MS1), the silencing of pluripotency genes (Oct4, Nanog) and the absence of activation of neural crest (Snai2, FoxD3) and mesodermal (Acta1) markers. Moreover, confocal images of hpNSC cultures exhibited ubiquitous expression of NSC markers Nestin, Sox1, Sox2 and Vimentin. Differentiating hpNSCs for 28 days generated neural subtypes with neural cell type-specific morphology and expression of neuronal and glial markers, including Tuj1, NeuN, Map2, GFAP, O4, Tau, Synapsin1 and GABA. hpNSCs also responded to region-specific differentiation signals and differentiated into regional phenotypes such as midbrain dopaminergic- and motoneuron-type cells. hpESC-derived neurons showed typical neuronal Na+/K+ currents in voltage clamp mode, elicited multiple action potentials with a maximum frequency of 30 Hz. Cell depicted a typical neuron-like current pattern that responded to selective pharmacological blockers of sodium (tetrodotoxin) and potassium (tetraethylammonium) channels. Furthermore, in hpESCs and hpNSCs the majority of CpGs of the differentially methylated regions (DMRs) KvDMR1 were methylated whereas DMR1 (H19/Igf2 locus) showed partial or complete absence of CpG methylation, which is consistent with a parthenogenetic (PG) origin. Upon differentiation parent-of-origin-specific gene expression was maintained in hpESCs and hpNSCs as demonstrated by imprinted gene expression analyses. Together this shows that despite the lack of a paternal genome, hpNSCs are proficient in differentiating into glial- and neuron-type cells, which exhibit electrical activity similar to newly formed neurons. Moreover, maternal-specific gene expression and imprinting-specific DNA-methylation are largely maintained upon neural differentiation. hpESCs are a means to generate histocompatible and disease allele-free ESCs. Additionally, hpESCs are a unique model to study the influence of imprinting on neurogenesis.
N2  - Imprinted Gene spielen eine wichtige Rolle bei der Gehirnentwicklung. Da das neurale Entwicklungspotenzial von hpESCs bisher noch nicht ausführlich untersucht wurde, war das Ziel dieser Arbeit das Differenzierungspotenzial von hpESCs zu verschiedenen neuralen Subtypen zu untersuchen. Außerdem wurden die DNA-Methylierung und Expression imprinted Gene in hpESCs während der neuralen Differenzierung analysiert. Die Ergebnisse zeigten, dass von hpESCs abgeleitete neurale Stammzellen (hpNSCs) die NSC-Marker Sox1, Nestin, Pax6 und Musashi1 (MS1) exprimierten, Pluripotenzmarker-Gene (Oct4, Nanog) abschalteten und keine Aktivierung von Markern der Neuralleistenzellen (Snai2, FoxD3) sowie dem mesodermalen Marker Acta1 stattfand. Immunfärbungen zeigten weiterhin, dass aus hpESCs abgeleitete Stammzellen die NSC-Marker Nestin, Sox1, Sox2 und Vimentin auf Proteinebene exprimierten. Durch gerichtete neurale Differenzierung für 28 Tage konnten aus hpESCs neurale Subtypen abgeleitet werden, die eine neurale Zelltyp-spezifische Morphologie aufweisen und positiv für neuronale und gliale Marker wie Tuj1, NeuN, Map2, GFAP, O4, Tau, Synapsin1 und GABA sind. Um aus hpNSCs dopaminerge und Motoneuronen abzuleiten, wurden während der Differenzierung Morphogene und trophische Faktoren zugegeben. Elektrophysiologische Analysen konnten zeigen, dass die in vitro differenzierten Neuronen, die von hpESCs abgeleitet wurden, für Neurone typische Na+/K+ Ströme sowie Aktionspotentiale (30 Hz) vorweisen ausbilden und auf ausgewählte pharmakologische Natrium- (Tetrodotoxin) und Kalium- (Tetraethylammonium) Kanal-Blocker reagierten. Desweiteren war der Großteil der CpGs von differentiell methylierten Regionen (DMRs) KvDMR1 in hpESCs und hpNSCs methyliert, während DMR1 (H19/Igf2 Locus) eine partiell oder komplett abwesende CpG-Methylierung zeigte, was dem parthenogenetischen Ursprung entspricht. Während der Differenzierung wurde die elternabhängige (parent-of-origin) spezifische Genexpression in hpESCs und hpNSCs aufrechterhalten, wie mit Genexpressionsanalysen imprinted Gene gezeigt werden konnte. In der Summe zeigen die hier dargestellten Ergebnisse, dass hpESCs, die kein paternales Genom besitzen, keine Beeinträchtigung im neuralen Differenzierungspotential zeigten und zu Gliazellen und Neurone differenziert werden konnten. Elektrophysiologische Analysen zeigten ferner, dass von hpESCs abgeleitete Neurone funktionell sind. Zudem wird die Expression maternal-spezifischer Gene und die Imprinting-spezifische DNA-Methylierung während der Differenzierung größtenteils aufrechterhalten. In der Summe stellen hpESCs ein einzigartiges Modell dar, um den Einfluss des Imprintings auf die Neurogenese zu untersuchen.
KW  - Embryonale Stammzelle
KW  - Neurogenese
KW  - Zelldifferenzierung
KW  - Stammzelle
KW  - human parthenogenetic stem cells
KW  - in vitro neural differentiation
KW  - human parthenogenetic neural stem cells
KW  - PG neurons
KW  - imprinting.
Y1  - 2012
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-75935
ER  - 
TY  - JOUR
A1  - Aguzzi, A.
A1  - Wagner, E. F.
A1  - Netzer, K. O.
A1  - Bothe, K.
A1  - Anhauser, I.
A1  - Rethwilm, Axel
T1  - Human foamy virus proteins accumulate in neurons and induce multinucleated giant cells in the brain of transgenic mice
N2  - Humanfoamy virus (HFV) is a retrovirus encoding structural genes and, like human immunodeficiency virus and human T ceU leukemia virus I, several anciUary reading frames collectively termed the belgenes. We have previously shown that HFV transgenic mice develop an encephalopathy with neuronal loss in hippocampus and cerebral cortex. We have now raised and characterized rabbit antisera to various recombinant portions of gag, pot, env, and bel-I, the viraltransactivator. Immunoreactivity for gag and bel-I was observed in nuclei and processes of hippocampal and cortical neurons before the onset of morphological lesions and correlated with the appearance of HFV mRNA. Astrocyte-derived multinucleated giant ceUs containing HFV proteins were present in the brain oftransgenic mice coexpressingfuU- length HFV genes but not in mice expressing truncated gag and env, suggesting that these genes contain afusogenic domain. Expression of fuU-length structural genes decreased the life expectancy oftransgenic mice, implying an a4Juvant rolefor these proteins in HFV-induced brain damage. (Am] Pathol 1993, 142:1061-1072)
KW  - Molekularpathologie
Y1  - 1993
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-47356
ER  - 
TY  - JOUR
A1  - Aguzzi, A.
A1  - Both, K.
A1  - Anhauser, I.
A1  - Horak, I.
A1  - Rethwilm, Axel
A1  - Wagner, EF.
T1  - Expression of human foamy virus is differentially regulated during development in transgenic mice
N2  - Tbe human foamy virus (HFV) is a recently characterized member ofthe spumavirus family. Although no diseases have been unequivocally associated with HFV infection, expression of HFV regulatory genes in transgenie mice induces a characteristic aeute neuro degenerative disease and a myopathy. To better eharaeterize the sequenee of events leading to disease, and to gain a better understanding of the underlying pathogenetic meehanisms, we have analyzed in detail the transgene expression pattern during development. Transcription of a construet containing all regulatory elements and aneillary genes of mv was analyzed by in situ hybridization and was shown to occur in two distinct phases. At midgestation, low but widespread expression was first deteeted in eells of extraembryonie tissues. Later, various tissues originating from embryonie mesoderm, neuroeetoderm, and neural erest transeribed the transgene at moderate levels. However, expression deereased dramatically during late gestation and was suppressed shortly after birth. After a latency period of up to 5 weeks, transeription of the transgene resumed in single eelJs distributed irregularly in the central nervous system and in the skeletal museIe. By the age of 8 weeks, an increasing number of eells displayed much higher expression levels than in embryonie Iife and eventually underwent severe degenerative ehanges. These findings demonstrate that HFV transgene expression is differentially regulated in development and that HFV cytotoxicity may be dose-dependent. Such biphasic pattern of expression differs from that of murine retroviruses and may be explained by the specificity of HFV regulatory elements in combination with cellular faetors. Future studies of this model system should, therefore, provide novel insights in the mechanisms controlling retrovirallatency.
KW  - Virologie
Y1  - 1992
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-55290
ER  - 
TY  - JOUR
A1  - Agranovsky, A. A.
A1  - Dolya, V. V.
A1  - Gorboulev, Valentin G.
A1  - Kozlov, J. V.
A1  - Atabekov, J. G.
T1  - Aminoacylation of barley stripe mosaic virus RNA: polyadenylate-containing RNA has a 3'-terminal tyrosine-accepting structure
N2  - Barley stripe mosaic virus (BSMV) RNA which was previously reported to contain poly(A) sequences (Agranovsky et al., 1978) can be specifically esterified with tyrosine in vitro in the presence of an aminoacyl-tRNA synthetase fraction from wheat embryos. All the three RNA components of the BSMV strain with a three-component genome (Norwich) and both RNA components of a two-component strain (Russian) can be tyrosylated. The poly(A)-containing (bound to oligo(dT)-cellulose) and poly(A)-deficient(not bound to oligo(dT)-cellulose) fractions of BSMV RNA display a similar amino acidaccepting ability. The nucleotide sequence which accepts tyrosine is coupled with the intact genomic polyadenylated BSMV RNA. The viral RNA isolated after sucrose density gradient centrifugation under drastic denaturing conditions retains its aminoacylating activity, which suggests that this activity is not due to the presence in a BSMV RNA preparation of a tyrosine tRNA associated with BSMV RNA. Inhibition of aminoacylation of the 3’-oxidized (treated with sodium metaperiodate) BSMV RNA suggests that the tyrosine-accepting structure is localized at the 3’ terminus of BSMV RNA molecules. It is shown that segments of different lengths obtained upon random fragmentation can be tyrosylated. The 3’-terminal (tyrosine-accepting) poly(A)+ segments can be isolated. The shortest segments of viral RNA capable of being aminoacylated [i.e., containing both tRNA-like structure and poly(A)] consists of approximately 150-200 nucleotides. The analysis of the oligonucleotides derived from individual BSMV RNA components labeled with 32P at the 3’ end revealed two types of 3’-terminal sequences different from poly(A). It is suggested that a poly(A) sequence is intercalated between a 3’-terminal tyrosineaccepting structure and the 5’-terminal portion of poly(A)+ BSMV RNA.
Y1  - 1981
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-32566
ER  - 
TY  - JOUR
A1  - Agoston, Zsuzsa
A1  - Li, Naixin
A1  - Haslinger, Anja
A1  - Wizenmann, Andrea
A1  - Schulte, Dorothea
T1  - Genetic and physical interaction of Meis2, Pax3 and Pax7 during dorsal midbrain development
JF  - BMC Developmental Biology
N2  - Background: During early stages of brain development, secreted molecules, components of intracellular signaling pathways and transcriptional regulators act in positive and negative feed-back or feed-forward loops at the mid-hindbrain boundary. These genetic interactions are of central importance for the specification and subsequent development of the adjacent mid-and hindbrain. Much less, however, is known about the regulatory relationship and functional interaction of molecules that are expressed in the tectal anlage after tectal fate specification has taken place and tectal development has commenced. 
Results: Here, we provide experimental evidence for reciprocal regulation and subsequent cooperation of the paired-type transcription factors Pax3, Pax7 and the TALE-homeodomain protein Meis2 in the tectal anlage. Using in ovo electroporation of the mesencephalic vesicle of chick embryos we show that (i) Pax3 and Pax7 mutually regulate each other's expression in the mesencephalic vesicle, (ii) Meis2 acts downstream of Pax3/7 and requires balanced expression levels of both proteins, and (iii) Meis2 physically interacts with Pax3 and Pax7. These results extend our previous observation that Meis2 cooperates with Otx2 in tectal development to include Pax3 and Pax7 as Meis2 interacting proteins in the tectal anlage. 
Conclusion: The results described here suggest a model in which interdependent regulatory loops involving Pax3 and Pax7 in the dorsal mesencephalic vesicle modulate Meis2 expression. Physical interaction with Meis2 may then confer tectal specificity to a wide range of otherwise broadly expressed transcriptional regulators, including Otx2, Pax3 and Pax7.
KW  - dosage
KW  - quali-chick chimeras
KW  - drosophila embryo
KW  - neural crest
KW  - transcription activation
KW  - hindbrain boundary
KW  - isthmic oragnizer
KW  - sonic hedghog
KW  - expression
KW  - induction
Y1  - 2012
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-132626
VL  - 12
IS  - 10
ER  - 
TY  - THES
A1  - Agnetta, Luca
T1  - Novel Photoswitchable and Dualsteric Ligands Acting on Muscarinic Acetylcholine Receptors for Receptor Function Investigation
T1  - Neue lichtschaltbare und dualstere Liganden für die muskarinischen Acetylcholin Rezeptoren zur Untersuchung der Rezeptorfunktion
N2  - G protein-coupled receptor research looks out for new technologies to elucidate the complex
processes of receptor activation, function and downstream signaling with spatiotemporal
resolution, preferably in living cells and organisms. A thriving approach consists in making use
of the unsurpassed properties of light, including its high precision in space and time, noninvasiveness
and high degree of orthogonality regarding biological processes. This is realized
by the incorporation of molecular photoswitches, which are able to effectively respond to light,
such as azobenzene, into the structure of a ligand of a given receptor. The muscarinic
acetylcholine receptors belong to class A GPCRs and have received special attention in this
regard due to their role as a prototypic pharmacological system and their therapeutic potential.
They mediate the excitatory and inhibitory effects of the neurotransmitter acetylcholine and
thus regulate diverse important biological processes, especially many neurological functions in
our brain.
In this work, the application of photopharmacological tool compounds to muscarinic receptors
is presented, consisting of pharmacophores extended with azobenzene as light-responsive
motif. Making use of the dualsteric concept, such photochromic ligands can be designed to bind
concomitantly to the orthosteric and allosteric binding site of the receptor, which is
demonstrated for BQCAAI (M1) and PAI (M2) and may lead to subtype- and functionalselective
photoswitchable ligands, suitable for further ex vivo and in vivo studies.
Moreover, photoswitchable ligands based on the synthetic agonist iperoxo were investigated
extensively with regard to their photochemical behavior and pharmacological profile, outlining
the advantages and challenges of using red-shifted molecular photoswitches, such as tetraortho-
fluoro azobenzene. For the first time on a GPCR it was examined, which impact the
different substitution pattern has on both the binding and the activity on the M1 receptor. Results
show that substituted azobenzenes in photopharmacological compounds (F4-photoiperoxo and
F4-iper-azo-iper) not just represent analogs with other photophysical properties but can exhibit
a considerably different biological profile that has to be investigated carefully.
The achievements gained in this study can give important new insights into the binding mode
and time course of activation processes, enabling precise spatial and temporal resolution of the
complex signaling pathway of muscarinic receptors. Due to their role as exemplary model
system, these findings may be useful for the investigation into other therapeutically relevant
GPCRs.
N2  - Die Forschung an G-Protein-gekoppelten Rezeptoren verlangt nach neuen Technologien zur
Aufklärung der komplexen Prozesse der Rezeptoraktivierung, -funktion und ihrer
nachgeschalteten Signalwege mit räumlicher und zeitlicher Auflösung, vorzugsweise in
lebenden Zellen und Organismen. Ein erfolgreicher Ansatz besteht darin, die unübertroffenen
Eigenschaften des Lichts zu nutzen, welche die hohe Präzision in Raum und Zeit, die Nicht-
Invasivität und die hohe Orthogonalität in Bezug auf biologische Prozesse einschließt. Dies
wird durch den Einbau von molekularen Photoschaltern, wie z. B. Azobenzolen, in die Struktur
eines Liganden eines bestimmten Rezeptors realisiert, welche effektiv auf Licht reagieren. Die
muskarinischen Acetylcholin Rezeptoren gehören zur Klasse A der GPCRs und haben aufgrund
ihrer Rolle als prototypisches pharmakologisches System und ihres therapeutischen Potenzials
diesbezüglich besondere Beachtung gefunden. Sie vermitteln die stimulierenden und
hemmenden Wirkungen des Neurotransmitters Acetylcholin und regulieren somit verschiedene
wichtige biologische Prozesse, insbesondere viele neurologische Funktionen in unserem
Gehirn.
In dieser Arbeit wird die Anwendung photopharmakologischer „Tool“-Verbindungen auf die
muskarinischen Rezeptoren vorgestellt, die aus Pharmakophoren bestehen, welche mit
Azobenzol als lichtempfindlichem Motiv modifiziert wurden. Mit Hilfe des Konzepts der
Dualsterie können solche photochromen Liganden so gestaltet werden, dass sie gleichzeitig an
die orthosterische und allosterische Bindungsstelle des Rezeptors binden, was für BQCAAI
(M1) und PAI (M2) gezeigt wurde und zu subtypen- und funktionsselektiven photoschaltbaren
Liganden führen kann, die für weitere Ex- und In-Vivo-Studien geeignet sind.
Darüber hinaus wurden photoschaltbare Liganden auf Basis des synthetischen Agonisten
Iperoxo hinsichtlich ihres photochemischen Verhaltens und ihres pharmakologischen Profils
ausführlich untersucht, um die Vorteile und Herausforderungen der Verwendung
rotverschobener molekularer Photoschalter wie tetra-ortho-Fluor-azobenzol zu erläutern. Es
wurde erstmals an einem GPCR untersucht, welche Auswirkungen das unterschiedliche
Substitutionsmuster sowohl auf die Bindung, als auch auf die Aktivität am M1-Rezeptor hat.
Diese Ergebnisse zeigen, dass substituierte Azobenzole in photopharmakologischen
Verbindungen (F4-Photoiperoxo und F4-Iper-azo-iper) nicht nur Analoga mit anderen
photophysikalischen Eigenschaften darstellen, sondern auch ein deutlich unterschiedliches
biologisches Profil aufweisen können, das sorgfältig untersucht werden muss. Die in dieser
Studie erzielten Ergebnisse geben neue und wichtige Einblicke in den Bindungsmodus und den zeitlichen Verlauf von Aktivierungsprozessen und ermöglichen eine präzise räumliche und
zeitliche Auflösung der komplexen Signalwege von muskarinischen Rezeptoren. Aufgrund
ihrer Rolle als exemplarisches Modellsystem können diese Befunde für die Untersuchung
anderer therapeutisch relevanter GPCRs sehr nützlich sein.
KW  - Muscarinrezeptor
KW  - G-Protein gekoppelte Rezeptor
KW  - G Protein-coupled receptor
Y1  - 2019
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-187170
ER  - 
TY  - JOUR
A1  - Aghai, Fatemeh
A1  - Zimmermann, Sebastian
A1  - Kurlbaum, Max
A1  - Jung, Pius
A1  - Pelzer, Theo
A1  - Klinker, Hartwig
A1  - Isberner, Nora
A1  - Scherf-Clavel, Oliver
T1  - Development and validation of a sensitive liquid chromatography tandem mass spectrometry assay for the simultaneous determination of ten kinase inhibitors in human serum and plasma
JF  - Analytical and Bioanalytical Chemistry
N2  - A liquid chromatography tandem mass spectrometry method for the analysis of ten kinase inhibitors (afatinib, axitinib, bosutinib,cabozantinib, dabrafenib, lenvatinib, nilotinib, osimertinib, ruxolitinib, and trametinib) in human serum and plasma for theapplication in daily clinical routine has been developed and validated according to the US Food and Drug Administration andEuropean Medicines Agency validation guidelines for bioanalytical methods. After protein precipitation of plasma samples withacetonitrile, chromatographic separation was performed at ambient temperature using a Waters XBridge® Phenyl 3.5μm(2.1×50 mm) column. The mobile phases consisted of water-methanol (9:1, v/v) with 10 mM ammonium bicarbonate as phase A andmethanol-water (9:1, v/v) with 10 mM ammonium bicarbonate as phase B. Gradient elution was applied at a flow rate of 400μL/min. Analytes were detected and quantified using multiple reaction monitoring in electrospray ionization positive mode. Stableisotopically labeled compounds of each kinase inhibitor were used as internal standards. The acquisition time was 7.0 min perrun. All analytes and internal standards eluted within 3.0 min. The calibration curves were linear over the range of 2–500 ng/mLfor afatinib, axitinib, bosutinib, lenvatinib, ruxolitinib, and trametinib, and 6–1500 ng/mL for cabozantinib, dabrafenib, nilotinib,and osimertinib (coefficients of correlation≥0.99). Validation assays for accuracy and precision, matrix effect, recovery,carryover, and stability were appropriate according to regulatory agencies. The rapid and sensitive assay ensures high throughputand was successfully applied to monitor concentrations of kinase inhibitors in patients.
KW  - kinase inhibitors
KW  - therapeutic drug monitoring
KW  - liquid chromatography tandem mass spectrometry (LC-MS/MS
KW  - afatinib
KW  - osimertinib
Y1  - 2021
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-231925
SN  - 1618-2642
VL  - 413
ER  - 
TY  - BOOK
A1  - Agbokhan, Serena
A1  - Sandig, Anna
A1  - Haas, Thea
A1  - Valentin, Francesca
A1  - Gasteiger, Annika
A1  - von Keller, Anna
A1  - Friedmann, Fiona
A1  - Wicht, Rebecca
A1  - Wintermeyer, Nina
A1  - Hofmann, Anna-Lena
A1  - Liebich, Alexander
A1  - Bördlein, Sophie
A1  - Lüderitz, Cathrin
A1  - Philipp, Sonja
A1  - Watermann, Anne
A1  - Hercher, Anna
ED  - Nelson-Teutsch, Hannah
T1  - Insights;
N2  - The cluster of texts assembled here were imagined, crafted, and brought together as a collaborative writing project that emerged from the seminar titled "Words Matter Worlds: Activist Scholarship and Literary Praxis," which convened over the course of the 2021/22 winter semester as an offering of the American Studies department of the Julius-Maximilians-Universität Würzburg. Like the seminar that nurtured the considerations that evolve here, these contributions engage with how scholarly writing practices in general, and literary and cultural studies in particular, can remake the world.
KW  - Aktivist
KW  - Literaturwissenschaft
KW  - Amerikanistik
KW  - Feminist
KW  - Kreatives Schreiben
KW  - Activist Scholarship
KW  - Literary and Cultural Studies
KW  - American Studies
Y1  - 2023
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-317007
SN  - 978-3-945459-44-7
ER  - 
TY  - THES
A1  - Agarwal, Vaibhav
T1  - Role of PspC interaction with human polymeric immunoglobulin receptor and Factor H in Streptococcus pneumoniae infections and host cell induced signalling
N2  - Streptococcus pneumoniae ist ein Gram-positives Bakterium und ein Kommensale des humanen Nasenrachenraums. Pneumokokken sind andererseits auch die Verursacher schwerer lokaler Infektionen wie der Otitis media, Sinusitis und von lebensbedrohenden invasiven Erkrankungen. So sind Pneumokokken die wichtigsten Erreger einer ambulant erworbenen Pneumonie und sie sind häufige Verursacher von Septikämien und bakteriellen Meningitiden. Die initiale Phase der Pathogenese ist verbunden mit der Besiedelung der mukosalen Epithelzellen des Rachenraumes. Diese Kolonisierung erleichtert die Aufnahme der Bakterien in die Zelle bzw. deren Dissemination in submukosale Bereiche und den Blutstrom. Die Konversion des Kommensalen zu einem invasiven Mikroorganismus ist assoziiert mit der Anpassung des Krankheitserregers an die verschiedenen Wirtsnischen und wird auf der Wirtsseite durch die Zerstörung der transepithelialen Barriere begleitet. Die Anpassung des Erregers ist vermutlich ein in hohem Grade regulierter Prozess. Die Oberfläche von Streptococcus pneumoniae ist mit Proteinen bedeckt, die kovalent oder nicht kovalent mit der Zellwand verknüpft sind. Eine einzigartige Gruppe von Oberflächenproteinen in der Zellwand der Pneumokokken sind die cholinbindenden Proteine (CBPs). Für einige der CBPs konnte bereits die Bedeutung für die Virulenz gezeigt werden. PspC, auch als SpsA oder CbpA bezeichnet, ist ein multifunktionales Oberflächenprotein, das als Adhesin und Faktor H-Bindungsprotein eine wichtige Rolle in der Pathogenese der Pneumokokken hat. PspC vermittelt als Adhesin die Anheftung der Bakterien an die mukosalen Epithelzellen, indem es human-spezifisch an die sekretorische Komponente (SC) des polymeren Immunoglobulinrezeptors (pIgR) bindet. SC ist die Ektodomäne des pIgR und PspC kann ebenso die freie SC binden oder an die SC des sekretorischen IgA Moleküls binden. PspC interagiert auch mit dem löslichen Komplement Faktor H. Die SC und der Faktor erkennen zwei verschiedene Epitope im bakteriellen PspC Protein. Der genaue Mechanismus der jeweiligen Interaktionen unter physiologischen- bzw. wirtspezifischen Bedingungen ist noch nicht vollständig verstanden. In dieser Arbeit wurde die Auswirkung der PspC Interaktion mit dem humanen pIgR (hpIgR) bzw. dem Faktor H auf die Virulenz der Pneumokokken und die Wirtszellantwort, d.h. die induzierten Signalkaskaden in den eukaryotischen Zellen untersucht. Die molekulare Analyse und die Verwendung von spezifischen pharmakologischen Inhibitoren der Signalmoleküle zeigten, dass verschiedene Signalmoleküle an der PspC-pIgR vermittelten Internalisierung beteiligt sind. Die Aktivierung, d.h. die Phosphorylierung der Signalmoleküle wurde in Immunblots demonstriert. Die Studien zeigten, dass das Aktinzytoskelett und die Mikrotubuli für die bakterielle Aufnahme essentiell sind. Es konnte auch zum ersten Mal nachgewiesen werden, dass Cdc42 die entscheidende GTPase für die Invasion der Pneumokokken in die Wirtsepithelzellen, vermittelt über den PspC-hpIgR Mechanismus, ist. Der Einsatz von PI3-kinase und Akt Kinase Inhibitoren reduzierte signifikant die hpIgR-vermittelte Aufnahme der Pneumokokken in die Wirtszelle. Zusätzlich durchgeführte Infektionen von hpIgR exprimierenden Zellen zeigten eine zeitabhängige Phosphorylierung von Akt und der p85&#945; Untereinheit der PI3-Kinase. Damit ist neben der GTPase Cdc42 der PI3K und Akt Signalweg entscheidend für die PspC-pIgR vermittelte Invasion der Pneumokokken. Des Weiteren sind an der Infektion mit Pneumokokken auch die Protein Tyrosin Kinasen Src, ERK1/2 und JNK beteiligt. Dabei wird die Src Kinase unabhängig von der PI3K in hpIgR exprimierenden Zellen aktiviert. Inhibitionsexperimente und genetische Knockdown Versuche mit siRNA bewiesen, dass die Endozytose der Pneumokokken über PspC-pIgR ein Clathrin und Dynamin abhängiger Mechanismus ist. Im weiterenn Teil der Arbeit wurde der Einfluss des PspC gebundenen Faktor H auf die Anheftung an und Invasion in die Epithelzellen analysiert. Die Bindung von Faktor H erfolgte unabhängig vom PspC-Subtyp. Die Bindungsversuche bewiesen, dass die Kapselmenge negativ korreliert mit der Bindung des Faktor H. Der Einsatz von Faktor H aus Maus oder Ratte zeigte keine typische Bindung. Daraus kann abgeleitet werden, dass diese Interaktion humanspezifisch ist. Die Infektionsexperimente demonstrierten, dass Faktor H die Adhärenz und die Invasion der Bakterien in die Nasenrachenraumzellen (Detroit562), alveolären Lungenepithelzellen (A549) und humanen Hirnendothelzellen (HBMEC) steigert. Der Faktor H hat Heparin Bindestellen. Diese Bindestellen vermitteln die Adhärenz der Faktor H gebundenen Pneumokokken mit Epithelzellen. Inhibitionsstudien mit spezifischen monoklonalen Antikörpern, die gegen die short consensus repeats (SCRs) von Faktor H gerichtet waren, konnten die essentielle Bedeutung der SCR19-20 für die Anheftung der Pneumokokken über Faktor H an die Wirtszellen nachweisen. Die Faktor H vermittelte Assoziation der Pneumokokken an polymorphonukleäre Leukozyten (PMNs) erfolgt über das Integrin CD11b/CD18. Die weiteren Inhibitionsstudien zeigten dann auch zum ersten Mal den Einfluss des Aktinzytoskeletts der Wirtszelle auf die Faktor H-vermittelten bakterieller Internalisierung und den dabei bedeutsamen Signaltransduktionswegen in der eukaryotischen Zelle. Dabei wurden insbesondere die Proteintyrosinkinasen und die PI3K als wichtige Signalmoleküle für die Faktor H vermittelte Invasion der Pneumokokken identifiziert. Die in dieser Arbeit erhaltenen Resultate belegen, dass die Faktor H vermittelte Infektion der Zellen mit S. pneumoniae ein konzertierter Mechanismus ist, bei dem Oberflächen-Glycosaminoglycane, Integrine und Signaltransduktionswege der Wirtsepithelzellen involviert sind. Des Weiteren wurde aufgezeigt, dass die PspC-pIgR-vermittelte Invasion in mukosale Epithelzellen unterschiedliche Signalwege wie z.B. den PI3K und Akt Weg induziert und abhängig von Cdc42 und einer Clathrin vermittelten Endozytosemechanismus ist.
N2  - Streptococcus pneumoniae (pneumococci) are Gram-positive bacteria and commensals of the nasopharyngeal cavity. Besides colonization, pneumococci are responsible for severe local infections such as otitis media, sinusitis and life-threatening invasive diseases, including pneumonia, sepsis and meningitis. The surface of pneumococci is decorated with proteins that are covalently or non-covalently anchored to the cell wall. The most unique group of cell wall associated proteins in pneumococci are the choline-binding proteins (CBPs). PspC, also known as SpsA or CbpA, is a multifunctional choline-binding protein that plays an essential role in pneumococcal pathogenesis by functioning as an adhesin. PspC promotes adherence of pneumococci to mucosal epithelial cells by interacting in a human specific manner with the free secretory component (SC) or to SC as part of the secretory IgA (SIgA) or polymeric immunoglobulin receptor (pIgR). PspC also interacts specifically with the soluble complement Factor H. Apparently, PspC uses two different epitopes for binding the soluble host protein Factor H and SC of pIgR. However, the mechanism by which these independent interactions facilitate pneumococcal infections under physiological and host specific conditions have not yet been completely elucidated. This study aims to explore the impact of the PspC interaction with human pIgR (hpIgR) or complement regulator Factor H on pneumococcal virulence. Here the cellular and molecular basis of PspC-mediated adherence to and invasion of host epithelial and endothelial cells was demonstrated. The genetic approach, specific pharmacological inhibitors and immunoblot analysis demonstrated the complexity of the induced signal transduction pathways during PspC-hpIgR mediated pneumococcal uptake by host cells. Inhibition studies with specific inhibitors of actin cytoskeleton and microtubules demonstrated that the dynamics of host cell cytoskeleton are essential for pneumococcal uptake by mucosal epithelial cells. Moreover, this study reports for the first time that the small GTPase Cdc42 is essential for pneumococcal internalization into epithelial cells via the PspC-hpIgR mechanism. In addition, in infection experiments performed in presence of specific inhibitors of PI3-kinase/Akt and protein tyrosine kinase (PTKs), hpIgR-mediated pneumococcal uptake by host cells was significantly blocked. Amongst PTKs the Src kinase pathway, ERK1/2 and JNK pathways were implicated during pneumococcal ingestion by hpIgR expressing cells. In addition, inhibition experiments performed in the presence of individual inhibitors or with a combination of inhibitors suggested the independent activation of PI3-kinase/Akt and Src kinase pathways during pneumococcal infections of hpIgR expressing cells. By employing specific inhibitors and siRNA in cell culture infection experiments it was further demonstrated that pneumococcal endocytosis by host epithelial cells via the PspC-hpIgR mechanism depends on clathrin and dynamin. PspC recruits also Factor H to the pneumococcal cell surface. Consequently, the impact of pneumococcal cell surface bound Factor H on adherence to host cells and the molecular mechanism facilitating the uptake of Factor H bound pneumococci by epithelial cells was investigated. Flow cytometry and immunoblots revealed that S. pneumoniae has evolved the ability to recruit both purified Factor H as well as Factor H from human plasma or serum. Moreover, it was demonstrated that the recruitment of Factor H is independent of the PspC-subtypes and that capsular polysaccharide (CPS) interferes with its recruitment. Factor H bound to pneumococci significantly increased bacterial attachment to and invasion of host epithelial cells including nasopharyngeal cells (Detroit562), lung epithelial cells (A549), and human brain-derived endothelial cells (HBMEC). Blocking experiments demonstrated that bacteria bound Factor H interacts via the heparin binding sites on Factor H with eukaryotic cell surface glycosaminoglycans and that this interaction promotes pneumococcal adherence to host cells. In addition, inhibition studies with mAbs recognizing specifically different short consensus repeats (SCR) of Factor H suggested that SCR 19-20 of Factor H are essential for the pneumococcal interaction with host epithelial cells via Factor H. In the presence of Factor H, attachment of pneumococci to human polymorphonuclear leukocytes (PMNs) is enhanced. The integrin CD11b/CD18 was identified as the cellular receptor on PMNs. By using pharmacological inhibitors the impact of host cell cytoskeleton and signalling molecules, such as PTKs and PI3-kinase, for Factor H-mediated pneumococcal internalization into eukaryotic cells was shown. Taken together, the results revealed that Factor-H mediated pneumococcal infection requires a concerted role of host epithelial cell surface glycosaminoglycans, integrins and host cell signalling pathways.
KW  - Streptococcus pneumoniae
KW  - Polymeric Immunoglobulin receptor
KW  - Factor H
Y1  - 2008
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-36526
ER  - 
TY  - THES
A1  - Agarwal, Shruti
T1  - Functional characterization of four CDK-like kinases and one Calmodulin-dependent kinase of the human malaria parasite, Plasmodium falciparum
T1  - Funktionelle Charakterisierung von vier CDK-like kinasen und eine Calmodulin-dependent kinasen des human Malaria parasite, Plasmodium falciparum
N2  - Malaria still persists as one of the deadliest infectious disease in addition to AIDS and tuberculosis. lt is a leading cause of high mortality and morbidity rates in the developing world despite of groundbreaking research on global eradication of the disease initiated by WHO, about half a century ago. Lack of a commercially available vaccine and rapid spread of drug resistance have hampered the attempts of extinguishing malaria, which still leads to an annual death toll of about one million people. Resistance to anti-malarial compounds thus renders search for new target proteins imperative. The kinome of the human malaria parasite Plasmodium falciparum comprises representatives of most eukaryotic protein kinase groups, including kinases which regulate proliferation and differentiation processes. Several reports till date have suggested involvement of parasite kinases in the human host and as well as in the mosquito vector. Kinases essential for life cycle stages of the parasite represent promising targets for anti-malarial compounds thus, provoking characterization of additional malarial kinases. Despite extensive research on most plasmodial enzymes, very little information is available regarding the four identified members of the cyclin dependent kinase like kinase (CLK) family. Thus, the present thesis dealt with the functional characterization of four members of the PfCLK kinase family of the parasite denoted as PfCLK-1/Lammer, PfCLK-2, PfCLK-3 and PfCLK-4 with a special focus on the first two kinases. Additionally, one Ca2+/Calmodulin dependent putative kinase-related protein, PfPKRP, presumed to be involved in sexual stage development of the parasite, was investigated for its expression in the life cycle of the parasite. In other eukaryotes, CLK kinases regulate mRNA splicing through phosphorylation of Serine/Arginine-rich proteins. Transcription analysis revealed abundance of PfCLK kinase genes throughout the asexual blood stages and in gametocytes. By reverse genetics approach it was demonstrated that all four kinases are essential for completion of the asexual replication cycle of P. falciparum. PfCLK 1/Lammer possesses two nuclear localization signals and PfCLK-2 possesses one of these signals upstream of the C-terminal catalytic domains. Protein level expression and sub-cellular localization of the two kinases was determined by generation of antiserum directed against the kinase domains of the respective kinase. Indirect immunofluorescence, Western blot and electron microscopy data confirm that the kinases are primarily localized in the parasite nucleus, and in vitro assays show that both enzymes are associated with phosphorylation activity. Finally, mass spectrometric analysis of co immunoprecipitated proteins shows interactions of the two PfCLK kinases with proteins, which have putative nuclease, phosphatase or helicase functions. PfPKRP on the other hand is predominantly expressed during gametocyte differentiation as identified from transcriptional analysis. Antiserum directed against the catalytic domain of PfPKRP detected the protein expression profile in both asexual and gametocyte parasite lysates. Via immunofluorescence assay, the kinase was localized in the parasite cytoplasm in a punctuated manner, mostly in the gametocyte stages. Reverse genetics resulted in the generation of PfPKRP gene-disruptant parasites, thus demonstrating that unlike CLK kinases, PfPKRP is dispensable for asexual parasite survival and hence might have crucial role in sexual development of the parasite. On one hand, characterization of PfCLK kinases exemplified the kinases involved in parasite replication cycle. Successful gene-disruption and protein expression of PfPKRP kinase on the other hand, demonstrated a role of the kinase in sexual stage development of the parasite. Both kinase families therefore, represent potential candidates for anti-plasmodial compounds.
N2  - Malaria stellt neben AIDS und Tuberkulose weiterhin eine der bedeutendsten Infektionskrankheiten dar. Trotz intensiver, auf die Auslöschung der Krankheit abzielender Forschung, welche vor etwa 50 Jahren durch die Weltgesundheitsorganisation initiiert wurde, bleibt Malaria einer der Hauptgründe für hohe Mortalität und Morbidität in Entwicklungsländern. Das Fehlen eines Impfstoffes und die schnelle Ausbreitung von Resistenzen erschweren die Versuche, Malaria zu eliminieren, welche jährlich weiterhin eine Todesrate von einer Millionen Menschen aufweist. Aufgrund der Zunahme an Resistenzen ist die Suche nach neuen Angriffspunkten für Antimalariamedikamente zwingend erforderlich. Das Kinom des humanpathogen Parasiten Plasmodium falciparum besteht aus Vertretern der meisten eukaryotischen Proteinkinasegruppen, einschließlich einiger Kinasen, welche Proliferations- und Differenzierungsprozesse regulieren. Verschiedenen Berichten zufolge ist eine Rolle von Parasitenkinasen sowohl im menschlichen Wirt als auch in der die Krankenheit übertragende Mücke denkbar. Kinasen, welche für verschiedene Parasitenstadien essentiell sind, stellen viel versprechende Angriffspunkte für Malariamedikamente dar. Dies bestätigt die Bedeutung der Erforschung von weiteren, bisher uncharakterisierten Kinasen. Trotz extensiver Forschungsarbeit an den meisten Enzymen des Parasiten ist bisher sehr wenig über die vier identifizierten Mitglieder der Proteinfamilie Zyklin-abhängige Kinase-ähnlicher Kinasen (cyclin-dependent kinase like kinases, CLK) bekannt. Aufgrund dessen war die Charakterisierung der vier Mitglieder der PfCLK Kinasefamilie, PfCLK-1/PfLAMMER, PfCLK-2, PfCLK-3 und PfCLK-4 Bestandteil dieser Arbeit. Der Forschungsschwerpunkt lag hierbei auf den beiden erstgenannten Kinasen. Zusätzlich wurde die stadienspezifische Expression von PfPKRP, einer Kinase, welche vermutlich in der Entwicklung der Sexualstadien des Parasiten beteiligt ist, untersucht. In anderen Eukaryoten regulieren die CLK kinases das Spleißen von mRNA durch die Phosphorylierung von Serin-/Arginin-reichen Proteinen. Untersuchungen hinsichtlich der Expression der CLK kinase zeigten eine Transkriptabundanz in allen asexuellen Blutstadien sowie in Gametozyten. Mit Hilfe der Reverse-Genetics-Technik, wurde festgestellt, dass alle vier Kinasen essentiell sind für die asexuelle Replikation von P. falciparum. PfCLK-1/Lammer besitzt zwei Kernlokalisationssequenzen, während PfCLK-2 ein solches Signal stromaufwärts der C-terminalen katalytischen Domäne aufweist. Die Expression auf Proteinebene sowie die subzelluläre Lokalisation der beiden Kinasen wurde durch die Herstellung von Antiseren gegen die jeweilige Kinasedomainen hergestellt. Indirekte Immunfluoreszenzstudien, Westernblots und elektronenmikroskopische Daten bestätigten die Lokalisation vornehmlich in Zellkern des Parasiten. In-vitro-Studien demonstrierten, das beide Enzyme mit Phosphorylierungsaktivität assoziierte sind. Die massenspektrometrische Analyse von ko-immunopräzipitierten Proteinen zeigten Interaktionen der beiden PfCLK Kinasen mit Proteinen, welche vermutlich Nuklease-, Phosphatase- oder Helikase-Funktion besitzen. Im Gegensatz zu den CLK-Kinasen wird PfPKRP wird hauptsächlich während der Differenzierung der Gametozyten exprimiert wie Transkriptanalysen zeigten. Antiseren gegen die katalytische Domäne von PfPKRP detektierten jedoch Proteinexpression sowohl in Lysaten asexueller Parasiten als auch in Gametozytenlysaten. In Immunfluoreszenzstudien wurde ein punktiertes Expressionsmuster im Zytoplasma beobachtet, wobei die Expression vornehmlich in Gametozyten stattfand. Die Tatsache, dass die Herstellung einer PfPKRP-Knock out Mutante möglich war, zeigt, dass PfPKRP für das Überleben asexueller Parasiten entbehrlich ist, weshalb eine wichtige Rolle in der sexuellen Entwicklung der Parasiten möglich ist. Zum Einen dient die Charakterisierung der PfCLK-Kinasen als Beispiel für Kinasen, welche eine wichtige Rolle im Replikationszyklus der Parasiten spielen. Das erfolgreiche Ausschalten von PfPKRP sowie Untersuchungen zur Expression der PfPKRP-Kinase lassen zum Anderen eine Rolle in den Sexual- oder Transmissionstadien vermuten. Aufgrund dessen stellen beide Kinasefamilien viel versprechende Kandidaten für die Herstellung von malariamedikamenten dar.
KW  - Plasmodium falciparum
KW  - Kinasen
KW  - RNS-Spleißen
KW  - Malaria
KW  - Kinase
KW  - Calcium
KW  - Splicing
Y1  - 2010
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-48522
ER  - 
TY  - JOUR
A1  - Agarwal, Shailesh R.
A1  - Yang, Pei-Chi
A1  - Rice, Monica
A1  - Singer, Cherie A.
A1  - Nikolaev, Viacheslav O.
A1  - Lohse, Martin J.
A1  - Clancy, Colleen E.
A1  - Harvey, Robert D.
T1  - Role of Membrane Microdomains in Compartmentation of cAMP Signaling
JF  - PLOS ONE
N2  - Spatially restricting cAMP production to discrete subcellular locations permits selective regulation of specific functional responses. But exactly where and how cAMP signaling is confined is not fully understood. Different receptors and adenylyl cyclase isoforms responsible for cAMP production are not uniformly distributed between lipid raft and non-lipid raft domains of the plasma membrane. We sought to determine the role that these membrane domains play in organizing cAMP responses in HEK293 cells. The freely diffusible FRET-based biosensor Epac2-camps was used to measure global cAMP responses, while versions of the probe targeted to lipid raft (Epac2-MyrPalm) and non-raft (Epac2-CAAX) domains were used to monitor local cAMP production near the plasma membrane. Disruption of lipid rafts by cholesterol depletion selectively altered cAMP responses produced by raft-associated receptors. The results indicate that receptors associated with lipid raft as well as non-lipid raft domains can contribute to global cAMP responses. In addition, basal cAMP activity was found to be significantly higher in non-raft domains. This was supported by the fact that pharmacologic inhibition of adenylyl cyclase activity reduced basal cAMP activity detected by Epac2-CAAX but not Epac2-MyrPalm or Epac2-camps. Responses detected by Epac2-CAAX were also more sensitive to direct stimulation of adenylyl cyclase activity, but less sensitive to inhibition of phosphodiesterase activity. Quantitative modeling was used to demonstrate that differences in adenylyl cyclase and phosphodiesterase activities are necessary but not sufficient to explain compartmentation of cAMP associated with different microdomains of the plasma membrane.
KW  - protein-coupled-receptors
KW  - adenylyl-cyclase isoforms
KW  - adult cardiac myocytes
KW  - plasma membrane
KW  - lipid rafts
KW  - cholesterol depletion
KW  - BETA(2)-adrenergic receptor
KW  - living vells
KW  - cyclic-AMP
KW  - domains
Y1  - 2014
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-116673
SN  - 1932-6203
VL  - 9
IS  - 4
ER  - 
TY  - JOUR
A1  - Afonso-Grunz, Fabian
A1  - Hoffmeier, Klaus
A1  - Müller, Sören
A1  - Westermann, Alexander J.
A1  - Rotter, Björn
A1  - Vogel, Jörg
A1  - Winter, Peter
A1  - Kahl, Günter
T1  - Dual 3'Seq using deepSuperSAGE uncovers transcriptomes of interacting Salmonella enterica Typhimurium and human host cells
JF  - BMC Genomics
N2  - Background: 
The interaction of eukaryotic host and prokaryotic pathogen cells is linked to specific changes in the cellular proteome, and consequently to infection-related gene expression patterns of the involved cells. To simultaneously assess the transcriptomes of both organisms during their interaction we developed dual 3'Seq, a tag-based sequencing protocol that allows for exact quantification of differentially expressed transcripts in interacting pro-and eukaryotic cells without prior fixation or physical disruption of the interaction. 

Results: 
Human epithelial cells were infected with Salmonella enterica Typhimurium as a model system for invasion of the intestinal epithelium, and the transcriptional response of the infected host cells together with the differential expression of invading and intracellular pathogen cells was determined by dual 3'Seq coupled with the next-generation sequencing-based transcriptome profiling technique deepSuperSAGE (deep Serial Analysis of Gene Expression). Annotation to reference transcriptomes comprising the operon structure of the employed S. enterica Typhimurium strain allowed for in silico separation of the interacting cells including quantification of polycistronic RNAs. Eighty-nine percent of the known loci are found to be transcribed in prokaryotic cells prior or subsequent to infection of the host, while 75% of all protein-coding loci are represented in the polyadenylated transcriptomes of human host cells.

Conclusions: 
Dual 3'Seq was alternatively coupled to MACE (Massive Analysis of cDNA ends) to assess the advantages and drawbacks of a library preparation procedure that allows for sequencing of longer fragments. Additionally, the identified expression patterns of both organisms were validated by qRT-PCR using three independent biological replicates, which confirmed that RELB along with NFKB1 and NFKB2 are involved in the initial immune response of epithelial cells after infection with S. enterica Typhimurium.
KW  - complete genome sequence
KW  - secretion systems
KW  - RNA-Seq
KW  - deepSuperSAGE
KW  - transcriptome
KW  - gene expression
KW  - serovar Typhimurium
KW  - human macrophages
KW  - epithelial cells
KW  - infection
KW  - SuperSAGE
KW  - receptors
KW  - Dual 3'seq
KW  - MACE
KW  - tag based
KW  - simultaneous
KW  - genome wide
KW  - gene expression profiling
KW  - host pathogen interaction
KW  - Salmonella enterica Typhimurium strain SL1344
Y1  - 2015
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-143230
VL  - 16
IS  - 323
ER  - 
TY  - THES
A1  - Afify, Samar
T1  - Drug targeting delivery systems for treatment of Raf-1 induced lung tumors in mice
T1  - Trägersystem der Medikamente für Raf1- induzierte Lungentumor in Mäusen anzuzielen
N2  - The aim of the present study was to design different dosage forms as carrier systems to deliver sorafenib to the lung of BXB-23 transgenic mice using different routes of administration. Three dosage forms were used one of them was an oil-in-water emulsion and the oral route was chosen for this experiment. The other delivery system was a liposome preparation for intratracheal instillation. In this case the oral route was considered as a control experiment. The last dosage form was PLGA microspheres. Before sorafenib administration it was important to develop a HPLC method to assess sorafenib absorption after its administration and to determine its concentrations in mouse serum. The HPLC method allowed sorafenib quantification in small volumes (30 µl) of mouse serum and tissues. The developed HPLC method was validated resulting in satisfactory selectivity, good linearity, good accuracy and precision over the concentration range examined. Sorafenib was successfully incorporated in a fat emulsion (o/w) using a traditional method resulting in a white homogenous emulsion and no particle aggregation was observed. Sorafenib exhibited antitumor activity on the lung adenoma in BXB-23 transgenic mice when administered orally (2 mg sorafenib per mouse) in the emulsion preparation. The determined effect was an approximately 29 % reduction in the tumor area of the adenoma foci and a proliferation reduction. In order to improve the pharmacological effects of sorafenib on the lung adenoma in BXB-23 mice, the targeting of sorafenib directly to the site of action (the lung) was an attractive concept. For this purpose the intratracheal route was used. Since sorafenib administration by instillation required incorporation of sorafenib in a dosage form suitable for its lipophilic nature, a liposome suspension was the second dosage form used. A lyophilization method was employed for sorafenib liposome preparation utilizing dilauroylphosphatidylcholine (DLPC) which is safe and tolerable for the lung. Incorporation of sorafenib in the liposomes did not influence the particle size and its distribution. The sorafenib liposomes showed high encapsulation efficiency, good stability at 4 °C for one month and satisfactory in vitro release properties and inhibited Raf-1 mediated activation of ERK in cell culture assay. In a pharmacokinetic experiment sorafenib loaded liposomes were instilled directly into the lung. The results revealed that a significant level of sorafenib was achieved in the lung tissues after 2 hours and then reduced after 48 h and remained nearly constant for one week. On the other hand, only traces of sorafenib were found in the mice serum up to 48 h. Subsequently, the pharmacological activity of sorafenib (1 mg per mouse) was studied when delivered in a liposomal suspension intratracheally to treat the lung adenoma of BXB-23 mice. The data of this experiment demonstrated that sorafenib intratracheal instillation resulted in a reduction of tumor area of adenoma foci (67 %) and an elevation of the percent of apoptotic cells. In contrast, prolongation of the treatment period did not further enhance sorafenib activity on the lung adenoma. This previous finding suggested a development of multidrug resistance (MDR) by the adenoma foci cells against sorafenib instillation, which was examined by immunohistochemistry staining. The percent of MDR positive cells was higher after two and three weeks sorafenib liposome instillation treatment than that after one week treatment. The last dosage form used for sorafenib was microspheres, which were prepared by emulsion-diffusion-evaporation method using biodegradable PLGA 50:50 resulting in a white lyophilized powder. The system was characterized physicochemically and revealed a good microspheres yield, high encapsulation efficiency, a homogenous particle size distribution and slow in vitro release of sorafenib. The other strategy studied in the present research project was gene delivery to target the lung bearing tumor of BXB-23 mice using a non-viral vector (polyethylenimine). Polyethylenimine (PEI) was used to investigate its efficiency in transfecting lung bearing tumor of BXB-23 mice model and its ability to transfect the adenoma foci cells. LacZ, which encodes Beta-galactosidase was used in the present study as a reporter gene and was complexed with PEI before delivered intravenously. A high LacZ expression in the alveolar region with some expression in the adenoma foci was observed. On contrary, a low LacZ expression in the alveoli and in the adenoma foci was achieved after instillation of the same polyplex intratracheally.
N2  - Das Ziel der vorliegenden Dissertation war es, verschiedene galenische Darreichungsformen als Trägersystem für Sorafenib zu entwickeln, um den direkten Transport des Arzneistoffes zum Zielorgan Lunge von BXB-23 transgenen Mäusen zu ermöglichen. Für die verschiedenen Applikationswege wurden drei Darreichungsformen gewählt. Eine Öl-in-Wasser-Emulsion sollte oral verabreicht werden. Für die intratracheale Instillation wurde ein liposomales Präparat gewählt. Die letzte Darreichungsform stellten PLGA Mikrosphären dar. Um die Absorption von Sorafenib nach Administration bestimmen zu können, wurde die Konzentration des Arzneistoffes im Mäuseserum gemessen. Zur Quantifizierung von Sorafenib in einem geringen Volumen Serum und in Gewebe wurde eine HPLC-Methode entwickelt und validiert. Sorafenib wurde erfolgreich in eine Fettemulsion (o/w) mittels einer traditionellen Methode eingearbeitet. Nach oraler Verabreichung der Emulsion (2 mg/Maus) zeigte Sorafenib auf Lungenadenome eine Antitumor-Aktivität, wobei eine Reduktion der Tumorfläche der Adenomfoci um etwa 29 % und eine Reduktion der Proliferation verzeichnet werden konnte. Zur Verbesserung der pharmakologischen Effekte von Sorafenib auf die Lungenadenome in BXB-23 Mäusen zu verbessern, sollte Sorafenib direkt dem Zielorgan Lunge zugeführt werden. Zu diesem Zweck wurde der intratracheale Administrationsweg gewählt. Da die Instillation von Sorafenibaufgrund seiner lipophilen Natur nur durch Einschluß in eine andere Darreichungsform zu erreichen ist, wurde für die zweite Darreichungsform eine Liposomen-Suspension verwendet. Für die Zubereitung von Sorafenib in Liposomen wurde eine Lyophilisierungsmethode unter Verwendung von DPLC erarbeitet. Die Einschluss-Effektivität der Sorafenib-beladenen Liposomen war hoch und zeigte bei 4°C eine gute Stabilität für einen Monat. Die erzielten Effekte bei der in vitro Freisetzung und die Hemmung der von Raf1-induzierten Aktivierung von ERK in Zellkulturexperimenten lieferten zufrieden stellende Ergebnisse. In einem pharmakokinetischen Experiment wurden mit Sorafenib beladenen Liposomen direkt in die Lunge appliziert. Die Ergebnisse zeigten, dass nach 2 h eine signifikante Konzentration von Sorafenib im Lungengewebe erreicht wurde. Nach 48 h nahm diese Konzentration ab und blieb dann für eine Woche fast konstant. Andererseits wurden bis zu 48 h nach Gabe des Arzneistoffes nur Spuren von Sorafenib im Mäuseserum gefunden. Folglich wurde die pharmakologische Aktivität von Sorafenib (1 mg/Maus) bei intratrachealer Verabreichung in einer liposomalen Suspension untersucht. Die Ergebnisse zeigten, dass die intratracheale Gabe von Sorafenib eine Reduktion der Tumorfläche der Adenomfoci um 67 % bewirkte, sowie eine Erhöhung des prozentualen Anteils apoptotischer Zellen. Eine Verlängerung der Behandlungszeit zeigte keine zusätzliche Verbesserung der Effekte. Dies lies vermuten, dass hier eine Entwicklung von Multidrug-Resistenz in den Adenomfocizellen gegenüber der Instillation von Sorafenib erfolgte. Dies wurde in immunochemischen Anfärbe-Experimenten untersucht. Die Prozentzahl von MDR-positiven Zellen war nach zwei und drei Wochen Instillation von Sorafenib-Liposomen höher als nach einer Woche. Die letzte verwendete Darreichungsform für Sorafenib waren Mikrosphären, die durch Emulsions-Diffusions-Evaporations-Methoden in biologisch abbaubarem PLGA 50:50 hergestellt wurden. Dies ergab ein weißes, lyophilisiertes Pulver. Das System wurde physiochemisch charakterisiert und ergab ein gutes Mikrosphären-Ergebnis, hohe Einschluss-Effektivität, eine homogene Verteilung der Partikelgrößen und eine langsame in vitro Freisetzung von Sorafenib. Die andere untersuchte Strategie war Gen-Delivery, um den Lungentumor von BXB-23 Mäusen mittels eines nicht-viralen Vektors (Polyethylenimin, PEI) anzuzielen. PEI wurde verwendet, um die Effektivität der Transfektion des Lungentumors zu untersuchen und seine Fähigkeit, die Adenomfocizellen zu transfizieren. LacZ, das Beta-Galactosidase codiert, diente bei diesem Experiment als Reportergen und wurde vor intravenöser Gabe mit PEI komplexiert. Eine hohe LacZ-Expression in der alveolaren Region, aber nur eine geringe Expression in den Adenomfoci wurde beobachtet. Im Gegensatz dazu wurde eine geringe Expression von LacZ in den Alveolen und den Adenomfoci nach intratrachealer Instillation des gleichen Polyplex erreicht.
KW  - Maus
KW  - Transgene Tiere
KW  - Targeted drug delivery
KW  - Lungenkrebs
KW  - Sorafenib
KW  - Liposomen
KW  - MDR
KW  - Mikrosphären
KW  - Antitumor
KW  - Sorafenib
KW  - liposomes
KW  - MDR
KW  - microspheres
KW  - Antitumor
Y1  - 2007
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-22249
ER  - 
TY  - JOUR
A1  - Aeschlimann, Martin
A1  - Brixner, Tobias
A1  - Cinchetti, Mirko
A1  - Frisch, Benjamin
A1  - Hecht, Bert
A1  - Hensen, Matthias
A1  - Huber, Bernhard
A1  - Kramer, Christian
A1  - Krauss, Enno
A1  - Loeber, Thomas H.
A1  - Pfeiffer, Walter
A1  - Piecuch, Martin
A1  - Thielen, Philip
T1  - Cavity-assisted ultrafast long-range periodic energy transfer between plasmonic nanoantennas
JF  - Light: Science & Applications
N2  - Radiationless energy transfer is at the core of diverse phenomena, such as light harvesting in photosynthesis\(^1\), energy-transfer-based microspectroscopies\(^2\), nanoscale quantum entanglement\(^3\) and photonic-mode hybridization\(^4\). Typically, the transfer is efficient only for separations that are much shorter than the diffraction limit. This hampers its application in optical communication and quantum information processing, which require spatially selective addressing. Here, we demonstrate highly efficient radiationless coherent energy transfer over a distance of twice the excitation wavelength by combining localized and delocalized\(^5\) plasmonic modes. Analogous to the Tavis-Cummings model, two whispering-gallery-mode antennas\(^6\) placed in the foci of an elliptical plasmonic cavity\(^7\) fabricated from single-crystal gold plates act as a pair of oscillators coupled to a common cavity mode. Time-resolved two-photon photoemission electron microscopy (TR 2P-PEEM) reveals an ultrafast long-range periodic energy transfer in accordance with the simulations. Our observations open perspectives for the optimization and tailoring of mesoscopic energy transfer and long-range quantum emitter coupling.
KW  - chemistry
KW  - nanocavities
KW  - nanophotonics and plasmonics
KW  - photonic devices
Y1  - 2017
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-173265
VL  - 6
ER  - 
TY  - JOUR
A1  - Aeschlimann, Martin
A1  - Bauer, Michael
A1  - Bayer, Daniela
A1  - Brixner, Tobias
A1  - Cunovic, Stefan
A1  - Fischer, Alexander
A1  - Melchior, Pascal
A1  - Pfeiffer, Walter
A1  - Rohmer, Martin
A1  - Schneider, Christian
A1  - Strüber, Christian
A1  - Tuchscherer, Philip
A1  - Voronine, Dimitri V.
T1  - Optimal open-loop near-field control of plasmonic nanostructures
N2  - Optimal open-loop control, i.e. the application of an analytically derived control rule, is demonstrated for nanooptical excitations using polarization-shaped laser pulses. Optimal spatial near-field localization in gold nanoprisms and excitation switching is realized by applying a shift to the relative phase of the two polarization components. The achieved near-field switching confirms theoretical predictions, proves the applicability of predefined control rules in nanooptical light–matter interaction and reveals local mode interference to be an important control mechanism.
KW  - Chemie
Y1  - 2012
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-75256
ER  - 
TY  - JOUR
A1  - Aerts, An
A1  - Eberlein, Uta
A1  - Holm, Sören
A1  - Hustinx, Roland
A1  - Konijnenberg, Mark
A1  - Strigari, Lidia
A1  - van Leeuwen, Fijs W. B.
A1  - Glatting, Gerhard
A1  - Lassmann, Michael
T1  - EANM position paper on the role of radiobiology in nuclear medicine
JF  - European Journal of Nuclear Medicine and Molecular Imaging
N2  - With an increasing variety of radiopharmaceuticals for diagnostic or therapeutic nuclear medicine as valuable diagnostic or treatment option, radiobiology plays an important role in supporting optimizations. This comprises particularly safety and efficacy of radionuclide therapies, specifically tailored to each patient. As absorbed dose rates and absorbed dose distributions in space and time are very different between external irradiation and systemic radionuclide exposure, distinct radiation-induced biological responses are expected in nuclear medicine, which need to be explored. This calls for a dedicated nuclear medicine radiobiology. Radiobiology findings and absorbed dose measurements will enable an improved estimation and prediction of efficacy and adverse effects. Moreover, a better understanding on the fundamental biological mechanisms underlying tumor and normal tissue responses will help to identify predictive and prognostic biomarkers as well as biomarkers for treatment follow-up. In addition, radiobiology can form the basis for the development of radiosensitizing strategies and radioprotectant agents. Thus, EANM believes that, beyond in vitro and preclinical evaluations, radiobiology will bring important added value to clinical studies and to clinical teams. Therefore, EANM strongly supports active collaboration between radiochemists, radiopharmacists, radiobiologists, medical physicists, and physicians to foster research toward precision nuclear medicine.
KW  - radionuclide therapy
KW  - radiobiology
KW  - dosimetry
KW  - biodosimetry
KW  - biomarkers
Y1  - 2021
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-265595
VL  - 48
IS  - 11
ER  - 
TY  - JOUR
A1  - Adrián-Martínez, S.
A1  - Albert, A.
A1  - André, M.
A1  - Anton, G.
A1  - Ardid, M.
A1  - Aubert, J.-J.
A1  - Avgitas, T.
A1  - Baret, B.
A1  - Barrios-Martí, J.
A1  - Basa, S.
A1  - Bertin, V.
A1  - Biagi, S.
A1  - Bormuth, R.
A1  - Bouwhuis, M.C.
A1  - Bruijn, R.
A1  - Brunner, J.
A1  - Busto, J.
A1  - Capone, A.
A1  - Caramete, L.
A1  - Carr, J.
A1  - Celli, S.
A1  - Chiarusi, T.
A1  - Circella, M.
A1  - Coleiro, A.
A1  - Coniglione, R.
A1  - Costantini, H.
A1  - Coyle, P.
A1  - Creusot, A.
A1  - Deschamps, A.
A1  - De Bonis, G.
A1  - Distefano, C.
A1  - Donzaud, C.
A1  - Dornic, D.
A1  - Drouhin, D.
A1  - Eberl, T.
A1  - El Bojaddaini, I.
A1  - Elsässer, D.
A1  - Enzenhöfer, A.
A1  - Fehn, K.
A1  - Felis, I.
A1  - Fusco, L.A.
A1  - Galatà, S.
A1  - Gay, P.
A1  - Geißelsöder, S.
A1  - Geyer, K.
A1  - Giordano, V.
A1  - Gleixner, A.
A1  - Glotin, H.
A1  - Gracia-Ruiz, R.
A1  - Graf, K.
A1  - Hallmann, S.
A1  - van Haren, H.
A1  - Heijboer, A.J.
A1  - Hello, Y.
A1  - Hernández-Rey, J.J.
A1  - Hößl, J.
A1  - Hofestädt, J.
A1  - Hugon, C.
A1  - Illuminati, G.
A1  - James, C.W.
A1  - de Jong, M.
A1  - Jongen, M.
A1  - Kadler, M.
A1  - Kalekin, O.
A1  - Katz, U.
A1  - Kießling, D.
A1  - Kouchner, A.
A1  - Kreter, M.
A1  - Kreykenbohm, I.
A1  - Kulikovskiy, V.
A1  - Lachaud, C.
A1  - Lahmann, R.
A1  - Lefèvre, D.
A1  - Leonora, E.
A1  - Loucatos, S.
A1  - Marcelin, M.
A1  - Margiotta, A.
A1  - Marinelli, A.
A1  - Martínez-Mora, J.A.
A1  - Mathieu, A.
A1  - Melis, K.
A1  - Michael, T.
A1  - Migliozzi, P.
A1  - Moussa, A.
A1  - Mueller, C.
A1  - Nezri, E.
A1  - Pavalas, G.E.
A1  - Pellegrino, C.
A1  - Perrina, C.
A1  - Piattelli, P.
A1  - Popa, V.
A1  - Pradier, T.
A1  - Racca, C.
A1  - Riccobene, G.
A1  - Roensch, K.
A1  - Saldaña, M.
A1  - Samtleben, D.F.E.
A1  - Sánchez-Losa, A.
A1  - Sanguineti, M.
A1  - Sapienza, P.
A1  - Schnabel, J.
A1  - Schüssler, F.
A1  - Seitz, T.
A1  - Sieger, C.
A1  - Spurio, M.
A1  - Stolarczyk, Th.
A1  - Taiuti, M.
A1  - Tönnis, C.
A1  - Trovato, A.
A1  - Tselengidou, M.
A1  - Turpin, D.
A1  - Vallage, B.
A1  - Vallée, C.
A1  - Van Elewyck, V.
A1  - Vivolo, D.
A1  - Wagner, S.
A1  - Wilms, J.
A1  - Zornoza, J.D.
A1  - Zúñiga, J.
T1  - Limits on dark matter annihilation in the sun using the ANTARES neutrino telescope
JF  - Physics Letters B
N2  - A search for muon neutrinos originating from dark matter annihilations in the Sun is performed using the data recorded by the ANTARES neutrino telescope from 2007 to 2012. In order to obtain the best possible sensitivities to dark matter signals, an optimisation of the event selection criteria is performed taking into account the background of atmospheric muons, atmospheric neutrinos and the energy spectra of the expected neutrino signals. No significant excess over the background is observed and 90% C.L. upper limits on the neutrino flux, the spin-dependent and spin-independent WIMP-nucleon cross-sections are derived for WIMP masses ranging from 50 GeV to 5 TeV for the annihilation channels WIMP + WIMP→ b\(\overline{b}\), W\(^{+}\)W\(^{−}\) and τ\(^{+}\)τ\(^{−}\).
KW  - dark matter
KW  - WIMP
KW  - neutralino
KW  - indirect detection
KW  - neutrino telescope
KW  - sun
Y1  - 2016
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-166642
VL  - 759
ER  - 
TY  - JOUR
A1  - Adrián-Martínez, S.
A1  - Albert, A.
A1  - André, M.
A1  - Anton, G.
A1  - Ardid, M.
A1  - Aubert, J.-J.
A1  - Avgitas, T.
A1  - Baret, B.
A1  - Barrios-Martí, J.
A1  - Basa, S.
A1  - Bertin, V.
A1  - Biagi, S.
A1  - Bormuth, R.
A1  - Bou-Cabo, M.
A1  - Bouwhuis, M.C.
A1  - Bruijn, R.
A1  - Brunner, J.
A1  - Busto, J.
A1  - Capone, A.
A1  - Caramete, L.
A1  - Carr, J.
A1  - Celli, S.
A1  - Chiarusi, T.
A1  - Circella, M.
A1  - Coleiro, A.
A1  - Coniglione, R.
A1  - Costantini, H.
A1  - Coyle, P.
A1  - Creusot, A.
A1  - Deschamps, A.
A1  - De Bonis, G.
A1  - Distefano, C.
A1  - Donzaud, C.
A1  - Dornic, D.
A1  - Drouhin, D.
A1  - Eberl, T.
A1  - El Bojaddaini, I.
A1  - Elsässer, D.
A1  - Enzenhöfer, A.
A1  - Fehn, K.
A1  - Felis, I.
A1  - Fusco, L.A.
A1  - Galatà, S.
A1  - Gay, P.
A1  - Geißelsöder, S.
A1  - Geyer, K.
A1  - Giordano, V.
A1  - Gleixner, A.
A1  - Glotin, H.
A1  - Gracia-Ruiz, R.
A1  - Graf, K.
A1  - Hallmann, S.
A1  - van Haren, H.
A1  - Heijboer, A.J.
A1  - Hello, Y.
A1  - Hernández-Rey, J.-J.
A1  - Hößl, J.
A1  - Hofestädt, J.
A1  - Hugon, C.
A1  - Illuminati, G.
A1  - James, C.W.
A1  - de Jong, M.
A1  - Kadler, M.
A1  - Kalekin, O.
A1  - Katz, U.
A1  - Kießling, D.
A1  - Kouchner, A.
A1  - Kreter, M.
A1  - Kreykenbohm, I.
A1  - Kulikovskiy, V.
A1  - Lachaud, C.
A1  - Lahmann, R.
A1  - Lefèvre, D.
A1  - Leonora, E.
A1  - Loucatos, S.
A1  - Marcelin, M.
A1  - Margiotta, A.
A1  - Marinelli, A.
A1  - Martínez-Mora, J.A.
A1  - Mathieu, A.
A1  - Michael, T.
A1  - Migliozzi, P.
A1  - Moussa, A.
A1  - Mueller, C.
A1  - Nezri, E.
A1  - Păvălaș, G.E.
A1  - Pellegrino, C.
A1  - Perrina, C.
A1  - Piattelli, P.
A1  - Popa, V.
A1  - Pradier, T.
A1  - Racca, C.
A1  - Riccobene, G.
A1  - Roensch, K.
A1  - Saldaña, M.
A1  - Samtleben, D.F.E.
A1  - Sanguineti, M.
A1  - Sapienza, P.
A1  - Schnabel, J.
A1  - Schüssler, F.
A1  - Seitz, T.
A1  - Sieger, C.
A1  - Spurio, M.
A1  - Stolarczyk, Th.
A1  - Sánchez-Losa, A.
A1  - Taiuti, M.
A1  - Trovato, A.
A1  - Tselengidou, M.
A1  - Turpin, D.
A1  - Tönnis, C.
A1  - Vallage, B.
A1  - Vallée, C.
A1  - Van Elewyck, V.
A1  - Vivolo, D.
A1  - Wagner, S.
A1  - Wilms, J.
A1  - Zornoza, J.D.
A1  - Zúñiga, J.
T1  - A search for Secluded Dark Matter in the Sun with the ANTARES neutrino telescope
JF  - Journal of Cosmology and Astroparticle Physics
N2  - A search for Secluded Dark Matter annihilation in the Sun using 2007-2012 data of the ANTARES neutrino telescope is presented. Three different cases are considered: a) detection of dimuons that result from the decay of the mediator, or neutrino detection from: b) mediator that decays into a dimuon and, in turn, into neutrinos, and c) mediator that decays directly into neutrinos. As no significant excess over background is observed, constraints are derived on the dark matter mass and the lifetime of the mediator.
KW  - dark matter experiments
KW  - neutrino detectors
KW  - dark matter detectors
KW  - neutrino astronomy
Y1  - 2016
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-189035
VL  - 2016
IS  - 5
ER  - 
TY  - JOUR
A1  - Adrián-Martínez, S.
A1  - Albert, A.
A1  - André, M.
A1  - Anghinolfi, M.
A1  - Anton, G.
A1  - Ardid, M.
A1  - Aubert, J.-J.
A1  - Baret, B.
A1  - Barrios-Marti, J.
A1  - Basa, S.
A1  - Bertin, V.
A1  - Biagi, S.
A1  - Bormuth, R.
A1  - Bouwhuis, M.C.
A1  - Bruijn, R.
A1  - Brunner, J.
A1  - Buto, J.
A1  - Capone, A.
A1  - Caramete, L.
A1  - Carr, J.
A1  - Chiarusi, T.
A1  - Circella, M.
A1  - Coniglione, R.
A1  - Costantini, H.
A1  - Coyle, P.
A1  - Creusot, A.
A1  - Dekeyser, I.
A1  - Deschamps, A.
A1  - De Bonis, G.
A1  - Distefano, C.
T1  - Stacked search for time shifted high energy neutrinos from gamma ray bursts with the ANTARES neutrino telescope
JF  - European Physical Journal C
N2  - A search for high-energy neutrino emission correlated with gamma-ray bursts outside the electromagnetic prompt-emission time window is presented. Using a stacking approach of the time delays between reported gamma-ray burst alerts and spatially coincident muon-neutrino signatures, data from the Antares neutrino telescope recorded between 2007 and 2012 are analysed. One year of public data from the IceCube detector between 2008 and 2009 have been also investigated. The respective timing profiles are scanned for statistically significant accumulations within 40 days of the Gamma Ray Burst, as expected from Lorentz Invariance Violation effects and some astrophysical models. No significant excess over the expected accidental coincidence rate could be found in either of the two data sets. The average strength of the neutrino signal is found to be fainter than one detectable neutrino signal per hundred gamma-ray bursts in the Antares data at 90% confidence level.
KW  - Search window
KW  - Neutrino data
KW  - Neutrino telescope
KW  - Neutrino emission
KW  - Accidental coincidence
KW  - Gamma-ray bursts
Y1  - 2017
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-181251
VL  - 77
IS  - 1
ER  - 
TY  - JOUR
A1  - Adrián-Martínez, S.
A1  - Albert, A.
A1  - André, M.
A1  - Anghinolfi, M.
A1  - Anton, G.
A1  - Ardid, M.
A1  - Aubert, J.-J.
A1  - Avgitas, T.
A1  - Baret, B.
A1  - Barrios-Martí, J.
A1  - Basa, S.
A1  - Bertin, V.
A1  - Biagi, S.
A1  - Bormuth, R.
A1  - Bouwhuis, M.C.
A1  - Bruijn, R.
A1  - Brunner, J.
A1  - Busto, J.
A1  - Capone, A.
A1  - Caramete, L.
A1  - Carr, J.
A1  - Celli, S.
A1  - Chiarusi, T.
A1  - Circella, M.
A1  - Coleiro, A.
A1  - Coniglione, R.
A1  - Constantini, H.
A1  - Coyle, P.
A1  - Creusot, A.
A1  - Deschamps, A.
A1  - De Bonis, G.
A1  - Distefano, C.
A1  - Donzaud, C.
A1  - Dornic, D.
A1  - Drouhin, D.
A1  - Eberl, T.
A1  - El Bojaddaini, I.
A1  - Elsässer, D.
A1  - Enzenhöfer, A.
A1  - Fehn, K.
A1  - Felis, I.
A1  - Fusco, L.A.
A1  - Galatà, S.
A1  - Gay, P.
A1  - Geißelsöder, S.
A1  - Geyer, K.
A1  - Giordano, V.
A1  - Gleixner, A.
A1  - Glotin, H.
A1  - Gracia-Ruiz, R.
A1  - Graf, K.
A1  - Hallmann, S.
A1  - van Haren, H.
A1  - Heijboer, A.J.
A1  - Hello, Y.
A1  - Hernández-Rey, J.J.
A1  - Hößl, J.
A1  - Hofestädt, J.
A1  - Hugon, C.
A1  - Illuminati, G.
A1  - James, C.W.
A1  - de Jong, M.
A1  - Kadler, M.
A1  - Kalekin, O.
A1  - Katz, U.
A1  - Kießling, D.
A1  - Kouchner, A.
A1  - Kreter, M.
A1  - Kreykenbohm, I.
A1  - Kulikovskiy, V.
A1  - Lachaud, C.
A1  - Lahmann, R.
A1  - Lefèvre, D.
A1  - Leonora, E.
A1  - Loucatos, S.
A1  - Marcelin, M.
A1  - Margiotta, A.
A1  - Marinelli, A.
A1  - Martínez-Mora, J.A.
A1  - Mathieu, A.
A1  - Michael, T.
A1  - Migliozzi, P.
A1  - Moussa, A.
A1  - Mueller, C.
A1  - Nezri, E.
A1  - Pavalas, G.E.
A1  - Pellegrino, C.
A1  - Perrina, C.
A1  - Piattelli, P.
A1  - Popa, V.
A1  - Pradier, T.
A1  - Racca, C.
A1  - Riccobene, G.
A1  - Roensch, K.
A1  - Saldaña, M.
A1  - Samtleben, D.F.E.
A1  - Sánchez-Losa, A.
A1  - Sanguineti, M.
A1  - Sapienza, P.
A1  - Schnabel, J.
A1  - Schüssler, F.
A1  - Seitz, T.
A1  - Sieger, C.
A1  - Spurio, M.
A1  - Stolarczyk, Th.
A1  - Taiuti, M.
A1  - Trovato, A.
A1  - Tselengidou, M.
A1  - Turpin, D.
A1  - Tönnis, C.
A1  - Vallage, B.
A1  - Vallée, C.
A1  - Van Elewyck, V.
A1  - Visser, E.
A1  - Vivolo, D.
A1  - Wagner, S.
A1  - Wilms, J.
A1  - Zornoza, J.D.
A1  - Zúñiga, J.
T1  - Constraints on the neutrino emission from the Galactic Ridge with the ANTARES telescope
JF  - Physics Letters B
N2  - A highly significant excess of high-energy astrophysical neutrinos has been reported by the IceCube Collaboration. Some features of the energy and declination distributions of IceCube events hint at a North/South asymmetry of the neutrino flux. This could be due to the presence of the bulk of our Galaxy in the Southern hemisphere. The ANTARES neutrino telescope, located in the Mediterranean Sea, has been taking data since 2007. It offers the best sensitivity to muon neutrinos produced by galactic cosmic ray interactions in this region of the sky. In this letter a search for an extended neutrino flux from the Galactic Ridge region is presented. Different models of neutrino production by cosmic ray propagation are tested. No excess of events is observed and upper limits for different neutrino flux spectral indices Γ are set. For Γ=2.4 the 90% confidence level flux upper limit at 100 TeV for one neutrino flavour corresponds to Φ\(^{1f}_{0}\) (100 TeV) = 2.0 · 10\(^{−17}\) GeV\(^{−1}\) cm\(^{−2}\)s\(^{−1}\)sr\(^{−1}\). Under this assumption, at most two events of the IceCube cosmic candidates can originate from the Galactic Ridge. A simple power-law extrapolation of the Fermi-LAT flux to account for IceCube High Energy Starting Events is excluded at 90% confidence level.
KW  - neutrino emission
KW  - Galactic Ridge
KW  - ANTARES telescope
Y1  - 2016
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-166608
VL  - 760
ER  - 
TY  - JOUR
A1  - Adrián-Martínez, S.
A1  - Ageron, M.
A1  - Aharonian, F.
A1  - Aiello, S.
A1  - Albert, A.
A1  - Ameli, F.
A1  - Annasontzis, E.
A1  - Andre, M.
A1  - Androulakis, G.
A1  - Anghinolfi, M.
A1  - Anton, G.
A1  - Ardid, M.
A1  - Avgitas, T.
A1  - Barbarino, G.
A1  - Baret, B.
A1  - Barrios-Martí, J.
A1  - Belhorma, B.
A1  - Belias, A.
A1  - Berbee, A.
A1  - van den Berg, A.
A1  - Bertin, V.
A1  - Beurthey, S.
A1  - van Beeveren, V.
A1  - Beverini, N.
A1  - Biagi, S.
A1  - Biagioni, A.
A1  - Billault, M.
A1  - Bondì, M.
A1  - Bormuth, R.
A1  - Bouhadef, B.
A1  - Bourlis, G.
A1  - Bourret, S.
A1  - Boutonnet, C.
A1  - Bouwhuis, M.
A1  - Bozza, C.
A1  - Bruijn, R.
A1  - Brunner, J.
A1  - Buis, E.
A1  - Busto, J.
A1  - Cacopardo, G.
A1  - Caillat, L.
A1  - Calmai, M.
A1  - Calvo, D.
A1  - Capone, A.
A1  - Caramete, L.
A1  - Cecchini, S.
A1  - Celli, S.
A1  - Champion, C.
A1  - Cherkaoui El Moursli, R.
A1  - Cherubini, S.
A1  - Chiarusi, T.
A1  - Circella, M.
A1  - Classen, L.
A1  - Cocimano, R.
A1  - Coelho, J. A. B.
A1  - Coleiro, A.
A1  - Colonges, S.
A1  - Coniglione, R.
A1  - Cordelli, M.
A1  - Cosquer, A.
A1  - Coyle, P.
A1  - Creusot, A.
A1  - Cuttone, G.
A1  - D'Amico, A.
A1  - De Bonis, G.
A1  - De Rosa, G.
A1  - De Sio, C.
A1  - Di Capua, F.
A1  - Di Palma, I.
A1  - Díaz García, A. F.
A1  - Distefano, C.
A1  - Donzaud, C.
A1  - Dornic, D.
A1  - Dorosti-Hasankiadeh, Q.
A1  - Drakopoulou, E.
A1  - Drouhin, D.
A1  - Drury, L.
A1  - Durocher, M.
A1  - Eberl, T.
A1  - Eichie, S.
A1  - van Eijk, D.
A1  - El Bojaddaini, I.
A1  - El Khayati, N.
A1  - Elsaesser, D.
A1  - Enzenhöfer, A.
A1  - Fassi, F.
A1  - Favali, P.
A1  - Fermani, P.
A1  - Ferrara, G.
A1  - Filippidis, C.
A1  - Frascadore, G.
A1  - Fusco, L. A.
A1  - Gal, T.
A1  - Galatà, S.
A1  - Garufi, F.
A1  - Gay, P.
A1  - Gebyehu, M.
A1  - Giordano, V.
A1  - Gizani, N.
A1  - Gracia, R.
A1  - Graf, K.
A1  - Grégoire, T.
A1  - Grella, G.
A1  - Habel, R.
A1  - Hallmann, S.
A1  - van Haren, H.
A1  - Harissopulos, S.
A1  - Heid, T.
A1  - Heijboer, A.
A1  - Heine, E.
A1  - Henry, S.
A1  - Hernández-Rey, J. J.
A1  - Hevinga, M.
A1  - Hofestädt, J.
A1  - Hugon, C. M. F.
A1  - Illuminati, G.
A1  - James, C. W.
A1  - Jansweijer, P.
A1  - Jongen, M.
A1  - de Jong, M.
A1  - Kadler, M.
A1  - Kalekin, O.
A1  - Kappes, A.
A1  - Katz, U. F.
A1  - Keller, P.
A1  - Kieft, G.
A1  - Kießling, D.
A1  - Koffeman, E. N.
A1  - Kooijman, P.
A1  - Kouchner, A.
A1  - Kulikovskiy, V.
A1  - Lahmann, R.
A1  - Lamare, P.
A1  - Leisos, A.
A1  - Leonora, E.
A1  - Lindsey Clark, M.
A1  - Liolios, A.
A1  - Llorenz Alvarez, C. D.
A1  - Lo Presti, D.
A1  - Löhner, H.
A1  - Lonardo, A.
A1  - Lotze, M.
A1  - Loucatos, S.
A1  - Maccioni, E.
A1  - Mannheim, K.
A1  - Margiotta, A.
A1  - Marinelli, A.
A1  - Mariş, O.
A1  - Markou, C.
A1  - Martínez-Mora, J. A.
A1  - Martini, A.
A1  - Mele, R.
A1  - Melis, K. W.
A1  - Michael, T.
A1  - Migliozzi, P.
A1  - Migneco, E.
A1  - Mijakowski, P.
A1  - Miraglia, A.
A1  - Mollo, C. M.
A1  - Mongelli, M.
A1  - Morganti, M.
A1  - Moussa, A.
A1  - Musico, P.
A1  - Musumeci, M.
A1  - Navas, S.
A1  - Nicoleau, C. A.
A1  - Olcina, I.
A1  - Olivetto, C.
A1  - Orlando, A.
A1  - Papaikonomou, A.
A1  - Papaleo, R.
A1  - Păvălaş, G. E.
A1  - Peek, H.
A1  - Pellegrino, C.
A1  - Perrina, C.
A1  - Pfutzner, M.
A1  - Piattelli, P.
A1  - Pikounis, K.
A1  - Poma, G. E.
A1  - Popa, V.
A1  - Pradier, T.
A1  - Pratolongo, F.
A1  - Pühlhofer, G.
A1  - Pulvirenti, S.
A1  - Quinn, L.
A1  - Racca, C.
A1  - Raffaelli, F.
A1  - Randazzo, N.
A1  - Rapidis, P.
A1  - Razis, P.
A1  - Real, D.
A1  - Resvanis, L.
A1  - Reubelt, J.
A1  - Riccobene, G.
A1  - Rossi, C.
A1  - Rovelli, A.
A1  - Saldaña, M.
A1  - Salvadori, I.
A1  - Samtleben, D. F. E.
A1  - Sánchez García, A.
A1  - Sánchez Losa, A.
A1  - Sanguineti, M.
A1  - Santangelo, A.
A1  - Santonocito, D.
A1  - Sapienza, P.
A1  - Schimmel, F.
A1  - Schmelling, J.
A1  - Sciacca, V.
A1  - Sedita, M.
A1  - Seitz, T.
A1  - Sgura, I.
A1  - Simeone, F.
A1  - Siotis, I.
A1  - Sipala, V.
A1  - Spisso, B.
A1  - Spurio, M.
A1  - Stavropoulos, G.
A1  - Steijger, J.
A1  - Stellacci, S. M.
A1  - Stransky, D.
A1  - Taiuti, M.
A1  - Tayalati, Y.
A1  - Tézier, D.
A1  - Theraube, S.
A1  - Thompson, L.
A1  - Timmer, P.
A1  - Tönnis, C.
A1  - Trasatti, L.
A1  - Trovato, A.
A1  - Tsirigotis, A.
A1  - Tzamarias, S.
A1  - Tzamariudaki, E.
A1  - Vallage, B.
A1  - Van Elewyk, V.
A1  - Vermeulen, J.
A1  - Vicini, P.
A1  - Viola, S.
A1  - Vivolo, D.
A1  - Volkert, M.
A1  - Voulgaris, G.
A1  - Wiggers, L.
A1  - Wilms, J.
A1  - de Wolf, E.
A1  - Zachariadou, K.
A1  - Zornoza, J. D.
A1  - Zúñiga, J.
T1  - Letter of intent for KM3NeT 2.0
JF  - Journal of Physics G-Nuclear and Particle Physics
N2  - The main objectives of the KM3NeT Collaboration are (i) the discovery and subsequent observation of high-energy neutrino sources in the Universe and (ii) the determination of the mass hierarchy of neutrinos. These objectives are strongly motivated by two recent important discoveries, namely: (1) the high-energy astrophysical neutrino signal reported by IceCube and (2) the sizable contribution of electron neutrinos to the third neutrino mass eigenstate as reported by Daya Bay, Reno and others. To meet these objectives, the KM3NeT Collaboration plans to build a new Research Infrastructure consisting of a network of deep-sea neutrino telescopes in the Mediterranean Sea. A phased and distributed implementation is pursued which maximises the access to regional funds, the availability of human resources and the synergistic opportunities for the Earth and sea sciences community. Three suitable deep-sea sites are selected, namely off-shore Toulon (France), Capo Passero (Sicily, Italy) and Pylos (Peloponnese, Greece). The infrastructure will consist of three so-called building blocks. A building block comprises 115 strings, each string comprises 18 optical modules and each optical module comprises 31 photo-multiplier tubes. Each building block thus constitutes a three-dimensional array of photo sensors that can be used to detect the Cherenkov light produced by relativistic particles emerging from neutrino interactions. Two building blocks will be sparsely configured to fully explore the IceCube signal with similar instrumented volume, different methodology, improved resolution and
KW  - neutrino astronomy
KW  - eutrino physics
KW  - deep sea neutrino telescope
KW  - neutrino mass hierarchy
Y1  - 2016
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-188050
VL  - 43
IS  - 8
ER  -