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Sonstige beteiligte Institutionen
- Fraunhofer-Institut für Silicatforschung ISC (8)
- Helmholtz Institute for RNA-based Infection Research (HIRI) (7)
- Universitätsklinikum Würzburg (5)
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- Technische Hochschule Nürnberg Georg Simon Ohm (3)
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- B-1911-2015 (1)
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- C-2593-2016 (1)
- D-1250-2010 (1)
- D-3057-2014 (1)
- I-5818-2014 (1)
- J-8841-2015 (1)
- M-1240-2017 (1)
- N-2030-2015 (1)
- N-3741-2015 (1)
EU-Project number / Contract (GA) number
- 311781 (1)
- 320377 (1)
- EU (FP7/ 2007-2013) (1)
Background and Aims: PMA is a recently described rare tumor entity occuring most often in young children. Due the worse outcome of PMA-patients as compared to children with pilocytic astrocytoma (PA), it has received a grade II assignment in the latest WHO classification. Nevertheless, increasing evidence suggests that the two tumor types are indeed pathologically and genetically related. The radiological differentiation of PMAs from PAs is challenging and the limited available data could not yet provide unequivocal distinguishing imaging features. Furthermore, it is not completely clarified whether PMA cases are associated with a higher rate of CSF dissemination compared to similarly young patients with PA. The aim of our study was firstly to compare MR/CT imaging features of these tumors, and secondly, to evaluate the occurrence of CSF dissemination.
Material and Methods: The study population included 15 children with PMA and 32 children with PA. A third group consisted of eight children with PAs with focal pilomyxoid features. All cases had been registered in the German multicenter SIOP/HIT-LGG trials. The initial MRIs (and CT scans, if available) at establishing the diagnosis were retrospectively analyzed according to standardized criteria and the findings compared between PMAs and PAs. Furthermore, we compared the occurrence of imaging evidences of CSF tumor dissemination between children with PMA and PA, respectively.
Results: The imaging appearance of PMAs and PAs was very similar. However, PAs tended to show more frequently cystic components (p=0.03). As opposed to PAs, PMAs did not have large tumor cysts. We did not find differences with respect to tumor size and tumor margin. Gadolinium enhancement of PMAs was significantly more frequently homogeneous (p=0.006). PMAs appeared to show more often intratumoral hemorrhages (p=0.047). Furthermore, suprasellar PMAs tended to have a more homogeneus texture on T2-weighted MR images (p=0.026). Within the subgroup < 6 years of age the PMA histology tended to have a larger effect on the occurrence of CSF dissemination than the age (p=0.05 vs.0.12).
Conclusions: Although the radiological appearance of PMAs and PAs is similar, some imaging features, like enhancement pattern or presence of cysts or hemorrhage may help differentiating these low-grade gliomas. Our results corroborate previous scarce data suggesting higher rate of CSF dissemination in PMAs, even in the youngest patient population. Thus, in young children with a chiasmatic-hypothalamic tumor suggestive of a PMA, an intensive search for CSF dissemination along the entire neuraxis should be performed.
In a three-year study the current aeolian transportation processes were examined in a linear dune area previously used for grazing near Nizzana at the Israeli-Egyptian border. The research area was subject to heavy grazing across the border, which led to the total destruction of the natural vegetation in the period of 1967 to 1982. As a consequence, intensified aeolian activity and significant changes of the morphology of the dunes were observed. After the end of the grazingg on the Israeli side, a rapid return of the vegetation in the interdune corridors and on the footslopes of the dunes took place. In addition also a reduction of obviously active areas on the dune crests was observed. The situation on Egyptian territory west the border remained unchanged until today. This study is aimed at understanding the changed aeolian morphodynamics east the border. The emphasis was placed on the investigation of the spatial and temporal distribution of aeolian sand transport as well as on the influencing factors morphology, surface condition and vegetation.
Introduction.
Mobile health (mHealth) integrates mobile devices into healthcare, enabling remote monitoring, data collection, and personalized interventions. Machine Learning (ML), a subfield of Artificial Intelligence (AI), can use mHealth data to confirm or extend domain knowledge by finding associations within the data, i.e., with the goal of improving healthcare decisions. In this work, two data collection techniques were used for mHealth data fed into ML systems: Mobile Crowdsensing (MCS), which is a collaborative data gathering approach, and Ecological Momentary Assessments (EMA), which capture real-time individual experiences within the individual’s common environments using questionnaires and sensors. We collected EMA and MCS data on tinnitus and COVID-19. About 15 % of the world’s population suffers from tinnitus.
Materials & Methods.
This thesis investigates the challenges of ML systems when using MCS and EMA data. It asks: How can ML confirm or broad domain knowledge? Domain knowledge refers to expertise and understanding in a specific field, gained through experience and education. Are ML systems always superior to simple heuristics and if yes, how can one reach explainable AI (XAI) in the presence of mHealth data? An XAI method enables a human to understand why a model makes certain predictions. Finally, which guidelines can be beneficial for the use of ML within the mHealth domain? In tinnitus research, ML discerns gender, temperature, and season-related variations among patients. In the realm of COVID-19, we collaboratively designed a COVID-19 check app for public education, incorporating EMA data to offer informative feedback on COVID-19-related matters. This thesis uses seven EMA datasets with more than 250,000 assessments. Our analyses revealed a set of challenges: App user over-representation, time gaps, identity ambiguity, and operating system specific rounding errors, among others. Our systematic review of 450 medical studies assessed prior utilization of XAI methods.
Results.
ML models predict gender and tinnitus perception, validating gender-linked tinnitus disparities. Using season and temperature to predict tinnitus shows the association of these variables with tinnitus. Multiple assessments of one app user can constitute a group. Neglecting these groups in data sets leads to model overfitting. In select instances, heuristics outperform ML models, highlighting the need for domain expert consultation to unveil hidden groups or find simple heuristics.
Conclusion.
This thesis suggests guidelines for mHealth related data analyses and improves estimates for ML performance. Close communication with medical domain experts to identify latent user subsets and incremental benefits of ML is essential.
Ziel der prospektiven, klinischen und monozentrischen Beobachtungsstudie war es, die Eigenschaften der durch die DC/TMD (Diagnostic Criteria for Temporomandibular Disorders) eingeführten neuen Schemata der Schmerzzeichnung für Patienten mit Gesichtsschmerzen zu untersuchen. Der Fokus lag dabei zum einen auf der Reliabilität der Schmerzzeichnung sowie auf der Korrelation mit dem Grad der Schmerzchronifizierung und einer potentiellen psychischen Störung.
218 Patienten mit orofazialen Schmerzen wurden konsekutiv rekrutiert und bearbeiteten einen Fragebogen mit GCPS V.2, PHQ-9 und der Schmerzzeichnung. Eine Untergruppe füllte den Fragebogen nach einer fünfwöchigen Akupunkturtherapie zur Erhebung einer möglichen Veränderung der Schmerzintensität erneut aus. Eine weitere Untergruppe bearbeitete die Fragebögen erneut am selben Tag. Mit einem mehrschrittigen Auswertungsverfahren wurden alle Schmerzzeichnungen ausgewertet.
Die Studienpopulation bestand mit 77,1% aus weiblichen Patienten. Für 44,5% der Kohorte ergab sich eine durch orofaziale Schmerzen bedingte Beeinträchtigung. Die Auswertungsmethoden der Schmerzzeichnung ergaben starke geschlechtsspezifische Unterschiede. Das laterale Kopfschema wies sowohl für Frauen als auch für Männer mit Schmerzbeeinträchtigung signifikant mehr markierte Regionen auf im Vergleich zu Patienten ohne Schmerzbeeinträchtigung. Männer mit dysfunktionalen Schmerzen zeigten zudem eine signifikant höhere prozentual markierte Schmerzoberfläche. Für die männlichen Patienten zeigte sich außerdem für die Anzahl der Regionen und die prozentuale Markierung einen signifikanten Zusammenhang mit einer depressiven Störung. Für Frauen konnten diesbezüglich kein Zusammenhang festgestellt werden und auch der modifizierte Ransford-Score stellte für beide Geschlechter kein valides Screeninginstrument dar, um psychische Beeinträchtigungen zu identifizieren. Die Wiederholungszuverlässigkeit der Schmerzzeichnung war signifikant hoch für das Kopfschema und das intraorale Schema, nicht aber für das Ganzkörperschema.
Insgesamt erwiesen sich die neuen Schemata der Schmerzzeichnung im Rahmen einer CMD Diagnostik als vorteilhaft. Das Geschlecht des Patienten, schmerzbedingte Funktionsstörungen sowie psychische Beeinträchtigungen beeinflussen die durch die Schmerzzeichnung erzielten Ergebnisse unterschiedlich und bestätigen eine vielschichtige Ätiologie der Erkrankung. Die Ergebnisse verweisen zudem auf die Relevanz einer getrennten Betrachtung der Geschlechter in zukünftigen Studien mit orofazialen Schmerzpatienten. Die Summe aller Regionen des Kopfschemas von lateral könnte hinsichtlich der Einschätzung des Ausmaßes einer Schmerzchronifizierung künftig als Auswertungskriterium der Schmerzzeichnung Anwendung finden.
Viele humane Sarkome sind durch spezifische chromosomale Translokationen oder typische genetische Amplifikationen definiert, welche in der Differentialdiagnostik insbesondere in Fällen, bei denen klinische Daten, Morphologie und Immunhistochemie alleine nicht ausreichend wegweisend sind. Die Formalin-fixiertem Paraffin-eingebetteten (FFPE-) Gewebe von 15 Ewing-Sarkomen, 4 Klarzellsarkomen, 9 Synovialsarkomen, 4 alveolären und 7 embryonalen Rhabdomyosarkomen und 25 Liposarkomen verschiedenen Subtyps wurden mittels Fluoreszenz-in-situ-Hybridisierung (FISH) untersucht um ein Sarkom-spezifisches FISH-Sondenset zur Detektion spezifischer chromosomaler Aberrationen in der Routinediagnostik zu etablieren. Es konnte gezeigt werden, dass die FISH in diesem Aufgabenfeld im Vergleich zur PCR ebenfalls eine hoch effiziente zytogenetische Methode mit hoher Spezifität und hohen positiven Vorhersagewerten mit dem Vorteil der unproblematischen Anwendung an FFPE-Geweben ist. Zur Detektion des Isochromosom 12p , i(12p), als Beispiel für komplexere chromosmale Aberrationen, wurden 7 FFPE-Gewebe aus Keimzelltumoren mit 12p- und 12q-detektierenden FISH-Sonden hybridisiert. Die Detektion des i(12p) konnte im Rahmen dieser Arbeit mittels FISH nicht erreicht werden. Zusammenfassend ist die FISH eine hoch effiziente zytogenetische Methode zur Detektion spezifischer chromosomaler Aberrationen in FFPE-Geweben aus humanen Sarkomen mit hoher Eignung zur Anwendung in der Routinediagnostik.
Die vorliegende Arbeit befasst sich mit den Gerichtsordnungen in würzburgischen Städten des 16.Jahrhunderts. Dabei werden insbesondere die Gerichtsordnungen dargestellt, die unter der Regierung Julius Echters erlassen wurden. So soll versucht werden, die Ordnungen Julius Echters sowohl aus dem alten Herkommen als auch von ihrer Entstehungsgeschichte her zu erklären.
The work presented in this thesis was mainly targeted at exploring the capabilities of evaporation based LC detectors as well as further alternatives for the control of impurities in substances not exhibiting a suitable chromophore for UV-detection. In the course of the work carried out, several new methods for the identification, impurities control and composition testing of APIs were elaborated. An evaporation based detector that entered into the field of pharmaceutical analysis in the recent years was the Evaporative Light Scattering Detector (ELSD). However, non-reproducible spikes were reported when injecting concentrated test solutions as they are usually required for the control of impurities. The reasons, for the appearance of these spikes as well as possibilities for their avoidance were explored in a systematic study. Moreover, the dependence of the detector sensitivity on different eluent composition, eluent flow-rate and ELSD settings was investigated. In the course of the revision of the Ph.Eur. monographs for aspartic acid and alanine, a C18 reversed phase ion-pair LC method using 1 mmol/L of perfluoroheptanoic acid as an ion-pair reagent and a charged aerosol detector (CAD) was developed and fully validated for the purity control of Asp. The method was capable of separating the organic acids and major amino acids known to occur as process related impurities. With a slight modification, the method was also applicable for the purity control of Ala. Based on the developed LC-CAD method for the impurity control of alanine, a comparative study of the performance characteristics of different evaporation based LC detectors, i.e. ELSD, CAD and the recently developed Nano Quantity Analyte Detector (NQAD) was carried out. Additionally, an MS detector and qNMR were included in this study. It was found that the control of impurities in Alanine at an ICH conform level could be ensured using LC coupled to CAD, MSD and NQAD detection as well as by the use of qNMR. In terms of performance, prize and ease of use CAD and NQAD were found to be the most suitable alternatives. In terms of repeatability and sensitivity, the CAD appeared slightly superior to the NQAD. The quality of streptomycin sulfate is not sufficiently controlled by the current Ph.Eur. monograph in that an appropriate test for the control of the related substances is missing. A study was carried out to develop a C18 reversed phase ion-pair LC method using pentafluoropropionic acid as an ion-pair reagent and a CAD for the identification and control of the related substances. The developed method allowed the separation of 21 impurities from streptomycin. Moreover, coupling of the method to MS allowed the identification of the separated impurities. The method was shown to be sufficiently sensitive to control the related substances with a disregard limit of 0.1% as it is normally applied in the Ph.Eur. for products derived from fermentation. Currently, the aescin content of horse-chestnut standardized dry extract is determined using a complex and laborious photometric determination. A more selective LC-UV assay determination for beta-aescin has been proposed for the Ph.Eur. draft monograph of horse-chestnut standardized dry extract. Possibilities were explored to further improve the LC-method using detection by CAD. It was demonstrated that by the use of a modified LC-CAD method several problems related to the differences in the UV-response of the various components contained in the active aescin fraction could be eliminated. Moreover the proposed reference standard strategy was reviewed. Eventually, it was demonstrated on the example of two different clusters of pharmacologically active peptides how low energy collision induced dissociation mass spectrometry (low energy CID-MS) can successfully be used for identification testing in pharmacopoeial monographs. In this respect, the combination of a direct confirmation of the molecular mass via the m/z-ratio of the molecule ions with structural sequence information obtained by low energy CID-MS experiments was found to deliver a higher degree of certainty of the identity of a given substance than the set of tests currently described in the monographs. A significant gain in efficiency and throughput and important reduction of the amount of sample consumed during testing were identified as being additional advantages of this approach. Taken together, it could be demonstrated on various examples how recent technological advancements in the field of analytical chemistry can contribute to improve the quality control of APIs.
Frizzled (FZD) are highly conserved receptors that belong to class F of the G protein-coupled receptor (GPCR) superfamily. They are involved in a great variety of processes during embryonic development, organogenesis, and adult tissue homeostasis. In particular, FZD5 is an important therapeutic target due to its involvement in several pathologies, such as tumorigenesis. Nevertheless, little is known regarding the activation of FZD receptors and the signal initiation, and their GPCR nature has been debated. In order to investigate the activation mechanism of these receptors, FRET (Förster Resonance Energy Transfer)-based biosensors for FZD5 have been developed and characterized. A cyan fluorescent protein (CFP) was fused to the C-terminus of the receptor and the specific FlAsH-binding sequence (CCPGCC) was inserted within the 2nd or the 3rd intracellular loop. Single-cell FRET experiments performed using one of these sensors, V5-mFZD5-FlAsH436-CFP, reported structural rearrangements in FZD5 upon stimulation with the endogenous ligand WNT-5A. These movements are similar to those observed in other GPCRs using the same technique, which suggests an activation mechanism for FZD reminiscent of GPCRs. Furthermore, stimulation of the FZD5 FRET-based sensor with various recombinant WNT proteins in a microplate FRET reader allowed to obtain concentration-response curves for several ligands, being possible to distinguish between full and partial agonists. This technology allowed to address the selectivity between WNTs and FZD5 using a full-length receptor in living cells. In addition, G protein FRET-based sensors revealed that WNT-5A specifically induced Gαq activation mediated by FZD5, but not Gαi activation. Other WNT proteins were also able to induce Gαq activation, but with lower efficacy than WNT-5A. In addition, a dual DAG/calcium sensor further showed that WNT-5A stimulation led to the activation of the Gαq-dependent signaling pathway mediated by FZD5, which outcome was the activation of Protein Kinase C (PKC) and the release of intracellular calcium. Altogether, these data provide evidence that the activation process of FZD5 resembles the general characteristics of class A and B GPCR activation, and this receptor also mediates the activation of the heterotrimeric Gαq protein and its downstream signaling pathway. In addition, the FZD5 receptor FRET-based sensor provides a valuable tool to characterize the pharmacological properties of WNTs and other potential ligands for this receptor.
In this work we wanted to investigate the role of NFATc1 in lymphocyte physiology and in pathological conditions (eg. psoriasis). NFATc1 is part of the signal transduction
pathways that regulates B cells activation and function. NFATc1 has different isoforms that are due to different promoters (P1 and P2), polyadenylation and alternative splicing. Moreover, we tried to elucidate the points of interactions between the NFAT and the NF-κB pathways in
activated B-cell fate. NFAT and NF-κB factors share several properties, such as a similar mode of induction and architecture in their DNA binding domain. We used mice which over-express a constitutive active version of NFATc1/α in their B cells with -or without- an ablated IRF4. IRF4 inhibits cell cycle progression of germinal center B cell-derived Burkitt’s lymphoma cells and
induces terminal differentiation toward plasma cells. Our experiments showed that a ‘double hit’ in factors affecting B cell activation (NFATc1 in this case) and late B cell Differentiation (IRF4 in this case) alter the development of the B cells, lead to increase in their numbers and increase in stimulation induced proliferation. Therefore, the overall picture indicates a link between these 2 genes and probable carcinogenic alterations that may occur in B cells.
We also show that in splenic B cells, c-Rel (of the NF-κB canonical pathway) Support the induction of NFATc1/αA through BCR signals. We also found evidence that the lack of NFATc1 affects the expression of Rel-B (of the NF-κB non-canonical pathway). These data suggest a tight interplay between NFATc1 and NF-κB in B cells, influencing the competence of B cells and their functions in peripheral tissues.
We also used IMQ-induced psoriasis-like inflammation on mice which either lack NFATc1 from B cell. Psoriasis is a systemic chronic immunological disease characterized
primarily by abnormal accelerated proliferation of the skin keratinocytes. In psoriasis, the precipitating event leads to immune cell activation. Our experiments showed that NFATc1 is needed for the development of psoriasis. It also showed that IL-10 is the link that enables NFAT
from altering the B cell compartment (eg Bregs) in order to affect inflammation. The important role of B cell in psoriasis is supported by the flared up psoriasis-like inflammation in mice that lack B cells. Bregs is a special type of B cells that regulate other B cells and T cells; tuning the immunological response through immunomodulatory cytokines.
Das kindliche Glaukom ist eine seltene Erkrankung. Die Patienten müssen ein ganzes Leben lang beobachtet werden. Eine erfolgreiche Operation verlängert zwar die Kontrollintervalle, kann sie aber nicht ersetzen. Ungefähr drei Viertel der Glaukomaugen wurde ein- oder zweimal operiert, bei den übrigen mussten drei Operationen oder mehr pro Auge durchgeführt werden. Der intraokulare Druck ist ein wichtiger Parameter für kurzfristige Kontrollen. Nach erfolgreicher Operation sinkt der intraokulare Druck unter 21 mmHg bei 72,1% der Glaukomaugen ohne Medikamente und bei 95,6% mit Medikamenten. Die Achsenlänge ist ein wichtiger Parameter für die langfristige Kontrolle. Der Unterschied zwischen der Achsenlänge der Glaukomaugen und dem altersentsprechenden Normwert blieb bei allen untersuchten Glaukomaugen signifikant, ebenso beim unilateralen kindlichen Glaukom zwischen Achsenlänge der Glaukomaugen und ihren Partneraugen. Bei operierten Glaukomaugen verläuft die Achsenlänge mit zunehmendem Alter ungefähr parallel zur Normkurve mit einem mittleren Unterschied von 1,8 ± 1,2 mm. Der Unterschied zwischen dem Hornhautdurchmesser der Glaukomaugen bei der ersten und letzten Untersuchung ist nicht signifikant. Die Werte des Hornhautdurchmessers zeigen mit zunehmendem Alter einen horizontalen Verlauf, insbesondere nach dem ersten Lebensjahr. Beim unilateralen kindlichen Glaukom verläuft der Hornhautdurchmesser parallel zum Hornhautdurchmesser der Partneraugen mit einem mittleren Unterschied von 1,0 ± 0,6 mm. Trotz eines Visus von 0,32 oder besser bei mehr als der Hälfte der Glaukomaugen blieb die Sehschärfe außerhalb des unteren Normbereichs. Zwei Drittel der unilateralen kindlichen Glaukomaugen zeigten bei der letzten Untersuchung eine Amblyopie von 2 Visusstufen oder mehr. Die Myopie ist der häufigste Refraktionsfehler. Ein Drittel der Glaukompatienten entwickelten einen Strabismus. Die Anisometropie ist der häufigste Grund der Okklusion bei der Mehrzahl der Glaukompatienten mit oder ohne Strabismus. Intaktes Stereosehen ist bei mehr als der Hälfte der Patienten nachweisbar. Die Korrelation zwischen IOD und Achsenlänge bei der letzten Untersuchung ist deutlich signifikant. Eine Abnahme der Achsenlänge während der Verlaufsbeobachtung wurde nur bei Augen mit IOD niedriger als 17 mmHg beobachtet. Die Achsenlänge wies eine signifikante Korrelation zu Visus und Myopie auf. Die Korrelation zum Hornhautdurchmesser war nur bei der Erstuntersuchung signifikant. Ein Hornhautdurchmesser mehr als oder 14 mm, eine mittlere bis höhergradige Myopie und ein Visus von weniger als oder 0,16 wurden häufiger festgestellt, wenn die Achsenlänge 24,5 mm überschritt. Der Visus mehr als oder 1,0 wurde nur bei Achsenlänge niedriger als oder 24,5 mm erreicht. Die Achsenlänge erwies sich gegenüber den Hornhautdurchmesser als der sicherere Parameter in der Diagnostik und der Verlaufskontrolle des kindlichen Glaukoms.
Basierend auf dem Auslauftrichter nach DIN ISO 4324 wurde ein neuartiges Gerät zur Bestimmung der Fließeigenschaften von Schüttgütern entwickelt. Der modifizierte Auslauftrichter zerstört mit Hilfe eines speziellen Rührwerkzeuges ausflussverhindernde Schüttgutbrücken. Durch Charakterisierung des Ausflussverhaltens eines Modellschüttgutes (Aerosil 200/Maisstärke) konnten verschiedene Prozessparameter identifiziert werden, die eine Abhängigkeit von unterschiedlichen Fließeigenschaften des Modellschüttgutes aufweisen. Mit Hilfe des modifizierten Auslauftrichters wurden im weiteren Teil dieser Arbeit binäre Mischungen aus einem Fließregulierungsmittel und Maisstärke auf ihr Fließverhalten untersucht. Hierdurch konnte eine Aussage über das fließregulierende Potential der Nanomaterialien erhalten werden. Es zeigte sich, dass die Primärpartikelgröße, die Aggregatfestigkeit und der hydrophile/hydrophobe Charakter der jeweiligen Nanomaterialien einen entscheidenden Einfluss auf das fließregulierende Potential der Nanomaterialien besitzten.
HINTERGRUND: Der brain-derived neurotrophic factor (BDNF) reguliert die synaptische Plastizität und spielt somit eine wichtige Rolle in der Gedächtnisbildung und -erhaltung. Deswegen gibt es eingehende Untersuchungen dieses neurotrophischen Faktors in Bezug auf Demenzerkrankungen, vor allem der Alzheimer Demenz. In dieser Studie wurde nach einem Zusammenhang zwischen BDNF Blutplasmawerten und der Alzheimer Demenz in einer longitudinalen Kohortenstudie, der Vienna-Transdanube-Aging(VITA)-Studie gesucht. METHODEN: Die VITA-Studie ist eine kommunale Kohortenstudie aller 75jährigen Einwohner einer geographischen Region Wiens. Es wurden die BDNF Plasmawerte der Basisuntersuchung und der ersten Folgeuntersuchung 30 Monate später als mögliche Biomarker für die Alzheimer Demenz untersucht. Assoziationen zwischen BDNF Plasmawerten und anderen epidemiologischen Eckdaten wurden ebenfalls analysiert. ERGEBNISSE: Wir konnten keine Assoziation zwischen BDNF Plasmawerten und der Entwicklung oder einer bereits bestehenden Alzheimer Demenz finden. Geschlecht, Body-Maß-Index und Depression stellten sich als Komorbiditäts-Faktoren von Demenz-erkrankungen dar. SCHLUSSFOLGERUNG: BDNF Plasmawerte sind diesen Ergebnissen nach kein so viel versprechender molekularer Marker für Alzheimer Demenz wie erhofft. BDNF wird jedoch weiterhin in vielen interessanten Studienprotokollen untersucht, da es sowohl im Blutserum als auch im Hirngewebe nachgewiesen werden kann und somit viele diagnostische und therapeutische Ansätze inspiriert.
Sustainability has become a critical topic in all areas of supply chain management. As discussed earlier, drivers for this development can be identified as both internal and external phenomena. Since customers are one of the key stakeholders in supply chain management, special attention is paid to the impact of costumers´ behavior on sustainable supply chain design decisions. In this context, two main research questions were analyzed:
1.What is the appropriate way to design a supply chain according to environmentally-oriented requirements of customers?
2.What is the impact of customer´s behavior regarding both usage and return of products on supply chain design decisions in an environmentally conscious closed-loop supply chain environment?
Therefore, three different optimization models with various main aspects are developed. To illustrate how the presented models can be applied in practical problem cases, guidelines for implementing an environmentally supply chain design project are presented.
This work developed during the first funding period of the subproject B05 in the framework of the interdisciplinary research consortium TRR 225 ‘From the Fundamentals of Biofabrication toward functional Tissue Models’ and was part of a cooperation between the Orthopedic Department represented by Prof. Dr. Regina Ebert and the Institute of Organic Chemistry represented by Prof. Dr. Jürgen Seibel.
This project dealed with cellular behavior during the bioprinting process and how to influence it by modifying the cell glycocalyx with functional target molecules. The focus was on the impact of potential shear stress, that cells experience when they get processed in thermoresponsive bioinks, and a way to increase the cell stiffness via metabolic glycoengineering to attenuate shear forces. For the characterization of the metabolic glycoengineering, four different peracetylated and four non-acetylated modified monosaccharides (two mannose and two sialic acid sugars) were tested in primary human mesenchymal stromal cells (hMSC) and telomerase-immortalized hMSC (hMSC-TERT). Viability results demonstrated a dose-dependent correlation for all sugars, at which hMSC-TERT seemed to be more susceptible leading to lower viability rates. The assessment of the incorporation efficiencies was performed by click chemistry using fluorescent dyes and revealed also a dose-dependent correlation for all mannose and sialic acid sugars, while glucose and galactose variants were not detected in the glycocalyx. However, incorporation efficiencies were highest when using mannose sugars in the primary hMSC. A subsequent analysis of the temporal retention of the incorporated monosaccharides showed a constant declining fluorescence signal up to 6 d for azido mannose in hMSC-TERT, whereas no signal could be detected for alkyne mannose after 2 d. Investigation of the differentiation potential and expression of different target genes revealed no impairment after incubation with mannose sugars, indicating a normal phenotype for hMSC-TERT. Following the successful establishment of the method, either a coumarin derivative or an artificial galectin 1 ligand were incorporated into the cell glycocalyx of hMSC-TERT as functional target molecule. The biophysical analysis via shear flow deformation cytometry revealed a slightly increased cell stiffness and lowered fluidity for both molecules. A further part of this project aimed to control lectin-mediated cell adhesion by artificial galectin 1 ligands. As that hypothesis was settled in the work group of Prof. Dr. Jürgen Seibel, this work supported with an initial characterization of galectin 1 as part of the hMSC biology. A stable galectin 1 expression at gene and protein level in both hMSC and hMSC-TERT could be confirmed, at which immunocytochemical stainings could detect the protein only in the glycocalyx. The treatment of hMSC-TERT with a galectin 1 ligand in different concentrations did not show an altered gene expression of galectin 1. However, these first data in addition to the investigation of stiffness confirmed the applicability of specific and artificial
IV
galectin 1 ligands in biofabrication approaches to alter cell properties of hMSC. To conclude, metabolic glycoengineering has been successfully implemented in hMSC and hMSC-TERT to introduce glycocalyx modifications which reside there for several days. A proof of concept was carried out by the increase of cell stiffness and fluidity by the incorporation of a coumarin derivative or an artificial galectin 1 ligand.
For the characterization of shear stress impact on cells after printing in thermoresponsive bioinks, the processing of hMSC-TERT (mixing or additionally printing) with Pluronic F127 or Polyoxazoline-Polyoxazine (POx-POzi) polymer solution was investigated. While there were no changes in viability when using POx-POzi bioink, processing with Pluronic F127 indicated slightly lower viability and increased apoptosis activity. Assessment of cellular responses to potential shear stress showed no reorganization of the cytoskeleton independent of the bioink, but highly increased expression of the mechanoresponsive proto-oncogene c Fos which was more pronounced when using Pluronic F127 and just mixed with the bioinks. Interestingly, processing of the mechanoresponsive reporter cell line hMSC-TERT-AP1 revealed slightly elevated mechanotransduction activity when using POx-POzi polymer and just mixed with the bioinks as well. In conclusion, hMSC-TERT embedded in thermoresponsive bioinks might shortly experience shear stress during the printing process, but that did not lead to remarkable cell damage likely due to the rheological properties of the bioinks. Furthermore, the printing experiments also suggested that cells do not sense more shear stress when additionally printed.
The superfamily of G protein-coupled receptors (GPCRs) comprises more than 800 members, which are divided into five families based on phylogenetic analyses (GRAFS classification): Glutamate, Rhodopsin, Adhesion, Frizzled/Taste2 and Secretin. The adhesion G protein-coupled receptor (aGPCR) family forms with 33 homologs in Mammalia the second largest and least investigated family of GPCRs. The general architecture of an aGPCR comprises the GPCR characteristics of an extracellular region (ECR), a seven transmembrane (7TM) domain and an intracellular region (ICR). A special feature of aGPCRs is the extraordinary size of the ECR through which they interact with cellular and matricellular ligands via adhesion motif folds. In addition, the ECR contains a so-called GPCR autoproteolysis-inducing (GAIN) domain, which catalyzes autoproteolytic cleavage of the protein during maturation. This cleavage leads to the formation of an N-terminal (NTF) and a C-terminal fragment (CTF), which build a unit by means of hydrophobic interactions and therefore appear as a heterodimeric receptor at the cell surface. In the past, it has been shown that the first few amino acids of the CTF act as a tethered agonist (TA) that mediates the activation of the receptor through the interaction with the 7TM domain. However, the molecular mechanism promoting the TA-7TM domain interaction remains elusive. This work reveals a novel molecular mechanism that does not require the dissociation of the NTF-CTF complex to promote release of the TA and thus activation of the aGPCR. The introduction of bioorthogonal labels into receptorsignaling- relevant regions of the TA of various aGPCRs demonstrated that the TA is freely accessible within the intact GAIN domain. This suggests a structural flexibility of the GAIN domain, which allows a receptor activation independent of the NTF-CTF dissociation, as found in cleavage-deficient aGPCR variants. Furthermore, the present study shows that the cellular localization and the conformation of the 7TM domain depends on the activity state of the aGPCR, which in turn indicates that the TA mediates conformational changes through the interaction with the 7TM domain, which ultimately regulates the receptor activity. In addition, biochemical analyses showed that the GAIN domain-mediated autoproteolysis of the human aGPCR CD97 (ADGRE5/E5) promotes further cleavage events within the receptor. This suggests that aGPCRs undergo cleavage cascades, which are initialized by the autoproteolytic reaction of the GAIN domain. Thus, it can be assumed that aGPCRs are subject to additional proteolytic events. Finally, the constitutive internalization of the NTF and the CTF of E5 was demonstrated by various labeling methods. It was possible to label both fragments independently and to follow their subcellular location in vitro. In summary, these obtained results contribute to a better understanding about the molecular mechanisms of activity and signaling of aGPCRs.
Unter den sechs Arten der Gattung Listeria finden sich nur zwei pathogene Spezies. L. monocytogenes ist pathogen für Mensch und Tier, L. ivanovii nur tierpathogen. Beide Arten besitzen ein Virulenzgencluster, das auch als Pathogenitätsinsel LIPI-1 bezeichnet wird. Pathogenitätsinseln (PAIs) sind bei gram-negativen Bakterien weit verbreitet, wurden bei gram-positiven Pathogenen bisher jedoch nur selten beschrieben. In L. ivanovii wurde nun ein weiterer Virulenz-assoziierter, instabiler Chromosomenabschnitt entdeckt, der in einem Teilbereich Eigenschaften einer Pathogenitätsinsel besitzt. Ausgehend von einem spontanen, aber reproduzierbaren Deletionsereignis eines großen Genomabschnitts, der einige schon bekannte Virulenz-assoziierte Gene umfasst (i-inlE, i-inlF, smcL), wurden in Zusammenarbeit mit den Kooperationspartnern an der "Universidad Complutense de Madrid", insbesondere mit G. Domínguez-Bernal die komplette deletierte Region sowie flankierende Genombereiche genauer analysiert. Im Rahmen dieser Arbeit konnten rechts von dem bereits charakterisierten Gen smcL 13 neue Open Reading Frames (ORFs) bzw. Gene (ydeI, rnaH, norA) von L. ivanovii identifiziert werden, die größtenteils in der Deletionsmutante L. ivanovii GD-3 deletiert waren. Für die meisten Open Reading Frames konnten Homologien zu ORFs in den Genomsequenzen von L. monocytogenes und der apathogenen Art L. innocua gefunden werden. Eigene experimentelle Analysen zeigten zudem, dass diese ORFs in ähnlicher Anordnung auch in den apathogenen Arten L. seeligeri und L. welshimeri vorhanden sind, was wahrscheinlich macht, dass sie nicht an der Virulenz von Listerien beteiligt sind. G. Domínguez-Bernal fand im links von smcL liegenden Bereich eine Reihe neuer Internalingene, die alle spezifisch für L. ivanovii sind. Für die Gene i-inlE, i-inlF und smcL ist bereits bekannt, dass diese Virulenz-assoziiert sind. Dies führte zur Definition einer neuen, LIPI-2 genannten Pathogenitätsinsel in L. ivanovii, die außer smcL und i-inlFE alle neu gefundenen Internalingene umfasst. In dieser Arbeit durchgeführte Untersuchungen der LIPI-2 flankierenden Bereiche zeigten, dass diese in L. monocytogenes und auch den apathogenen Arten L. innocua, L. seeligeri und L. welshimeri bemerkenswert konserviert sind. Durch Transkriptionsuntersuchungen mittels RT-PCR wurde die Expression der neu identifizierten Gene analysiert. Hierbei wurden verschiedene Kulturbedingungen untersucht sowie die Transkription nach Infektion mehrerer Zelllinien bestimmt. Bei der Sequenzanalyse wurde für fast alle Internalingene eine PrfA-Box identifiziert und es bestätigte sich in dieser Arbeit, dass die meisten der Internalingene PrfA-abhängig exprimiert werden. Allerdings wiesen die einzelnen Gene kein einheitliches Transkriptionsprofil unter verschiedenen in vitro-Bedingungen auf. Eine Analyse der Genexpression nach Infektion verschiedener Zelllinien zeigte schließlich, dass die Internalingene während einer Infektion differentiell transkribiert werden und möglicherweise am Infektionsgeschehen beteiligt sind. Das Expressionsmuster der zu LIPI-2 benachbarten Open Reading Frames bestätigte, dass diese Gene PrfA-unabhängig und unter verschiedenen Bedingungen konstitutiv exprimiert werden. Das Expressionsmuster dieser Gene läßt den Schluss zu, dass sie vermutlich nicht zur Virulenz von L. ivanovii beitragen. Die Untersuchung der Virulenzclustergene in LIPI-1 schließlich zeigte eine deutliche PrfA-Abhängigkeit der Genexpression. Es konnte bestätigt werden, dass deren Transkription unter PrfA-induzierenden Bedingungen verstärkt wird. Zudem fand sich auch nach Infektion eine deutliche Expression dieser Gene.
Fremdschämen or Fremdscham, a negative emotion which arises while observing someone behave inappropriately, comes to fame after the turn of the millennium in german speaking countries. There, they name it literally „other‘s shame“ and it becomes obvious that this emotion happens most commonly while watching TV: reality shows, talent shows and bad comedies. The word even makes it to the dictionaries starting 2009, as its use increases unstoppably in everyday language, starting to get used in more and more situations, seemingly as a synonym of embarrassing or shameful. Still, a look in the emotional research on the subject returns exactly zero results as of 2011, leaving open the question as of what this emotion might be, and what it is not. The present wort aims at explaining not only the phenomenon of Fremdschämen, but also the Emotion behind it - Embarrassment -, at a process level.
Infectious diseases caused by pathogenic microorganisms are one of the largest socioeconomic burdens today. Although infectious diseases have been studied for decades, in numerous cases, the precise mechanisms involved in the multifaceted interaction between pathogen and host continue to be elusive. Thus, it still remains a challenge for researchers worldwide to develop novel strategies to investigate the molecular context of infectious diseases in order to devise preventive or at least anti-infective measures. One of the major drawbacks in trying to obtain in-depth knowledge of how bacterial pathogens elicit disease is the lack of suitable infection models to authentically mimic the disease progression in humans. Numerous studies rely on animal models to emulate the complex temporal interactions between host and pathogen occurring in humans. While they have greatly contributed to shed light on these interactions, they require high maintenance costs, are afflicted with ethical drawbacks, and are not always predictive for the infection outcome in human patients. Alternatively, in-vitro two-dimensional (2D) cell culture systems have served for decades as representatives of human host environments to study infectious diseases. These cell line-based models have been essential in uncovering virulence-determining factors of diverse pathogens as well as host defense mechanisms upon infection. However, they lack the morphological and cellular complexity of intact human tissues, limiting the insights than can be gained from studying host-pathogen interactions in these systems.
The focus of this thesis was to establish and innovate intestinal human cell culture models to obtain in-vitro reconstructed three-dimensional (3D) tissue that can faithfully mimic pathogenesis-determining processes of the zoonotic bacterium Campylobacter jejuni (C. jejuni). Generally employed for reconstructive medicine, the field of tissue engineering provides excellent tools to generate organ-specific cell culture models in vitro, realistically recapitulating the distinctive architecture of human tissues. The models employed in this thesis are based on decellularized extracellular matrix (ECM) scaffolds of porcine intestinal origin. Reseeded with intestinal human cells, application of dynamic culture conditions promoted the formation of a highly polarized mucosal epithelium maintained by functional tight and adherens junctions. While most other in-vitro infection systems are limited to a flat monolayer, the tissue models developed in this thesis can display the characteristic 3D villi and crypt structure of human small intestine.
First, experimental conditions were established for infection of a previously developed, statically cultivated intestinal tissue model with C. jejuni. This included successful isolation of bacterial colony forming units (CFUs), measurement of epithelial barrier function, as well as immunohistochemical and histological staining techniques. In this way, it became possible to follow the number of viable bacteria during the infection process as well as their translocation over the polarized epithelium of the tissue model. Upon infection with C. jejuni, disruption of tight and adherens junctions could be observed via confocal microscopy and permeability measurements of the epithelial barrier. Moreover, C. jejuni wildtype-specific colonization and barrier disruption became apparent in addition to niche-dependent bacterial localization within the 3D microarchitecture of the tissue model. Pathogenesis-related phenotypes of C. jejuni mutant strains in the 3D host environment deviated from those obtained with conventional in-vitro 2D monolayers but mimicked observations made in vivo. Furthermore, a genome-wide screen of a C. jejuni mutant library revealed significant differences for bacterial factors required or dispensable for interactions with unpolarized host cells or the highly prismatic epithelium provided by the intestinal tissue model. Elucidating the role of several previously uncharacterized factors specifically important for efficient colonization of a 3D human environment, promises to be an intriguing task for future research.
At the frontline of the defense against invading pathogens is the protective, viscoelastic mucus layer overlying mucosal surfaces along the human gastrointestinal tract (GIT). The development of a mucus-producing 3D tissue model in this thesis was a vital step towards gaining a deeper understanding of the interdependency between bacterial pathogens and host-site specific mucins. The presence of a mucus layer conferred C. jejuni wildtype-specific protection against epithelial barrier disruption by the pathogen and prevented a high bacterial burden during the course of infection. Moreover, results obtained in this thesis provide evidence in vitro that the characteristic corkscrew morphology of C. jejuni indeed grants a distinct advantage in colonizing mucous surfaces.
Overall, the results obtained within this thesis highlight the strength of the tissue models to combine crucial features of native human intestine into accessible in-vitro infection models. Translation of these systems into infection research demonstrated their ability to expose in-vivo like infection outcomes. While displaying complex organotypic architecture and highly prismatic cellular morphology, these tissue models still represent an imperfect reflection of human tissue. Future advancements towards inclusion of human primary and immune cells will strive for even more comprehensive model systems exhibiting intricate multicellular networks of in-vivo tissue. Nevertheless, the work presented in this thesis emphasizes the necessity to investigate host-pathogen interactions in infection models authentically mimicking the natural host environment, as they remain among the most vital parts in understanding and counteracting infectious diseases.
In einem Zeitraum von Oktober 1997 bis Mai 1998 werden an 19 Patienten 22 Untersuchungen der Becken- und Bein-Arterien sowohl in MRA-Technik als auch als i.a. DSA durchgeführt. Hierbei finden im Rahmen der MRA-Untersuchung in allen Fällen die zeitaufgelöste, Kontrastmittel-unterstützte 3d-Flash-Sequenz und die EKG-getriggerte 2d-Flash-Multivenc-Pha-senkontrast-Sequenz Anwendung. Beide Methoden werden in der Diagnostik der pAVK von der Aortenbifurkation bis zum distalen Unterschenkel getestet und in 3 Fällen im Rahmen einer periinterventionellen Kontrolle vor und nach PTA eingesetzt. Das Patientenkollektiv setzt sich ausnahmslos aus Patienten mit pAVK zusammen, die häufig Nebenbefunde wie zum Beispiel einen Diabetes mellitus oder eine Niereninsuffizienz aufweisen. Die Auswertung der Angiographien erfolgt durch die Zuordnung der verschiedenen arte-riellen Abschnitte zu verschiedenen Stenosegraden und dem anschließenden statistischen Ver-gleich der Befunde der MRA und der i.a.DSA. Als Ergebnisse erhalten wir für die Kontrastmittel-unterstützte MRA eine Übereinstim-mungsrate mit der i.a. DSA von 79% sowie eine Sensitivität von 96,7% und eine Spezifität von 97% für die Abbildung hämodynamisch relevanter Stenosen. Die Sensitivität für die Detektion von Verschlüssen beträgt 97,8% und die entsprechende Spezifität 99,2%. Die Phasenkontrast-MRA zeigt im Vergleich mit der i.a.DSA eine schwächere Überein-stimmungsrate von 65,4% sowie eine Sensitivität von 88,3% und eine Spezifität von 85,6% für die Darstellung hämodynamisch relevanter Stenosen. Für die Diagnose eines Gefäßverschlus-ses ist die Sensitivität 89% und die Spezifität 91,8%. Als Schlußfolgerung wird festgestellt, daß die MRA eine nichtinvasive, zur i.a.DSA äqui-valente Untersuchungsmethode darstellt, die bei Kontraindikationen gegen die i.a.DSA einge-setzt werden kann. Im Vergleich zur Phasenkontrast-MRA ist die Kontrastmittel-unterstützte MRA sowohl ein schnelleres als auch ein präziseres Verfahren zur Diagnostik von Gefäßläsio-nen der Becken-Bein-Arterien und bietet den Vorteil der 3-dimensionalen Darstellung. Die Phasenkontrast-MRA ist insbesondere durch die einfache Durchführbarkeit und die fehlende Invasivität ebenfalls als Verfahren zur Diagnostik der peripheren AVK denkbar, jedoch ist zur exakten Stenosegraduierung im Bereich der Läsion eine nachgeschaltete Untersuchung mit weiteren Methoden nötig. Die MRA kann in der postinterventionellen, angiographischen Kontrolle eingesetzt werden. Für die Empfehlung zum routinemäßigen Einsatz in diesem Bereich sind jedoch Studien mit größeren Fallzahlen nötig. In naher Zukunft läßt sich die MRA-Technik durch die Entwicklung von leistungsfähi-geren Gradientenspulensystemen, neuen Prototypen von Oberflächenspulen, intelligenteren Nachverarbeitungs-Algorhytmen und Blutpool-Kontrastmitteln noch weiter optimieren. Die Evolution der MRA-Technik wird ihre Integration in die Routinediagnostik vereinfachen und ihr Indikationsspektrum erweitern.
The interaction between circadian clocks and metabolism is of increasing interest, since clock dysfunction often correlates with metabolic pathologies. Many research articles have been published analysing the impact of factors such as circadian clock, light, feeding time and diet-type on energy homeostasis in various tissues/organs of organisms with most of the findings done in mammals. Little is known about the impact of circadian clock and the above-mentioned factors on circulating lipids, especially the transport form of lipids - diacylglycerol (DG) and membrane lipids such as phosphatidylethanolamine (PE) and phosphatidylcholine (PC) in the Drosophila hemolymph. The fruit fly Drosophila is a prime model organism in circadian, behaviour and metabolism research.
To study the role of circadian clock and behaviour in metabolism, we performed an extensive comparative hemolymph lipid (diacylglycerol: DG, phosphatidylethanolamine: PE, phosphatidylcholine: PC) analysis using ultra performance liquid chromatography coupled to time-of-flight mass spectrometry (UPLC-MS) between wild-type flies (WTCS) and clock disrupted mutants (per01). In addition, clock controlled food intake– feeding behaviour was investigated. Time-dependent variation of transport (DG) and membrane lipids (PE and PC) were not rhythmic in WTCS under constant darkness and in per01 under LD, suggesting an impact of light and clock genes on daily lipid oscillations. Day-time and night-time restriction of food led to comparable lipid profiles, suggesting that lipid oscillations are not exclusively entrained by feeding but rather are endogenously regulated. Ultradian oscillations in lipid levels in WTCS under LD were masked by digested fatty acids since lipid levels peaked more robustly at the beginning and end of light phase when flies were fed a lipid- and protein-free diet. These results suggest that metabolite (DG, PE and PC) oscillation is influenced by complex interactions between nutrient-type, photic conditions, circadian clock and feeding time.
In conclusion, the results of this thesis suggest that circadian clocks determine transport and membrane lipid oscillation in Drosophila hemolymph in complex interactions between nutrient-type, photic conditions and feeding behaviour.
Im Zellkern eukaryotischer Zellen werden Gene in mRNAs transkribiert, welche umfangreich prozessiert und aus dem Zellkern exportiert werden. Im Zytoplasma erfolgt die Translation der mRNAs in Proteine, ein Prozess, welcher viel Energie benötigt und daher mittels vielfältiger Mechanismen streng reguliert wird. Ein Beispiel hierfür stellt die Klasse der TOP-mRNAs dar, eine RNA-Spezies, welche hauptsächlich Transkripte von Genen umfasst, die selbst in die Translation involviert sind. Die prominentesten Vertreter dieser Klasse sind die Proteine der kleinen und großen ribosomalen Untereinheiten. TOP-mRNAs zeichnen sich durch ein gemeinsames Sequenz-Motiv am Anfang Ihrer 5’-UTR aus, welches aus einem Pyrimidinstrang besteht und unmittelbar nach dem Cap mit einem Cytosin beginnt. Dieses allen TOP-RNAs gemeinsame Motiv ermöglicht die zeitgleiche Translationskontrolle dieser RNA-Klasse. So kann die Translation der TOP-mRNAs unter Stressbedingungen wie z.B. Nährstoffmangel koordiniert inhibiert werden, wodurch Energie eingespart wird.
Bereits lange wird nach einem Regulator gesucht, der an dieses TOP-Motiv bindet und die koordinierte Regulation ermöglicht. Man kann sich hier einen Inhibitor oder auch einen Aktivator vorstellen. Verschiedene Proteine wurden bereits in Erwägung gezogen. In dieser Arbeit wurde das Protein TIAR mittels Massenspektrometrie als TOP-interagierender Faktor identifiziert und dessen Bindungseigenschaften mit dem TOP-Motiv durch Shift Assays untersucht. Hierbei konnten Minimalkonstrukte verschiedener Organismen sowie RNA-TOP – Sequenzen identifiziert werden, welche sich für Strukturanalysen eignen würden. Als weiterer TOP-interagierender Faktor wurde über verschiedene sequenzielle Reinigungsschritte das Protein 14-3-3ε identifiziert.
Weiterhin wurden die TOP-Motiv-bindenden Proteine LARP1 und LARP7 auf Ihre Bindungseigenschaften mit Ihren Zielsequenzen untersucht. Während gezeigt werden konnte, dass LARP1 einen inhibierenden Einfluss auf TOP-RNAs hat, wurde in weiteren Shift-Assays die Bindungseigenschaften von LARP7 mit 7SK untersucht, wobei ebenfalls ein minimales LARP7–Konstrukt sowie 7SK-Konstrukte für Strukturanalysen identifiziert werden konnten. Weiterhin konnte gezeigt werden, dass verschiedene Substanzen wie tRNA und Arginin einen starken Einfluss auf die LARP7-7SK – Interaktion ausüben, welcher in weiteren Studien berücksichtigt werden sollte.
In the present thesis the MBE growth and sample characterization of HgTe structures is investigated
and discussed. Due to the first experimental discovery of the quantum Spin Hall effect
(QSHE) in HgTe quantum wells, this material system attains a huge interest in the spintronics
society. Because of the long history of growing Hg-based heterostructures here at the Experimentelle
Physik III in Würzburg, there are very good requirements to analyze this material
system more precisely and in new directions. Since in former days only doped HgTe quantum
wells were grown, this thesis deals with the MBE growth in the (001) direction of undoped
HgTe quantum wells, surface located quantum wells and three dimensional bulk layers. All
Hg-based layers were grown on CdTe substrates which generate strain in the layer stack and
provide therefore new physical effects. In the same time, the (001) CdTe growth was investigated
on n-doped (001) GaAs:Si because the Japanese supplier of CdTe substrates had a
supply bottleneck due to the Tohoku earthquake and its aftermath in 2011.
After a short introduction of the material system, the experimental techniques were demonstrated
and explained explicitly. After that, the experimental part of this thesis is displayed.
So, the investigation of the (001) CdTe growth on (001) GaAs:Si is discussed in chapter 4.
Firstly, the surface preparation of GaAs:Si by oxide desorption is explored and analyzed.
Here, rapid thermal desorption of the GaAs oxide with following cool down in Zn atmosphere
provides the best results for the CdTe due to small holes at the surface, while e.g. an atomic
flat GaAs buffer deteriorates the CdTe growth quality. The following ZnTe layer supplies the
(001) growth direction of the CdTe and exhibits best end results of the CdTe for 30 seconds
growth time at a flux ratio of Zn/Te ~ 1/1.2. Without this ZnTe layer, CdTe will grow in the
(111) direction. However, the main investigation is here the optimization of the MBE growth
of CdTe. The substrate temperature, Cd/Te flux ratio and the growth time has to be adjusted
systematically. Therefore, a complex growth process is developed and established. This optimized
CdTe growth process results in a RMS roughness of around 2.5 nm and a FWHM value
of the HRXRD w-scan of 150 arcsec. Compared to the literature, there is no lower FWHM
value traceable for this growth direction. Furthermore, etch pit density measurements show
that the surface crystallinity is matchable with the commercial CdTe substrates (around 1x10^4
cm^(-2)). However, this whole process is not completely perfect and offers still room for improvements.
The growth of undoped HgTe quantum wells was also a new direction in research in contrast
to the previous n-doped grown HgTe quantum wells. Here in chapter 5, the goal of very low
carrier densities was achieved and therefore it is now possible to do transport experiments in
the n - and p - region by tuning the gate voltage. To achieve this high sample quality, very precise
growth of symmetric HgTe QWs and their HRXRD characterization is examined. Here,
the quantum well thickness can now determined accurate to under 0.3 nm. Furthermore, the transport analysis of different quantum well thicknesses shows that the carrier density and
mobility increase with rising HgTe layer thickness. However, it is found out that the band
gap of the HgTe QW closes indirectly at a thickness of 11.6 nm. This is caused by the tensile
strained growth on CdTe substrates. Moreover, surface quantum wells are studied. These
quantum wells exhibit no or a very thin HgCdTe cap. Though, oxidization and contamination
of the surface reduces here the carrier mobility immensely and a HgCdTe layer of around 5 nm
provides the pleasing results for transport experiments with superconductors connected to the
topological insulator [119]. A completely new achievement is the realization of MBE growth
of HgTe quantum wells on CdTe/GaAs:Si substrates. This is attended by the optimization of
the CdTe growth on GaAs:Si. It exposes that HgTe quantum wells grown in-situ on optimized
CdTe/GaAs:Si show very nice transport data with clear Hall plateaus, SdH oscillations, low
carrier densities and carrier mobilities up to 500 000 cm^2/Vs. Furthermore, a new oxide etching
process is developed and analyzed which should serve as an alternative to the standard
HCl process which generates volcano defects at some time. However, during the testing time
the result does not differ in Nomarski, HRXRD, AFM and transport measurements. Here,
long-time tests or etching and mounting in nitrogen atmosphere may provide new elaborate
results.
The main focus of this thesis is on the MBE growth and standard characterization of HgTe bulk
layers and is discussed in chapter 6. Due to the tensile strained growth on lattice mismatched
CdTe, HgTe bulk opens up a band gap of around 22 meV at the G-point and exhibits therefore
its topological surface states. The analysis of surface condition, roughness, crystalline quality,
carrier density and mobility via Nomarski, AFM, XPS, HRXRD and transport measurements
is therefore included in this work. Layer thickness dependence of carrier density and mobility
is identified for bulk layer grown directly on CdTe substrates. So, there is no clear correlation
visible between HgTe layer thickness and carrier density or mobility. So, the carrier density is
almost constant around 1x10^11 cm^(-2) at 0 V gate voltage. The carrier mobility of these bulk
samples however scatters between 5 000 and 60 000 cm^2/Vs almost randomly. Further experiments
should be made for a clearer understanding and therefore the avoidance of unusable
bad samples.But, other topological insulator materials show much higher carrier densities and
lower mobility values. For example, Bi2Se3 exhibits just density values around 1019 cm^(-2)
and mobility values clearly below 5000 cm2/Vs. The carrier density however depends much
on lithography and surface treatment after growth. Furthermore, the relaxation behavior and
critical thickness of HgTe grown on CdTe is determined and is in very good agreement with
theoretical prediction (d_c = 155 nm). The embedding of the HgTe bulk layer between HgCdTe
layers created a further huge improvement. Similar to the quantum well structures the carrier
mobility increases immensely while the carrier density levels at around 1x10^11 cm^(-2) at 0
V gate voltage as well. Additionally, the relaxation behavior and critical thickness of these
barrier layers has to be determined. HgCdTe grown on commercial CdTe shows a behavior as
predicted except the critical thickness which is slightly higher than expected (d_c = 850 nm).
Otherwise, the relaxation of HgCdTe grown on CdTe/GaAs:Si occurs in two parts. The layer
is fully strained up to 250 nm. Between 250 nm and 725 nm the HgCdTe film starts to relax
randomly up to 10 %. The relaxation behavior for thicknesses larger than 725 nm occurs than
linearly to the inverse layer thickness. A explanation is given due to rough interface conditions
and crystalline defects of the CdTe/GaAs:Si compared to the commercial CdTe substrate. HRXRD and AFM data support this statement. Another point is that the HgCdTe barriers protect the active HgTe layer and because of the high carrier mobilities the Hall measurements provide new transport data which have to be interpreted more in detail in the future. In addition, HgTe bulk samples show very interesting transport data by gating the sample from the top and the back. It is now possible to manipulate the carrier densities of the top and bottom surface states almost separately. The back gate consisting of the n-doped GaAs substrate and the thick insulating CdTe buffer can tune the carrier density for Delta(n) ~ 3x10^11 cm^(-2). This is sufficient to tune the Fermi energy from the p-type into the n-type region [138].
In this thesis it is shown that strained HgTe bulk layers exhibit superior transport data by embedding between HgCdTe barrier layers. The n-doped GaAs can here serve as a back gate.
Furthermore, MBE growth of high crystalline, undoped HgTe quantum wells shows also new
and extended transport output. Finally, it is notable that due to the investigated CdTe growth
on GaAs the Hg-based heterostructure MBE growth is partially independent from commercial
suppliers.
Malaria and HIV are among the most important global health problems of our time and together are responsible for approximately 3 million deaths annually. These two diseases overlap in many regions of the world including sub-Saharan Africa, Southeast Asia and South America, leading to a higher risk of co-infection. In this study, we generated and characterized hybrid molecules to target P. falciparum and HIV simultaneously for a potential HIV/malaria combination therapy. Hybrid molecules were synthesized by covalent fusion between azidothymidine (AZT) and dihydroartemisinin (DHA), tetraoxane or chloroquine (CQ); and a small library was generated and tested for antiviral and antimalarial activity. Our data suggest that dihyate is the most potent molecule in vitro, with antiplasmodial activity comparable to that of DHA (IC50 = 26 nM, SI > 3000), a moderate activity against HIV (IC50 = 2.9 µM; SI > 35) and safe to HeLa cells at concentrations used in the assay (CC50 > 100 µM). Pharmacokinetic studies further revealed that dihyate is metabolically unstable and is cleaved following an O-dealkylation once in contact with cytochrome P450 enzymes. The later further explains the uneffectiveness of dihyate against the CQ-sensitive P. berghei N strain in mice when administered by oral route at 20 mg/kg. Here, we report on a first approach to develop antimalarial/anti-HIV hybrid molecules and future optimization efforts will aim at producing second generation hybrid molecules to improve activity against HIV as well as compound bioavailability. With the emergence of resistant parasites against all the counterpart drugs of artemisinin derivatives used in artemisinin based combination therapies (ACTs), the introduction of antibiotics in the treatment of malaria has renewed interest on the identification of antibiotics with potent antimalarial properties. In this study we also investigated the antiplasmodial potential of thiostrepton and derivatives, synthesized using combinations of tail truncation, oxidation, and addition of lipophilic thiols to the terminal dehydroamino acid. We showed that derivatives SS231 and SS234 exhibit a better antiplasmodial activity (IC50 = 1 µM SI > 59 and SI > 77 respectively) than thiostrepton (IC50 = 8.95 µM, SI = 1.7). The antiplasmodial activity of these derivatives was observed at concentrations which are not hemolytic and non-toxic to human cell lines. Thiostrepton and derivatives appeared to exhibit transmission blocking properties when administered at their IC50 or IC90 concentrations and our data also showed that they attenuate proteasome activity of Plasmodium, which resulted in an accumulation of ubiquitinated proteins after incubation with their IC80 concentrations. Our results indicate that the parasite’s proteasome could be an attractive target for therapeutic intervention. In this regard, thiostrepton derivatives are promising candidates by dually acting on two independent targets, the proteasome and the apicoplast, with the capacity to eliminate both intraerythrocytic asexual and transmission stages of the parasite. To further support our findings, we evaluated the activity of a new class of antimalarial and proteasome inhibitors namely peptidyl sulfonyl fluorides on gametocyte maturation and analogues AJ34 and AJ38 were able to completely suppress gametocytogenesis at IC50 concentrations (0.23 µM and 0.17 µM respectively) suggesting a strong transmission blocking potential. The proteasome, a major proteolytic complex, responsible for the degradation and re-cycling of non-functional proteins has been studied only indirectly in P. falciparum. In addition, an apparent proteasome-like protein with similarity to bacterial ClpQ/hslV threonine-peptidases was predicted in the parasite. Antibodies were generated against the proteasome subunits alpha type 5 (α5-SU), beta type 5 (β5-SU) and pfhslV in mice and we showed that the proteasome is expressed in both sexual and asexual blood stages of P. falciparum, where they localize in the nucleus and in the cytoplasm. However, expression of PfhslV was only observed in trophozoites and shizonts. The trafficking of the studied proteasome subunits was further investigated by generating parasites expressing GFP tagged proteins. The expression of α5-SU-GFP in transgenic parasite appeared to localize abundantly in the cytoplasm of all blood stages, and no additional information was obtained from this parasite line. In conclusion, our data highlight two new tools towards combination therapy. Hybrid molecules represent promising tools for the cure of co-infected individuals, while very potent antibiotics with a wide scope of activities could be useful in ACTs by eliminating resistant parasites and limiting transmission of both, resistances and disease.
To grow larger, insects must shed their old rigid exoskeleton and replace it with a new one. This process is called molting and the motor behavior that sheds the old cuticle is called ecdysis. Holometabolic insects have pupal stages in between their larval and adult forms, during which they perform metamorphosis. The pupal stage ends with eclosion, i.e., the emergence of the adult from the pupal shell. Insects typically eclose at a specific time during the day, likely when abiotic conditions are at their optimum. A newly eclosed insect is fragile and needs time to harden its exoskeleton. Hence, eclosion is regulated by sophisticated developmental and circadian timing mechanisms.
In Drosophila melanogaster, eclosion is limited to a daily time window in the morning, regarded as the “eclosion gate”. In a population of laboratory flies entrained by light/dark cycles, most of the flies eclose around lights on. This rhythmic eclosion pattern is controlled by the circadian clock and persists even under constant conditions.
Developmental timing is under the control of complex hormonal signaling, including the steroid ecdysone, insulin-like peptides, and prothoracicotropic hormone (PTTH). The interactions of the central circadian clock in the brain and a peripheral clock in the prothoracic gland (PG) that produces ecdysone are important for the circadian timing of eclosion. These two clocks are connected by a bilateral pair of peptidergic PTTH neurons (PTTHn) that project to the PG. Before each molt, the ecdysone level rises and then falls shortly before ecdysis. The falling ecdysone level must fall below a certain threshold value for the eclosion gate to open. The activity of PTTHn is inhibited by short neuropeptide F (sNPF) from the small ventrolateral neurons (sLNvs) and inhibition is thought to lead to a decrease in ecdysone production.
The general aim of this thesis is to further the understanding of how the circadian clock and neuroendocrinal pathways are coordinated to drive eclosion rhythmicity and to identify when these endocrinal signaling pathways are active. In Chapter I, a series of conditional PTTHn silencing-based behavioral assays, combined with neuronal activity imaging techniques such as non-invasive ARG-Luc show that PTTH signaling is active and required shortly before eclosion and may serve to phase-adjust the activity of the PG at the end of pupal development. Trans-synaptic anatomical stainings identified the sLNvs, dorsal neurons 1 (DN1), dorsal neurons 2 (DN2), and lateral posterior neurons (LPNs) clock neurons as directly upstream of the PTTHn.
Eclosion motor behavior is initiated by Ecdysis triggering hormone (ETH) which activates a pair of ventromedial (Vm) neurons to release eclosion hormone (EH) which positively feeds back to the source of ETH, the endocrine Inka cells. In Chapter II trans-synaptic tracing showed that most clock neurons provide input to the Vm and non-canonical EH neurons. Hence, clock can potentially influence the ETH/EH feedback loop. The activity profile of the Inka cells and Vm neurons before eclosion is described. Vm and Inka cells are active around seven hours before eclosion. Interestingly, all EH neurons appear to be exclusively peptidergic.
In Chapter III, using chemoconnectomics, PTTHns were found to express receptors for sNPF, allatostatin A (AstA), allatostatin C (AstC), and myosuppressin (Ms), while EH neurons expressed only Ms and AstA receptors. Eclosion assays of flies with impaired AstA, AstC, or Ms signaling do not show arrhythmicity under constant conditions. However, optogenetic activation of the AstA neurons strongly suppresses eclosion.
Chapter IV focuses on peripheral ventral’ Tracheal dendrite (v’Td) and class IV dendritic arborization (C4da) neurons. The C4da neurons mediate larval light avoidance through endocrine PTTH signaling. The v’Td neurons mainly receive O2/CO2 input from the trachea and are upstream of Vm neurons but are not required for eclosion rhythmicity. Conditional ablation of the C4da neurons or torso (receptor of PTTH) knock-out in the C4da neurons impaired eclosion rhythmicity. Six to seven hours before eclosion, PTTHn, C4da, and Vm neurons are active based on ARG-Luc imaging. Thus, C4da neurons may indirectly connect the PTTHn to the Vm neurons.
In summary, this thesis advances our knowledge of the temporal activity and role of PTTH signaling during pupal development and rhythmic eclosion. It further provides a comprehensive characterization of the synaptic and peptidergic inputs from clock neurons to PTTHn and EH neurons. AstA, AstC, and Ms are identified as potential modulators of eclosion circuits and suggest an indirect effect of PTTH signaling on EH signaling via the peripheral sensory C4da neurons.
Die vorliegende Arbeit zeigt eine Möglichkeit auf, die bisher meist erfolglose Chemotherapie des malignen Melanoms zu verbessern: Durch Inhibition des Transkriptionsfaktors NF-kB, der für die Regulation vieler tumorrelevanter Gene verantwortlich ist, konnten die Tumorzellen gegenüber der Wirkung von Zytostatika sensibilisiert werden. Zunächst wurden acht verschiedene Melanomzellen in Bezug auf ihre NF-kB-Aktivität und der Expression NF-kB-regulierter Proteine vergleichen. Es konnte gezeigt werden, dass die Mehrzahl der Melanomzellen über konstitutive Aktivität von NF-κB verfügt. Dabei bestand kein eindeutiger Zusammenhang zwischen der Expression NF-kB-regulierter Proteine und der Aktivität dieses Transkriptionsfaktors im Kern, was komplexe Regulationsmechanismen bei der Transkription und Translation vermuten lässt. Anhand einer ausgewählten Melanomzelllinie konnte gezeigt werden, dass zwei verschiedene NF-kB-Inhibitoren, der Proteasom-Inhibitor Bortezomib und der neue IKK-Inhibitor KINK-1 die Aktivität von NF-kB deutlich hemmen. Beim Vergleich beider NF-kB-Inhibitoren ließen sich unerwartet verschiedene molekulare Wirkungsmechanismen nachweisen: Während Bortezomib konzentrationsabhängig eine sehr starke Induktion von NOXA, eine Induktion von p53 sowie eine Abnahme von Cyclin D1 bewirkte, zeigte KINK-1 seine Effekte vor allem in der Reduktion von Chemokinen wie IL-8 und MCP-1. Passend zur Veränderung der Expression zellzyklus-relevanter Proteine hatte Bortezomib einen stärkeren Effekt auf den Zellzyklus als KINK-1. Beide Inhibitoren wurden mit verschiedenen Zytostatika kombiniert und konnten einerseits die Apoptoseinduktion durch Zytostatika verstärken und andererseits die durch Zytostatika reduzierte Invasion weiter reduzieren. Allerdings zeigte sich bei der Untersuchung tumorrelevanter Chemokine, dass KINK-1 im Gegensatz zu Bortezomib synergistische Effekte mit Camptothecin und Doxorubicin aufweist. Trotz molekularer Unterschiede bewirkten beide NF-kB-Inhibitoren vergleichbare funktionelle Effekte auf zellulärer Ebene. Dies galt auch für ein präklinisches in-vivo-Modell, in dem die experimentelle Lungenmetastasierung von B16F10-Melanomzellen in Mäusen ermittelt wurde: Hier wurden die Mäuse mit Camptothecin, KINK-1 und Bortezomib allein im Vergleich zu den jeweiligen Kombinationen aus Zytostatikum und NF-kB-Inhibitor behandelt. Beide Kombinationen zeigten eine signifikante Reduktion des Lungengewichts im Vergleich zu Camptothecin allein. Diese Arbeit konnte also den Nutzen aus NF-kB-Inhibition in Kombination mit Zytostatika für die hier verwendeten Substanzen bekräftigen und dabei einige molekulare Unterschiede aufdecken.
Nach wie vor ist die Zahl der Malaria-Neuerkrankungen mit ca. 500 Millionen Menschen weltweit sehr besorgniserregend. Durch zunehmende Resistenzen der Erreger gegen zahlreiche Arzneimittel wird die Situation zusätzlich verschärft. Daher ist die Suche und Entwicklung neuartiger Medikamente wichtiger denn je. Die Natur ist immer noch das größte Reservoir an neuen Wirkstoffen, welche als Leitstrukturen für Arzneistoffe fungieren. In den letzten Jahren wurde eine große Zahl neuartiger, biologisch aktiver Naturstoffe identifiziert und hinsichtlich ihres Potenzials für eine pharmazeutische Weiterentwicklung analysiert. Die Naphthylisochinolin-Alkaloide gehören zu solch einer vielversprechenden Wirkstoffklasse, da sie sich v.a. durch ihre hervorragenden pharmakologischen Eigenschaften auszeichnen. Kürzlich wurden die ersten N,C-gekuppelten Naphthyldihydroisochinolin-Alkaloide, Ancistrocladinium A und B, entdeckt. Diese Verbindungen weisen als strukturelle Besonderheit eine außergewöhnliche Iminium-Aryl-Achse auf und besitzen zudem exzellente anti-infektive Aktivitäten, insbesondere gegen den Erreger der Orientbeule, Leishmania major. Ziel der vorliegenden Dissertation war die Synthese neuartiger sterisch gehinderter und strukturell vereinfachter Naphthylisochinoline für weiterführende Struktur-Aktivitäts-Beziehungen (SAR-Studien) und die stereochemische Analyse dieser Verbindungen. Zudem sollte eine Syntheseroute zu den neuartigen dimeren C,C-gekuppelten Naphthylisochinolin-Alkaloiden Shuangancistrotectorin A und B entwickelt werden.
The one electron oxidation potential of ten TAAs with all permutations of Cl , OMe- and Me-substituents in the three p-positions were determined by CV. The half wave potential of the first oxidation wave correlates linearly with the number of Cl- and OMe-substituents. AM1-CISD derived values of the absorption energies are in good agreement with the experiments but differ strongly for the oscillator strengths as well as for neutral compounds and their corresponding mono radical cations. The small solvent dependence of the experimental UV/Vis spectra in CH2Cl2 and MeCN reflects a minor charge transfer character of the electronic transitions. The UV/Vis/NIR spectra of the series of TAAs and their corresponding radical cations and the AM1 computations reveal that even small substituents may lead to strong symmetry breaking and to a modified electronic structure. The spectroscopic properties of a series of four bis-TAA donor-bridge-donor X-B-X dimers, composed of two asymmetric TAA chromophores (monomers) were investigated. UV/vis-, fluorescence and transient absorption spectra were recorded and compared with those of the corresponding X-B monomers. The excited states of the dimers are described as MV states which show, depending on the chemical nature of the bridge, a varying amount of interactions. It was found that superradiant emission only proceeds in the case of weak and medium coupling. Whether the first excited state potential energy surface of the dimers is a single minimum or a double minimum potential depends on the solvent polarity and the electronic coupling. In the latter case, the dimer relaxes in a symmetry broken CT state. The [2.2]paracyclophane bridged dimer is an example for a weakly coupled system, because the spectroscopic behavior is very similar to the corresponding p xylene monomer. In contrast, anthracene as well as p-xylene bridges mediate a stronger coupling and reveal a significant cooperative influence on the optical properties. A series of [2.2]paracylophane bridged bis-TAA MV radical cations X-B-X+ were analyzed by a GMH three-level model which takes two transitions into account: the IV-CT band and the bridge band. From the GMH analysis, one can conclude that the [2.2]paracyclophane moiety is not the limiting factor which governs the intramolecular charge transfer. The electronic interactions are of course smaller than direct conjugation but from the order of magnitude of the couplings of the [2.2]paracyclophane MV species it can be assumed that this bridge is able to mediate significant through-space and through-bond interactions. From the exponential dependence of the electronic coupling V between the two TAA localized states on the distance r between the two redox centers, it was inferred that the HT proceeds via superexchange mechanism. The analysis reveals that even significantly longer conjugated bridges should still mediate significant electronic interactions, because the decay constant of a series of conjugated MV species is small. The absorption properties of a series of bis-TAA-[2.2]paracyclophane dications X+-B-X+ were presented. The localized and the CT transitions of these dications are explained and analyzed by an exciton coupling model which also considers the photophysical properties of the monomeric TAA radical cations. Together with AM1-CISD calculated transition moments, experimental transition moments and transition energies of the bis-TAA dications were used to calculate electronic couplings by a GMH approach. These couplings are a measure for interactions of the excited MV CT states. The modification of the diabatic states reveals similarities of the GMH three-level model and the exciton coupling model. Comparison of the two models shows that the transition moment between the excited mixed-valence states of the dimer equals the dipole moment difference of the ground and the excited bridge state of the corresponding monomer. Thianthrenophane (1) has a cavity which offers enough room to potentially enable endohedral coordination to small ions or molecules. For the complexation of silver(I) perchlorate, the complex stability constants of thianthrenophane logK1=5.45 and of thianthrene logK2=9.16 were determined by UV/Vis titration. Single competition transport experiments with ten metal salts demonstrate a very high selectivity of thianthrenophane as a carrier for silver(I) and a distinctly higher transport rate compared to carriers such as thianthrene and 14-ane-S4. Although the X-ray crystal structure analysis of the polymeric [Ag(1)]ClO4 shows an exohedral coordination to silver(I), the formation of an endohedral [Ag(1)]+ complex is suggested to be the explanation for the unusual carrier selectivity of silver(I) by 1 in bulk liquid membrane.
Tumor necrosis factor (TNF)-like weak inducer of apoptosis (TWEAK) is a member of the TNF superfamily (TNFSF) and is as such initially expressed as type II class transmembrane glycoprotein from which a soluble ligand form can be released by proteolytic processing. While the expression of TWEAK has been detected at the mRNA level in various cell lines and cell types, its cell surface expression has so far only been documented for dendritic cells, monocytes and interferon-γ stimulated NK cells. The fibroblast growth factor-inducible-14 (Fn14) is a TRAF2-interacting receptor of the TNF receptor superfamily (TNFRSF) and is the only receptor for TWEAK. The expression of Fn14 is strongly induced in a variety of non-hematopoietic cell types after tissue injury. The TWEAK/Fn14 system induces pleiotropic cellular activities such as induction of proinflammatory genes, stimulation of cellular angiogenesis, proliferation, differentiation, migration and in rare cases induction of apoptosis. On the other side, Toll-like receptor3 (TLR3) is one of DNA- and RNA-sensing pattern recognition receptors (PRRs), plays a crucial role in the first line of defense against virus and invading foreign pathogens and cancer cells. Polyinosinic-polycytidylic acid poly(I:C) is a synthetic analog of dsRNA, binds to TLR3 which acts through the adapter TRIF/TICAM1, leading to cytokine secretion, NF-B activation, IRF3 nuclear translocation, inflammatory response and may also elicit the cell death. TWEAK sensitizes cells for TNFR1-induced apoptosis and necroptosis by limiting the availability of protective TRAF2-cIAP1 and TRAF2-cIAP2 complexes, which interact with the TNFR1-binding proteins TRADD and RIPK1. In accordance with the fact that poly(I:C)-induced signaling also involves these proteins, we found enhanced necroptosis-induction in HaCaT and HeLa-RIPK3 by poly(I:C) in the presence of TWEAK (Figure 24). Analysis of a panel of TRADD, FADD, RIPK1 and caspase-8 knockout cells revealed furthermore similarities and differences in the way how these molecules act in cell death signaling by poly(I:C)/TWEAK and TNF and TRAIL. RIPK1 turned out to be essential for poly(I:C)/TWEAK-induced caspase-8-mediated apoptosis but was dispensable for these responses in TNF and TRAIL signaling. Lack of FADD protein abrogated TRAIL- but not TNF- and poly(I:C)-induced necroptosis. Moreover, we observed that both long and short FLIP rescued HaCaT and HeLa-RIPK3 cells from poly(I:C)-induced apoptosis or necroptosis.
To sum up, our results demonstrate that TWEAK, which is produced by interferon stimulated myeloid cells, controls the induction of apoptosis and necroptosis by the TLR3 ligand poly(I:C) and may thus contribute to cancer or anti-viral immunity treatment.
Within this thesis, three main approaches for the assessment and investigation of altered hemodynamics like wall shear stress, oscillatory shear index and the arterial pulse wave velocity in atherosclerosis development and progression were conducted:
1. The establishment of a fast method for the simultaneous assessment of 3D WSS and PWV in the complete murine aortic arch via high-resolution 4D-flow MRI
2. The utilization of serial in vivo measurements in atherosclerotic mouse models using high-resolution 4D-flow MRI, which were divided into studies describing altered hemodynamics in late and early atherosclerosis
3. The development of tissue-engineered artery models for the controllable application and variation of hemodynamic and biologic parameters, divided in native artery models and biofabricated artery models, aiming for the investigation of the relationship between atherogenesis and hemodynamics
Chapter 2 describes the establishment of a method for the simultaneous measurement of 3D WSS and PWV in the murine aortic arch at, using ultra high-field MRI at 17.6T [16], based on the previously published method for fast, self-navigated wall shear stress measurements in the murine aortic arch using radial 4D-phase contrast MRI at 17.6 T [4]. This work is based on the collective work of Dr. Patrick Winter, who developed the method and the author of this thesis, Kristina Andelovic, who performed the experiments and statistical analyses. As the method described in this chapter is basis for the following in vivo studies and undividable into the sub-parts of the contributors without losing important information, this chapter was not split into the single parts to provide fundamental information about the measurement and analysis methods and therefore better understandability for the following studies. The main challenge in this chapter was to overcome the issue of the need for a high spatial resolution to determine the velocity gradients at the vascular wall for the WSS quantification and a high temporal resolution for the assessment of the PWV without prolonging the acquisition time due to the need for two separate measurements. Moreover, for a full coverage of the hemodynamics in the murine aortic arch, a 3D measurement is needed, which was achieved by utilization of retrospective navigation and radial trajectories, enabling a highly flexible reconstruction framework to either reconstruct images at lower spatial resolution and higher frame rates for the acquisition of the PWV or higher spatial resolution and lower frame rates for the acquisition of the 3D WSS in a reasonable measurement time of only 35 minutes. This enabled the in vivo assessment of all relevant hemodynamic parameters related to atherosclerosis development and progression in one experimental session. This method was validated in healthy wild type and atherosclerotic Apoe-/- mice, indicating no differences in robustness between pathological and healthy mice.
The heterogeneous distribution of plaque development and arterial stiffening in atherosclerosis [10, 12], however, points out the importance of local PWV measurements. Therefore, future studies should focus on the 3D acquisition of the local PWV in the murine aortic arch based on the presented method, in order to enable spatially resolved correlations of local arterial stiffness with other hemodynamic parameters and plaque composition.
In Chapter 3, the previously established methods were used for the investigation of changing aortic hemodynamics during ageing and atherosclerosis in healthy wild type and atherosclerotic Apoe-/- mice using the previously established methods [4, 16] based on high-resolution 4D-flow MRI. In this work, serial measurements of healthy and atherosclerotic mice were conducted to track all changes in hemodynamics in the complete aortic arch over time. Moreover, spatially resolved 2D projection maps of WSS and OSI of the complete aortic arch were generated. This important feature allowed for the pixel-wise statistical analysis of inter- and intragroup hemodynamic changes over time and most importantly – at a glance. The study revealed converse differences of local hemodynamic profiles in healthy WT and atherosclerotic Apoe−/− mice, with decreasing longWSS and increasing OSI, while showing constant PWV in healthy mice and increasing longWSS and decreasing OSI, while showing increased PWV in diseased mice. Moreover, spatially resolved correlations between WSS, PWV, plaque and vessel wall characteristics were enabled, giving detailed insights into coherences between hemodynamics and plaque composition. Here, the circWSS was identified as a potential marker of plaque size and composition in advanced atherosclerosis. Moreover, correlations with PWV values identified the maximum radStrain could serve as a potential marker for vascular elasticity. This study demonstrated the feasibility and utility of high-resolution 4D flow MRI to spatially resolve, visualize and analyze statistical differences in all relevant hemodynamic parameters over time and between healthy and diseased mice, which could significantly improve our understanding of plaque progression towards vulnerability. In future studies the relation of vascular elasticity and radial strain should be further investigated and validated with local PWV measurements and CFD.
Moreover, the 2D histological datasets were not reflecting the 3D properties and regional characteristics of the atherosclerotic plaques. Therefore, future studies will include 3D plaque volume and composition analysis like morphological measurements with MRI or light-sheet microscopy to further improve the analysis of the relationship between hemodynamics and atherosclerosis.
Chapter 4 aimed at the description and investigation of hemodynamics in early stages of atherosclerosis. Moreover, this study included measurements of hemodynamics at baseline levels in healthy WT and atherosclerotic mouse models. Due to the lack of hemodynamic-related studies in Ldlr-/- mice, which are the most used mouse models in atherosclerosis research together with the Apoe-/- mouse model, this model was included in this study to describe changing hemodynamics in the aortic arch at baseline levels and during early atherosclerosis development and progression for the first time. In this study, distinct differences in aortic geometries of these mouse models at baseline levels were described for the first time, which result in significantly different flow- and WSS profiles in the Ldlr-/- mouse model. Further basal characterization of different parameters revealed only characteristic differences in lipid profiles, proving that the geometry is highly influencing the local WSS in these models. Most interestingly, calculation of the atherogenic index of plasma revealed a significantly higher risk in Ldlr-/- mice with ongoing atherosclerosis development, but significantly greater plaque areas in the aortic arch of Apoe-/- mice. Due to the given basal WSS and OSI profile in these two mouse models – two parameters highly influencing plaque development and progression – there is evidence that the regional plaque development differs between these mouse models during very early atherogenesis.
Therefore, future studies should focus on the spatiotemporal evaluation of plaque development and composition in the three defined aortic regions using morphological measurements with MRI or 3D histological analyses like LSFM. Moreover, this study offers an excellent basis for future studies incorporating CFD simulations, analyzing the different measured parameter combinations (e.g., aortic geometry of the Ldlr-/- mouse with the lipid profile of the Apoe-/- mouse), simulating the resulting plaque development and composition. This could help to understand the complex interplay between altered hemodynamics, serum lipids and atherosclerosis and significantly improve our basic understanding of key factors initiating atherosclerosis development.
Chapter 5 describes the establishment of a tissue-engineered artery model, which is based on native, decellularized porcine carotid artery scaffolds, cultured in a MRI-suitable bioreactor-system [23] for the investigation of hemodynamic-related atherosclerosis development in a controllable manner, using the previously established methods for WSS and PWV assessment [4, 16]. This in vitro artery model aimed for the reduction of animal experiments, while simultaneously offering a simplified, but completely controllable physical and biological environment. For this, a very fast and gentle decellularization protocol was established in a first step, which resulted in porcine carotid artery scaffolds showing complete acellularity while maintaining the extracellular matrix composition, overall ultrastructure and mechanical strength of native arteries. Moreover, a good cellular adhesion and proliferation was achieved, which was evaluated with isolated human blood outgrowth endothelial cells. Most importantly, an MRI-suitable artery chamber was designed for the simultaneous cultivation and assessment of high-resolution 4D hemodynamics in the described artery models. Using high-resolution 4D-flow MRI, the bioreactor system was proven to be suitable to quantify the volume flow, the two components of the WSS and the radStrain as well as the PWV in artery models, with obtained values being comparable to values found in literature for in vivo measurements. Moreover, the identification of first atherosclerotic processes like intimal thickening is achievable by three-dimensional assessment of the vessel wall morphology in the in vitro models. However, one limitation is the lack of a medial smooth muscle cell layer due to the dense ECM. Here, the utilization of the laser-cutting technology for the generation of holes and / or pits on a microscale, eventually enabling seeding of the media with SMCs showed promising results in a first try and should be further investigated in future studies. Therefore, the proposed artery model possesses all relevant components for the extension to an atherosclerosis model which may pave the way towards a significant improvement of our understanding of the key mechanisms in atherogenesis.
Chapter 6 describes the development of an easy-to-prepare, low cost and fully customizable artery model based on biomaterials. Here, thermoresponsive sacrificial scaffolds, processed with the technique of MEW were used for the creation of variable, biomimetic shapes to mimic the geometric properties of the aortic arch, consisting of both, bifurcations and curvatures. After embedding the sacrificial scaffold into a gelatin-hydrogel containing SMCs, it was crosslinked with bacterial transglutaminase before dissolution and flushing of the sacrificial scaffold. The hereby generated channel was subsequently seeded with ECs, resulting in an easy-to-prepare, fast and low-cost artery model. In contrast to the native artery model, this model is therefore more variable in size and shape and offers the possibility to include smooth muscle cells from the beginning. Moreover, a custom-built and highly adaptable perfusion chamber was designed specifically for the scaffold structure, which enabled a one-step creation and simultaneously offering the possibility for dynamic cultivation of the artery models, making it an excellent basis for the development of in vitro disease test systems for e.g., flow-related atherosclerosis research. Due to time constraints, the extension to an atherosclerosis model could not be achieved within the scope of this thesis. Therefore, future studies will focus on the development and validation of an in vitro atherosclerosis model based on the proposed bi- and three-layered artery models.
In conclusion, this thesis paved the way for a fast acquisition and detailed analyses of changing hemodynamics during atherosclerosis development and progression, including spatially resolved analyses of all relevant hemodynamic parameters over time and in between different groups. Moreover, to reduce animal experiments, while gaining control over various parameters influencing atherosclerosis development, promising artery models were established, which have the potential to serve as a new platform for basic atherosclerosis research.
Mehrere Autoren haben schon die Intra- und Interobserver-Variabilität bei der Bestimmung des Schilddrüsenvolumens und knotiger Herdbefunde mit Hilfe des zweidimensionalen (2D) Ultraschalls evaluiert. Darüber hinaus wurde über Interobserver-Korrelationen für Schilddrüsenvolumenmessungen berichtet. Es gibt jedoch keine prospektive verblindete Studie, die die Intra- bzw. Interobserver-Variabilität bei der Volumenbestimmung der gesamten Schilddrüse an gesunden Probanden bzw. einzelner Knoten unterschiedlicher Echogenität an einem Phantom untersucht hat. Die Ergebnisse der Einzelstudien sollen hier vorgestellt und – soweit möglich – miteinander verglichen werden. Im Rahmen einer quantitativen Studie mit dem hier präsentierten Schilddrüsenphantom soll die Intra- und Interobserver-Variabilität bei der 2D-Ultraschallvolumetrie einzelner Knoten unterschiedlicher Größe und Echogenität und der Schilddrüsenlappen evaluiert werden. Da Schilddrüsenknoten wegen des geringeren Volumens und ihrer oft unscharfen Randkontur schwieriger zu entdecken und auszumessen sind als die Gesamtschilddrüse, soll untersucht werden, welche Größenordnungen des Messfehlers auftreten und in welcher Relation sie zueinander stehen. Außerdem soll der methodenimmanente Fehler quantifiziert und detektierbare Volumenänderungen erfassbar gemacht werden. Bisher war in der Schilddrüsensonographie kein geeignetes Phantom verfügbar, das kommerziell erhältlich ist und mit dem qualitativ unterschiedliche intrathyreoidale Herdbefunde untersucht werden können. Die vorliegende Studie an gesunden Probanden hatte das primäre Ziel, die Frage nach der Quantifizierbarkeit von Unsicherheitsfaktoren in der Schilddrüsenvolumetrie durch den konventionellen 2D-Ultraschall im Vergleich zu 3D-Referenzvolumina bei gesunden Erwachsenen möglichst exakt zu beantworten und die Untersucherabhängigkeit der Methode zu demonstrieren. Damit soll die Genauigkeit (Richtigkeit und Präzision) der sonographischen Schilddrüsendiagnostik mathematisch erfasst und eine bessere Bewertungsgrundlage für die Frage nach der Reproduzierbarkeit von Ultraschall-Volumenbestimmungen der Schilddrüse und ihrer pathologischen Veränderungen geschaffen werden. Hierfür wurden möglichst aussagekräftige statistische Parameter wie die Intra- und Interobserver-Variabilität, der systematische und zufällige Fehler, der reine Fehler der Messmethode, minimale, sicher detektierbare Volumenänderungen und im Rahmen einer multivariaten Reliabilitätsanalyse die Reliabilitätskoeffizienten untersucht. Ein weiteres Ziel dieser Studie bestand darin, die Reliabilität der in der klinischen Routine benutzten Ellipsoidformel zur Berechnung des Schilddrüsenvolumens zu überprüfen.
It has been proposed that different features of a face provide a source of information for separate perceptual and cognitive processes. Properties of a face that remain rather stable over time, so called invariant facial features, yield information about a face’s identity, and changeable aspects of faces transmit information underlying social communication such as emotional expressions and speech movements. While processing of these different face properties was initially claimed to be independent, a growing body of evidence suggests that these sources of information can interact when people recognize faces with whom they are familiar. This is the case because the way a face moves can contain patterns that are characteristic for that specific person, so called idiosyncratic movements. As a face becomes familiar these idiosyncratic movements are learned and hence also provide information serving face identification. While an abundance of experiments has addressed the independence of invariant and variable facial features in face recognition, little is known about the exact nature of the impact idiosyncratic facial movements have on face recognition. Gaining knowledge about the way facial motion contributes to face recognition is, however, important for a deeper understanding of the way the brain processes and recognizes faces. In the following dissertation three experiments are reported that investigate the impact familiarity of changeable facial features has on processes of face recognition. Temporal aspects of the processing of familiar idiosyncratic facial motion were addressed in the first experiment via EEG by investigating the influence familiar facial movement exerts on event-related potentials associated to face processing and face recognition. After being familiarized with a face and its idiosyncratic movement, participants viewed familiar or unfamiliar faces with familiar or unfamiliar facial movement while their brain potentials were recorded. Results showed that familiarity of facial motion influenced later event-related potentials linked to memory processes involved in face recognition. The second experiment used fMRI to investigate the brain areas involved in processing familiar facial movement. Participants’ BOLD-signal was registered while they viewed familiar and unfamiliar faces with familiar or unfamiliar idiosyncratic movement. It was found that activity of brain regions, such as the fusiform gyrus, that underlie the processing of face identity, was modulated by familiar facial movement. Together these two experiments provide valuable information about the nature of the involvement of idiosyncratic facial movement in face recognition and have important implications for cognitive and neural models of face perception and recognition. The third experiment addressed the question whether idiosyncratic facial movement could increase individuation in perceiving faces from a different ethnic group and hence reduce impaired recognition of these other-race faces compared to own-race faces, a phenomenon named the own-race bias. European participants viewed European and African faces that were each animated with an idiosyncratic smile while their attention was either directed to the form or the motion of the face. Subsequently recognition memory for these faces was tested. Results showed that the own-race bias was equally present in both attention conditions indicating that idiosyncratic facial movement was not able to reduce or diminish the own-race bias. In combination the here presented experiments provide further insight into the involvement of idiosyncratic facial motion in face recognition. It is necessary to consider the dynamic component of faces when investigating face recognition because static facial images are not able to provide the full range of information that leads to recognition of a face. In order to reflect the full process of face recognition, cognitive and neural models of face perception and recognition need to integrate dynamic facial features as a source of information which contributes to the recognition of a face.
Im Rahmen der vorliegenden Studie wurde an 220 Patienten, die zwischen 1988 und 2007 im König-Ludwig-Haus in Würzburg durch einen Operateur wegen rezidivierender, überwiegend posttraumatischer ventraler Schulterinstabilität offen oder arthroskopisch mittels (modifizierter) Bankart-Prozedur operiert wurden, der „Instability Severity Index Score (ISIS)“ so erhoben, wie er aus den präoperativen Unterlagen zu ermitteln war. Alle Patienten wurden nach postoperativen Rezidivluxationen befragt und die Schulterfunktion wurde mittels standardisiertem und validiertem Fragebogen durch den „Constant Score“ und den „Oxford Shoulder Instability Score“ untersucht.
Ziel der Studie war es, den von Balg und Boileau 2007 vorgestellten „Instability Severity Index Score“ (ISIS) auf seine Aussagekraft hin am vorliegenden Kollektiv zu überprüfen. Zeitgleich sollten ein Vergleich der offenen mit den arthroskopischen Stabilisierungen sowie eine Analyse der Ursachen der Rezidivluxationen erfolgen.
Insgesamt kam es in acht Fällen zu Rezidivluxationen (3,6 %). Die offen Operierten wiesen eine Rate von 3,1 %, die Gruppe der arthroskopisch Operierten 8,7 % Rezidive auf. Patienten mit weniger oder gleich sechs Punkten im ISIS hatten in 2,7 % Reluxationen, Patienten mit mehr als sechs Punkten in 8,1 %.
Patienten, die rückblickend gemäß der Empfehlung aus dem ISIS operiert wurden, hatten in 5,3 % Rezidivluxationen. Patienten, die entgegen der Empfehlung operiert wurden, in 3,5 %. Alle Unterschiede waren statistisch nicht signifikant. In allen Gruppen konnten in den funktionellen Scores sehr gute Ergebnisse mit durchschnittlich über 87 % im alters- und geschlechtsadaptierten Constant Score und über 42 Punkten im Oxford Shoulder Instability Score ohne signifikante Unterschiede erzielt werden. Von den insgesamt acht Patienten mit Reluxationen lagen von zwei Patienten CT-Untersuchungen nach aufgetretener Reluxation vor. In beiden Fällen konnten signifikante Glenoidranddefekte gefunden werden.
Aus Sicht der erhobenen Daten und der erzielten Ergebnisse ist der ISIS als nützlich zur präoperativen Risikobewertung sowie zur Entscheidung über das operative Vorgehen einzuschätzen, wobei er keine imperative Handlungsanweisung darstellen sollte. Die Empfehlung zum Korakoidtransfer nach Latarjet ab sieben Punkten im ISIS kann anhand dieser Daten nicht bestätigt werden. Vielmehr konnte gezeigt werden, dass eine offene Bankart-Operation mit selektivem Kapselshift sehr gute Langzeitergebnisse bezüglich der Reluxationsraten und der funktionellen Ergebnisse liefert. Im Hinblick auf die erzielten Ergebnisse und Fehleranalysen ist weiterhin festzuhalten, dass bei Verdacht auf einen Glenoiddefekt in der Regel eine CT mit 3D-Rekonstruktion und Seiten-vergleich erfolgen sollte, um die Indikation zum offenen Knochenblocktransfer nicht zu verpassen. Offene und arthroskopische Stabilisierungen können bei richtiger Indikationsstellung kurz- und mittelfristig vergleichbar gute Ergebnisse liefern. Langfristig aber scheint das minimal-invasive Vorgehen höhere Raten an Rezidivluxationen aufzuweisen. Wie auch in dieser Arbeit gezeigt werden konnte, ist ein langer Beobachtungszeitraum bei Studien, die das klinische Ergebnis von Schulterstabilisierungen untersuchen, sehr wichtig, um das wahre Ausmaß an postoperativen Rezidivinstabilitäten zu erfassen.
Large-scale anatomical and functional analyses of the connectivity in both invertebrate and mammalian brains have gained intense attention in recent years. At the same time, the understanding of synapses on a molecular level still lacks behind. We have only begun to unravel the basic mechanisms of how the most important synaptic proteins regulate release and reception of neurotransmitter molecules, as well as changes of synaptic strength. Furthermore, little is known regarding the stoichiometry of presynaptic proteins at different synapses within an organism. An assessment of these characteristics would certainly promote our comprehension of the properties of different synapse types. Presynaptic proteins directly influence, for example, the probability of neurotransmitter release as well as mechanisms for short-term plasticity. We have examined the strength of expression of several presynaptic proteins at different synapse types in the central nervous system of Drosophila melanogaster using immunohistochemistry. Clear differences in the relative abundances of the proteins were obvious on different levels: variations in staining intensities appeared from the neuropil to the synaptic level. In order to quantify these differences, we have developed a ratiometric analysis of antibody stainings. By application of this ratiometric method, we could assign average ratios of presynaptic proteins to different synapse populations in two central relays of the olfactory pathway. In this manner, synapse types could be characterized by distinct fingerprints of presynaptic protein ratios. Subsequently, we used the method for the analysis of aberrant situations: we reduced levels of Bruchpilot, a major presynaptic protein, and ablated different synapse or cell types. Evoked changes of ratio fingerprints were proportional to the modifications we had induced in the system. Thus, such ratio signatures are well suited for the characterization of synapses. In order to contribute to our understanding of both the molecular composition and the function of synapses, we also characterized a novel synaptic protein. This protein, Drep-2, is a member of the Dff family of regulators of apoptosis. We generated drep-2 mutants, which did not show an obvious misregulation of apoptosis. By contrast, Drep-2 was found to be a neuronal protein, highly enriched for example at postsynaptic receptor fields of the input synapses of the major learning centre of insects, the mushroom bodies. Flies mutant for drep-2 were viable but lived shorter than wildtypes. Basic synaptic transmission at both peripheral and central synapses was in normal ranges. However, drep-2 mutants showed a number of deficiencies in adaptive behaviours: adult flies were locomotor hyperactive and hypersensitive towards ethanol-induced sedation. Moreover, the mutant animals were heavily impaired in associative learning. In aversive olfactory conditioning, drep-2 mutants formed neither short-term nor anaesthesia-sensitive memories. We could demonstrate that Drep-2 is required in mushroom body intrinsic neurons for normal olfactory learning. Furthermore, odour-evoked calcium transients in these neurons, a prerequisite for learning, were reduced in drep-2 mutants. The impairment of the mutants in olfactory learning could be fully rescued by pharmacological application of an agonist to metabotropic glutamate receptors (mGluRs). Quantitative mass spectrometry of Drep-2 complexes revealed that the protein is associated with a large number of translational repressors, among them the fragile X mental retardation protein FMRP. FMRP inhibits mGluR-mediated protein synthesis. Lack of this protein causes the fragile X syndrome, which constitutes the most frequent monogenic cause of autism. Examination of the performance of drep-2 mutants in courtship conditioning showed that the animals were deficient in both short- and long-term memory. Drep-2 mutants share these phenotypes with fmrp and mGluR mutants. Interestingly, drep-2; fmrp double mutants exhibited normal memory. Thus, we propose a model in which Drep-2 antagonizes FMRP in the regulation of mGluR-dependent protein synthesis. Our hypothesis is supported by the observation that impairments in synaptic plasticity can arise if mGluR signalling is imbalanced in either direction. We suggest that Drep-2 helps in establishing this balance.
In order to survive, organisms avoid threats and seek rewards. Classical conditioning is a simple model to explain how animals and humans learn associations between events that allow them to predict threats and rewards efficiently. In the classical conditioning paradigm, a neutral stimulus is paired with a biologically significant event (the unconditioned stimulus – US). In virtue of this association, the neutral stimulus acquires affective motivational properties, and becomes a conditioned stimulus (CS+). Defensive responses emerge for pairings with an aversive US (e.g., pain), and appetitive responses emerge for pairing with an appetitive event (e.g., reward). It has been observed that animals avoid a CS+ when it precedes an aversive US during a training phase (CS+ US; forward conditioning); whereas they approach a CS+ when it follows an aversive US during the training phase (US CS+; backward conditioning). These findings indicate that the CS+ acquires aversive properties after a forward conditioning, whereas acquires appetitive properties after a backward conditioning. It is thus of interest whether event timing also modulates conditioned responses in such an opponent fashion in humans, who are capable of explicit cognition about the associations. For this purpose, four experiments were conducted in which a discriminative conditioning was applied in groups of participants that only differed in the temporal sequence between CS+ onset and US onset (i.e., the interstimulus interval – ISI). During the acquisition phase (conditioning), two simple geometrical shapes were presented as conditioned stimuli. One shape (CS+) was always associated with a mild painful electric shock (i.e., the aversive US) and the other one (CS-) was never associated with the shock. In a between-subjects design, participants underwent either forward or backward conditioning. During the test phase (extinction), emotional responses to CS+ and CS- were tested and the US was never presented. Additionally, a novel neutral shape (NEW) was presented as control stimulus. To assess cognitive components, participants had to rate both the valence (the degree of unpleasantness or pleasantness) and the arousal (the degree of calmness or excitation) associated with the shapes before and after conditioning. In the first study, startle responses, an ancestral defensive reflex consisting of a fast twitch of facial and body muscles evoked by sudden and intense stimuli, was measured as an index of stimulus implicit valence. Startle amplitude was potentiated in the presence of the forward CS+ whilst attenuated in the presence of the backward CS+. Respectively, the former response indicates an implicit negative valence of the CS+ and an activation of the defensive system; the latter indicated an implicit positive valence of the CS+ and an activation of the appetitive system. In the second study, the blood-oxygen level dependent (BOLD) response was measured by means of functional magnetic resonance imaging (fMRI) to investigate neural responses after event learning. Stronger amygdala activation in response to forward CS+ and stronger striatum activation in response to backward CS+ were found in comparison to CS-. These results support the notion that the defensive motivational system is activated after forward conditioning since the amygdala plays a crucial role in fear acquisition and expression. Whilst the appetitive motivational system is activated after backward conditioning since the striatum plays a crucial role in reward processing. In the third study, attentional processes underlying event learning were observed by means of steady-state visual evoked potentials (ssVEPs). This study showed that both forward and backward CS+ caught attentional resources. More specifically, ssVEP amplitude was higher during the last seconds of forward CS+ that is just before the US, but during the first seconds of backward CS+ that is just after the US. Supposedly, attentional processes were located at the most informative part of CS+ in respect to the US. Participants of all three studies rated both forward and backward CS+ more negative and arousing compared to the CS-. This indicated that event timing did not influence verbal reports similarly as the neural and behavioral responses indicating a dissociation between the explicit and implicit responses. Accordingly, dual process theories propose that human behavior is determined by the output of two systems: (1) an impulsive implicit system that works on associative principles, and (2) a reflective explicit system that functions on the basis of knowledge about facts and values. Most importantly, these two systems can operate in a synergic or antagonistic fashion. Hence, the three studies of this thesis congruently suggest that the impulsive and the reflective systems act after backward association in an antagonistic fashion. In sum, event timing may turn punishment into reward in humans even though they subjectively rate the stimulus associated with aversive events as being aversive. This dissociation might contribute to understand psychiatric disorders, like anxiety disorders or drug addiction.
Infrared photodissociation spectroscopy of ionic hydrocarbons : microsolvation and protonation sites
(2007)
This work has presented a spectroscopic analysis of three types of hydrocarbon cations: two ionized aromatic hydrocarbons, two protonated aromatic hydrocarbons and the cation of a fundamental radical hydrocarbon. The experiments were centered on the proton stretch vibrations of mass-selected complexes of these systems and polar (H2O) and non polar (Ar, N2, CO2) ligands. The experiments have been done in a tandem mass spectrometer coupled with an electron impact ionization ion source; an OPO laser system was used as tunable IR light source. All the proposed dimer structures have been also modeled using quantum chemical calculations (QCC). These calculations have consistently been matched with the experimental results and have enabled clear identification of the spectral features observed. This has enabled the evaluation of thermochemical properties which could not be extracted directly from experiment. The experiments done on complexes of 1-Np+ and Im+ have allowed for the acidity of their various groups to be probed: the shifts in the frequency as well as the enhancement in the intensity of the OH and NH stretch vibrations resulting from the complexation have yielded dependences on both the species (L) and the number (n) of the ligands. OH bound 1-Np+···Ar has been detected for the first time, showing that the REMPI-IRPD method is severely limited with respect to the production of the most stable isomer of a given cationic complex. The detection of c-1-Np+···(N2)n corresponds to the first observation of c-1-Np+ complexes and enables thus direct comparison of both 1-Np+ rotamers. The shift of the NH vibration of Im+···N2(H) yielded the first experimental estimate for the PA of the imidazyl radical. It was also found that the most stable 1-Np+···Ar and Im+···Ar structures differ qualitatively from that of the corresponding neutral dimers (H-bound vs pi-bound), emphasizing the large impact of ionization on the interaction potential and the preferred recognition motif between acidic aromatic molecules (A) and nonpolar ligands. The IRPD spectra of 1-Np+···Ln and Im+···Ln yielded spectroscopic information about the CH, NH and OH stretch vibrations of bare 1-Np+ and Im+. The dependence of the shifts in the frequency of the OH and NH stretch vibrations allows for creating microsolvation models. The spectroscopic results obtained on size-selected 1-NpH+···Ln show that, in the output of the presently used ion source, three classes of 1-NpH+ isomers can be identified: oxonium ions (1-Np protonated at the O atom); carbenium ions obtained by protonation in the para and ortho positions with respect to the OH functional group; carbenium ions obtained by the addition of a proton to well-defined sites on the second naphthalene ring. The spectral identification of these three classes of protonation sites is supported by their different photofragmentation patterns. It was demonstrated that the spectroscopic monitoring of the microsolvation of ImH+ in Ar and N2 together with the QCCs paint a very detailed picture of the microsolvation process, evidencing clear differences between the microsolvation models as function of the PA of the ligands. Important differences have also been identified between the various binding sites, enabling the creation of a clear scale of priorities for occupation of the binding sites during microsolvation. The application of IRPD to the study of microhydrated ImH+ provided for the first time direct spectroscopic information on the properties of the N-H bonds of this biomolecular building block under controlled microhydration. It was demonstrated that, as protonation enhances the acidity of the NH groups, the ability for proton conductivity of ImH+ increases. A very important result is derived from the IRPD spectroscopy of C2H5+···L (L = Ar, N2, CO2, CH4) dimers. The equilibrium geometry of the C2H5+ has long been debated. Now, IRPD spectra were recorded over the range of the CH stretch fundamentals (covering possible sp3 and sp2 hybridization of C). Depending on the ligand species, the spectra are found to be dominated by the fingerprint of two largely different dimer geometries. Using the experimental C2H5+···Ar spectrum and the corresponding QCCs, the structure of the (weakly perturbed) C2H5+ was found to be the nonclassical one, with one proton straddling across the C=C bond of the H2C=CH2. On the other hand, ligands like N2 and CH4 are strongly influencing the geometry, as seen in the spectral signatures of the C2H5+···N2 and C2H5+···CH4, which correspond to the classical [H2CCH3]+. It was thus demonstrated that while the nonclassical C2H5+ is the global minimum on the PES of the free [C2,H5]+, the structure of the C2H5+ can be strongly influenced by the chemical properties of the environment.
Obwohl eine wirksame Schutzimpfung verfügbar ist, sind Masern noch immer weltweit verbreitet. Mit etwa 750.000 Todesfällen jährlich gehören sie zu den gefährlichsten Infektionskrankheiten im Kindesalter überhaupt. Nicht allein wegen der masernvirusinduzierten Immunsuppression treten sekundäre bakterielle Infektionen, darunter Otitiden oder Pneumonien, gehäuft auf. Eine Beteiligung des zentralen Nervensystems kann zur akuten postinfektiösen Masernenzephalitis (APME), die meist mit einer hohen Defektheilungsrate einhergeht, oder zur letal verlaufenden subakuten sklerosierenden Panenzephalitis (SSPE) führen. Besonders gefürchtet sind die schweren Komplikationen der Riesenzellpneumonie oder der measles inclusion body encephalitis (MIBE) bei immunsupprimierten Patienten. Viele pathogenetische Aspekte und pathophysiologische Vorgänge sind dabei noch nicht gänzlich verstanden. Vaskuläre Endothelzellen sind neben Epithelzellen, Monozyten und Makrophagen sowie Lymphozyten als wichtige Zielzellen für das Masernvirus bei der Ausbreitung der Masernvirusinfektion und Entstehung ihrer Komplikationen anzusehen. In immunhistochemisch aufbereiteten pathologischen Schnittpräparaten wurden in infizierten und stark entzündlich veränderten Arealen immer wieder infizierte Gefäßendothelzellen gefunden. Eine systematische Untersuchung der Interaktion von Masernviren mit humanen Gefäßendothelzellen in vitro lag allerdings bislang nicht vor. Das Ziel dieser Dissertation war es nun, die Interaktion von attenuierten und virulenten Masernvirusstämmen mit humanen Gefäßendothelzellen grundlegend und systematisch zu untersuchen und eine Basis für die Definition pathogenetisch bedeutsamer molekularer Mechanismen zu schaffen. Hierfür wurde mit primären Endothelzellen der menschlichen Nabelschnurvene (HUVEC) und einer humanen mikrovaskulären Hirnendothelzelllinie (HBMEC) ein rein humanes Zellkulturmodell gewählt und unter Verwendung attenuierter und virulenter Masernvirusstämme den natürlichen Bedingungen Rechnung getragen. Als essentielle Grundlage für die Untersuchungsreihen wurden die Endothelzellen auf endothelzellspezifische Markermoleküle hin untersucht und charakterisiert. Einzig die Oberflächenproteine membrane cofactor protein (MCP oder CD46) und signaling lymphocytic activation molecule (SLAM oder CD150) sind bislang als zelluläre Rezeptoren für das Masernvirus identifiziert worden. Es konnte hier eindeutig nachgewiesen werden, dass HUVEC und HBMEC auf verschiedenen zellulären Ebenen konstitutiv CD46, nicht aber SLAM exprimieren. Weder eine Aktivierung der Endothelzellen mit diversen Zytokinen und Stimulantien, noch der Kontakt der Endothelzellen mit inaktivierten Masernviren vermochte eine Expression von SLAM zu induzieren, obwohl eine Expression von toll-like receptor 2 (TLR2) klar aufgezeigt werden konnte. Es konnte hier ebenfalls belegt werden, dass sowohl der attenuierte Masernvirusstamm Edmonston (Edm) als auch die virulenten Masernvirusstämme WTFb, Wü4797 und Wü5679 Endothelzellen infizieren und eine morphologische Zellalteration mit Ausbildung eines zytopathischen Effekts hervorrufen können. Weitere Analysen zeigten für Edm und Wü4797 ein enormes Infektionsausmaß und eine sehr gute Ausbreitungseffizienz, die durch die Anwesenheit CD46-spezifischer Antikörper nur bei Edm klar reduziert werden konnte. Eine Aktivierung der Endothelzellen mit diversen Zytokinen und Stimulantien trug keinen eindeutigen begünstigenden oder hemmenden Effekt auf die Masernvirusinfektion mit sich, Interferon-α und -γ schienen das Infektionsausmaß abzuschwächen. Folgeversuche zur Rezeptormodulation durch Masernviren deuten darauf hin, dass CD46 nur für den attenuierten Masernvirusstamm Edm, nicht aber für die virulenten Masernvirusstämme WTFb, Wü4797 und Wü5679 als zellulärer Rezeptor fungiert. Die Ergebnisse dieser Dissertation belegen eine von den beiden Masernvirusrezeptoren CD46 und SLAM unabhängige Infektion humaner vaskulärer Endothelzellen mit Masernviruswildtypstämmen. Diese Beobachtungen lassen einen weiteren, bislang noch nicht bekannten zellulären Rezeptor oder einen von einem zellulären Rezeptor unabhängigen Aufnahme- und Ausbreitungsmechanismus bei Gefäßendothelzellen vermuten. Es darf weiterhin als sicher angesehen werden, dass Endothelzellen in der Pathogenese von masernvirusinduzierten Komplikationen, sei es direkt oder indirekt, involviert sind.
Effects of dopamine on BDNF / TrkB mediated signaling and plasticity on cortico-striatal synapses
(2021)
Progressive loss of voluntary movement control is the central symptom of Parkinson's disease (PD). Even today, we are not yet able to cure PD. This is mainly due to a lack of understanding the mechanisms of movement control, network activity and plasticity in motor circuits, in particular between the cerebral cortex and the striatum. Brain-derived neurotrophic factor (BDNF) has emerged as one of the most important factors for the development and survival of neurons, as well as for synaptic plasticity. It is thus an important target for the development of new therapeutic strategies against neurodegenerative diseases. Together with its receptor, the Tropomyosin receptor kinase B (TrkB), it is critically involved in development and function of the striatum. Nevertheless, little is known about the localization of BDNF within presynaptic terminals in the striatum, as well as the types of neurons that produce BDNF in the cerebral cortex. Furthermore, the influence of midbrain derived dopamine on the control of BDNF / TrkB interaction in striatal medium spiny neurons (MSNs) remains elusive so far. Dopamine, however, appears to play an important role, as its absence leads to drastic changes in striatal synaptic plasticity. This suggests that dopamine could regulate synaptic activity in the striatum via modulation of BDNF / TrkB function. To answer these questions, we have developed a sensitive and reliable protocol for the immunohistochemical detection of endogenous BDNF. We find that the majority of striatal BDNF is provided by glutamatergic, cortex derived afferents and not dopaminergic inputs from the midbrain. In fact, we found BDNF in cell bodies of neurons in layers II-III and V of the primary and secondary motor cortex as well as layer V of the somatosensory cortex. These are the brain areas that send dense projections to the dorsolateral striatum for control of voluntary movement. Furthermore, we could show that these projection neurons significantly downregulate the expression of BDNF during the juvenile development of mice between 3 and 12 weeks.
In parallel, we found a modulatory effect of dopamine on the translocation of TrkB to the cell surface in postsynaptic striatal Medium Spiny Neurons (MSNs). In MSNs of the direct pathway (dMSNs), which express dopamine receptor 1 (DRD1), we observed the formation of TrkB aggregates in the 6-hydroxydopamine (6-OHDA) model of PD. This suggests that DRD1 activity controls TrkB surface expression in these neurons. In contrast, we found that DRD2 activation has opposite effects in MSNs of the indirect pathway (iMSNs). Activation of DRD2 promotes a rapid decrease in TrkB surface expression which was reversible and depended on cAMP. In parallel, stimulation of DRD2 led to induction of phospho-TrkB (pTrkB). This effect was significantly slower than the effect on TrkB surface expression and indicates that TrkB is transactivated by DRD2. Together, our data provide evidence that dopamine triggers dual modes of plasticity on striatal MSNs by acting on TrkB surface expression in DRD1 and DRD2 expressing MSNs. This surface expression of the receptor is crucial for the binding of BDNF, which is released from corticostriatal afferents. This leads to the induction of TrkB-mediated downstream signal transduction cascades and long-term potentiation (LTP). Therefore, the dopamine-mediated translocation of TrkB could be a mediator that modulates the balance between dopaminergic and glutamatergic signaling to allow synaptic plasticity in a spatiotemporal manner. This information and the fact that TrkB is segregated to persistent aggregates in PD could help to improve our understanding of voluntary movement control and to develop new therapeutic strategies beyond those focusing on dopaminergic supply.
Fragestellung: Querschnittstudien konnten bei Kindern und Jugendlichen mit Deletion 22q11.2 eine Tendenz zu mit dem Alter zunehmenden Verhaltensauffälligkeiten verbunden mit einem Anstieg der elterlichen Stressbelastung zeigen. Die aktuelle Längsschnittstudie sollte diese Ergebnisse überprüfen.
Methodik: Mit Hilfe der deutschen Selbsthilfegruppe KiDS 22q11 wurden alle Hauptbezugspersonen, die bereits vier Jahre zuvor an einer Befragung zu Verhaltensauffälligkeiten und Stress teilgenommen hatten, anonymisiert um die Bearbeitung verschiedener Fragebögen gebeten.
Ergebnisse: 59 von 94 Hauptbezugspersonen sandten ausgefüllte Fragebögen zurück. Dabei wurden 54% aller Kinder und Jugendlichen (29 männlich, 30 weiblich, im Alter von 5,8 bis 18,9 Jahren, Mittelwert: 10,8 Jahre) von ihren Hauptbezugspersonen als verhaltensauffällig eingestuft (Gesamtwert Child Behavior Checklist [CBCL] bzw. Fragebogen über das Verhalten junger Erwachsener [YABCL]). In nahezu allen Bereichen der Child Behavior Checklist, mit der die Erfassung der Verhaltensauffälligkeiten erfolgte, kam es im Verlauf zu einer statistisch signifikanten Zunahme. Auch stieg die Stressbelastung der Hauptbezugspersonen, erfasst mittels Fragebogen Soziale Orientierungen von Eltern behinderter Kinder, im Vergleich zur Erstbefragung signifikant an, ohne dass sich jedoch die Lebenszufriedenheit signifikant verändert hätte. Das Ausmaß der elterlichen Stressbelastung korrelierte signifikant mit dem Gesamtproblemwert der CBCL.
Schlussfolgerungen: Die Ergebnisse der aktuellen Längsschnittstudie bestätigen die Befunde früherer Querschnittuntersuchungen hinsichtlich Verhaltensauffälligkeiten bei Kindern und Jugendlichen mit Deletion 22q11.2. Aufgrund der zunehmenden Verhaltensprobleme und der damit einhergehenden Stressbelastung ist mit einem erhöhten Beratungsbedarf der Hauptbezugspersonen und einer zunehmenden Behandlungsbedürftigkeit der Patienten zu rechnen.
Volumenregulatorische Transportwege von anorganischen und organischen Osmolyten in Säugetierzellen
(2014)
Die Aufrechterhaltung des Zellvolumens unter variablen osmotischen Bedingungen stellt für nahezu alle tierischen Zellen eine essenzielle Aufgabe dar. Um regulatorische Volumenanpassungen vorzunehmen besitzen sie daher effektive Mechanismen, mit deren Hilfe der zelluläre Gehalt an organischen und anorganischen Osmolyten erhöht (= regulatorische Volumenzunahme; RVI) oder gesenkt (= regulatorische Volumenabnahme; RVD) werden kann. Trotz langjähriger Forschung auf diesem Gebiet konnten die hieran beteiligten Transportwege für Osmolyte bisher nur unvollständig aufgeklärt werden.
Insbesondere bei T-Lymphozyten sind wichtige Zellfunktionen wie die Proliferation, Migration und die T-Zell-Aktivierung eng mit volumenregulatorischen Mechanismen verbunden. Bei all diesen Prozessen sind u. a. unterschiedliche Kaliumkanäle beteiligt, die insbesondere für die pharmakologische Manipulation von Immunsystemprozessen von wissenschaftlichem Interesse sind. Bisherige Modelle der hypotonen Volumenregulation von T-Lymphozyten berücksichtigen lediglich den spannungsabhängigen KV1.3 sowie den Ca2+-aktivierten IKCa1-Kanal, die zur Klasse der 6TM/P-K+-Kanäle gehören.
Im ersten Teil der vorliegenden Arbeit wurde eine potentielle Rolle von kürzlich entdeckten Zwei-Poren Domänen Kaliumkanälen (K2P) am RVD von murinen und humanen primären CD4+-T-Lymphozyten untersucht. In einem kombinierten genetischen und pharmakologischen Ansatz mittels knockout-Tiermodellen und dem Einsatz kanalspezifischer Inhibitoren konnte mithilfe zellvolumetrischer Analysen gezeigt werden, dass die K2P-Vertreter TASK1, TASK2, TASK3 und TRESK maßgeblich am schwellungsaktivierten Efflux von K+ beteiligt sind. Beurteilt an den Ergebnissen dieser Untersuchung sind der spannungsabhängige TASK2- und der Ca2+-aktivierte TRESK-Kanal für die hypotone Volumenregulation in T-Zellen deutlich bedeutender als TASK1 und TASK3. Der Beitrag der Kanäle TASK2 und TRESK am RVD-Prozess war über dies vergleichbar mit dessen des bisher bekannten KV1.3-Kanals. In dieser Arbeit wurde damit erstmals eine Beteiligung der K2P-Kanäle am RVD muriner und humaner CD4+-Lymphozyten identifiziert. Aufgrund der engen Verbindung zwischen T-Zell-Funktion und der Volumenregulation können Zwei-Poren Domänen K+-Kanäle damit in den engeren Kreis potentieller immunmodulierende Angriffspunkte aufgefasst werden.
Im zweiten und umfangreicheren Teil dieser Arbeit wurden darüber hinaus die schwellungsaktivierten Transportwege für organische Osmolyte (small organic osmolytes; SOOs) untersucht. SOOs stellen chemisch inerte Verbindungen dar, zu denen vor allem Polyole (Sorbitol, myo-Inositol), Methylamine (Betain, α-Glycerophosphocholin) sowie Aminosäuren (α- bzw. β-Alanin und Prolin) und deren Derivate (Taurin) zählen. Da SOOs weder die zelluläre Struktur noch die Funktion von Makromolekülen beeinträchtigen, sind sie wichtige Instrumente der Volumenregulation, die sich in hohen Konzentrationen im Zytosol nahezu aller Zellen wiederfinden. Werden tierische Zellen mit hypotonen Bedingungen konfrontiert, dann ist bei nahezu allen Zellen die Freisetzung organischer Osmolyte zu beobachten, wodurch die zelluläre Osmolarität unabhängig von Elektrolyten angepasst werden kann. Trotz der wichtigen Funktion der SOOs in der Osmoregulation tierischer Zellen konnte die molekulare Identität beteiligter Effluxwege (Kanäle bzw. Transporter) bisher nicht aufgeklärt werden.
Ungeachtet der molekularen Identität der SOO-Effluxwege war es aus zahlreichen biotechnologischen Anwendungen zu Beginn dieser Arbeit bekannt, dass die schwellungsaktivierten Transportwege für organische Osmolyte eine größenselektive Permeabilität für eine Reihe monomerer Zucker und verwandter Verbindungen aufweisen. Um diese Größenselektivität näher zu charakterisieren, wurde im ersten Schritt die schwellungsaktivierte Membranpermeabilität für eine Reihe strukturell homogener Polyethylenglykole unterschiedlicher Polymerlänge (PEG200–1500; hydrodynamische Radien zwischen ~0,5-1,5 nm) unter iso- und hypotonen Bedingungen in Jurkat-Lymphozyten untersucht. Unter milden hypotonen Bedingungen (200 mOsm) war die Plasmamembran der untersuchten Lymphozyten für PEG300-1500 undurchlässig, was aus der Fähigkeit der Zellen zur hypotonen Volumenregulation geschlossen werden konnte. Darüber hinaus wurde RVD in stark hypotonen Lösungen (100 mOsm) mit PEG600-1500 beobachtet, während PEG300-400 unter vergleichbaren osmotischen Bedingungen die Volumenregulation der Zellen inhibierten. Dieses Ergebnis deutet darauf hin, dass starkes hypotones Zellschwellen der Lymphozyten zur Permeabilisierung der Plasmamembran für PEG300-400, nicht jedoch für PEG600-1500, führt. Anhand der hydrodynamischen Radien Rh der verwendeten PEGs konnte ein cutoff-Radius von ~0,74 nm für schwellungsaktivierte Transportwege organischer Osmolyte bestimmt werden. Da diese schwellungsaktivierten Transportwege vielfältig für Zellbeladungstechniken verwendet werden, könnte dieses Ergebnis für zahlreiche biotechnologische und biomedizinische Anwendungen von Interesse sein.
Im zweiten Schritt wurde der Versuch unternommen, potentielle Transportwege für organische Osmolyte im RVD-Prozess molekular zu identifizieren. Da es grundlegend ungeklärt war, wie viele unterschiedliche Transporter bzw. Kanäle am Efflux der zahlreichen organischen Osmolyte beteiligt sind, erfolgte zunächst die vergleichende Analyse des schwellungsaktivierten Membrantransports strukturell verschiedener SOOs einschließlich der Aminosulfonsäure Taurin und des Polyols myo-Inositol. Hierbei wurde erstmals gezeigt, dass die schwellungsaktivierten Transportwege für Taurin und myo-Inositol deutlich unterschiedliche Aktivitätsprofile aufweisen. Während der Taurintransport bereits unter milden hypotonen Bedingungen, d.h. nach einer geringen Absenkung der Osmolalität von 300 auf ~230 mOsm, aktiviert wurde, erfolgte die Aktivierung der Membranpermeabilität für myo-Inositol bei einer viel niedrigeren Osmolalität von ~150 mOsm. Darüber hinaus wiesen die beiden Transportwege unter vergleichbarem hypotonen Stress von 100 mOsm deutlich unterschiedliche Aktivitätsdauern auf (Transport von Taurin ~95 min und myo-Inositol ~40 min). Somit deuteten diese Ergebnisse erstmals auf substrat-spezifische Transportwege für SOOs hin, die voneinander stark abweichende osmotische Aktivierungsprofile besitzen.
Als aussichtsreiche Kandidaten für diese Transportwege wurden zwei Mitglieder der Gruppe der Solute Carrier (SLC) untersucht, die klare Übereinstimmungen mit den gesuchten Transportern für SOOs aufweisen. Daher wurde im Weiteren eine RVD-Beteiligung dieser Transportergruppe mit einer Kombination aus molekularbiologischer und konventioneller bzw. hochaufgelöster mikroskopischen Techniken überprüft. Die semiqantitativen RT-PCR-Ergebnisse dieser Arbeit zeigen dabei, dass die Gentranskription der potentiellen SOO-Transporter SLC5A3 und SLC6A6 in den untersuchten Zelllinien Jurkat, HEK wie auch HepG2-Zellen durch hypotone Bedingungen deutlich verstärkt wird. Hierbei nimmt der zelluläre mRNA-Gehalt der Gene SLC5A3 zwischen 20-60% und SLC6A6 um 30-100% innerhalb von 10-20 min zu, was auf eine potentielle RVD-Beteiligung von SLC-Transportern hindeutet. Ausgehend von diesem Ergebnis wurde daraufhin die zelluläre Lokalisation des SLC5A3-Transporters unter isotonen und hypotonen Bedingungen mikroskopisch untersucht. Wie anhand der konfokalen lasermikroskopischen Untersuchung zu erkennen ist, findet unter hypotoner Stimulation eine zelluläre Umverteilung des mit EGFP fluoreszenzmarkierten Proteins SLC5A3 statt. Innerhalb von 10 min wird der Transporter dabei von intrazellulären Regionen in Richtung Plasmamembran verlagert. Darüber hinaus konnte mit Hilfe der hochauflösenden Mikroskopie-Technik dSTORM gezeigt werden, dass der Transporter SLC5A3 unter hypotoner Stimulation verstärkt mit der Plasmamembran assoziiert vorliegt. Diese verstärkte Membranassoziation des SLC5A3-Proteins deutet damit auf einen schwellungsinduzierten exozytotischen Einbau des Transporters hin.
Die Ergebnisse dieser Arbeit zeigen damit erstmals, dass SLC-Transporter wie SLC5A3, SLC6A6 und vermutlich andere Vertreter der SLC-Superfamilie potentiell am Mechanismus der hypotonen Volumenregulation beteiligt sind. Da SLC-Transporter als wichtige Transportsysteme für Therapeutika angesehen werden und die Mechanismen der Volumenregulation bereits in zahlreichen biotechnologischen Anwendungen implementiert sind, könnte der hier aufgedeckte Zusammenhang einen Erkenntnisgewinn für zahlreiche biomedizinische Forschungsgebiete darstellen.
BLIMP1 ist ein Transkriptionsfaktor und Schlüsselregulator in der Plasmazell-Differenzierung. Um die Rolle des BLIMP1 in der Lymphomentstehung zu untersuchen, wurde die BLIMP1 Expression im normalen humanen lymphatischen Gewebe und in 78 diffusen großzelligen B-Zell Lymphomen untersucht. BLIMP1 wurde in Plasmazellen und GC B-Zellen sowie in einer Population extrafollikulärer B-Zellen exprimiert. Die reifen Plasmazellen vom Marschalko-Typ waren CD138+CD20-MUM1+Ki67-BCL6-PAX5-BLIMP1+. Außerdem zeigten die Keimzentrums-B-Zellen keine Ki67-Expression. Im Gegensatz hierzu waren die BLIMP1+ EGBZ Ki67+p27-. BLIMP1 wurde in 19% (15/78) der DLBCL Fälle, darunter ABC- (7/15) und GCB- (8/15) Typ, exprimiert. BLIMP1+ DLBCL konnten entsprechend dem BLIMP1, BCL6 und PAX5 Expressionsprofil in drei pathogenetisch unterschiedliche Typen unterteilt werden. In den Typ A-Fällen waren die BLIMP1+ Tumor- zellen ständig BCL6-/PAX5- und waren alle vom ABC-Typ (CD10-/BCL6-/MUM1+). Im Typ B-DLBCL waren die meisten Tumorzellen ständig BLIMP1-/BCL6+/PAX5+ und BLIMP1 war nur in relativ kleinen Arealen herdförmig exprimiert. Die BLIMP1+ Zellen zeigten keine BCL6 und PAX5 Expression, und alle Typ B-Fälle zeigten ein GCB-Profil (CD10+ oder BCL6+ und MUM1-). Die Typ C-Fälle waren durch eine gleichzeitige BLIMP1 und BCL6 und/oder PAX5 Expression gekennzeichnet, was einem abärranten und nicht in normalen B-Zellen auftretenden Immunphänotyp entspricht. Weiterhin wurden in 7 Fällen mit Allelverluste auf der Genomregion 6q21, der das BLIMP1 Gen enthält, keine BLIMP1 Mutationen gefunden. Hinsichtlich einer BLIMP1 Expression im normalen lymphatischen Gewebe konnte festgestellt werden, dass das BLIMP1 nicht nur während der Plasmazellentwicklung aus den Keimzentrums-B-Zellen eine bedeutende Rolle spielt, sondern auch mit der Plasmazell-Differenzierung außerhalb des Keimzentrums assoziiert ist. Eine BLIMP1 Expression in DLBCL kennzeichnet die Fälle mit einer Plasmazell-Differenzierung. BLIMP1 ist in den Lymphomen größtenteils wie in normalen B-Zellen reguliert und besitzt die Kapazität, die Plasmazell-Entwicklung in die Tumorzellen zu induzieren. Jedoch reicht die BLIMP1 Expression weder aus, den Zellzyklus aufzuhalten, noch eine komplette terminale Plasmazell-Reifung in den DLBCL zu leiten. Allerdings scheint BLIMP1 nicht von den bekannten TSG Inaktivierungsmechanismen in den DLBCL betroffen zu sein, wobei es sehr unwahrscheinlich ist, dass das BLIMP1 ein TSG darstellt, dessen Verlust bei der Lymphomentwicklung eine wesentliche Rolle spielt.
Es wurden 6 verschiedene Brustimplantate mit unterschiedlichen Füllmaterialien auf ihre Strahlendurchlässigkeit geprüft. Ein Implantat mit dem Füllmaterial Sojaöl, zwei mit Silikon, davon eins mit Polyurethanbeschichtung und zwei mit PVP- Hydrogel gefüllt. Zur Simulation von in vivo - Bedingungen wurde weibliches Brustgewebe, welches bei Mammareduktionen gewonnen wurde, verwendet. Außerdem ein Phantom welches Tumorgewebe, Mikrokalk und fibröse Veränderungen imitieren sollte. Nach Durchführung der Mammographien mit 16 verschiedenen Gewebetaschen wurden die optischen Dicheten für die einzelnen Implantate mit einem Densitometer ermittelt (objektiv quantitative Auswertung) und desweiteren fünf Radiologen in einem Doppelblindverfahren vorgelegt (subjektiv qualitative Auswertung). Es zeigt sich signifikant höhere Strahlendurchlässigkeit für Sojaöl und PVP als Füllmaterial.
Die Untersuchung über Diedrich Becker versucht einen Brückenschlag zwischen musikhistorischer und soziokultureller Betrachtung eines sogenannten "Kleinmeisters": Diedrich Becker (1623-1679), der als Komponist von Sonaten- und Suitensammlungen eine gewisse musikhistorische Bedeutung hat, dessen Biographie aber etliche Lücken aufweist, wird daher im sozialen wie auch kulturellen Kontext seiner Zeit dargestellt. Eine eingehende Betrachtung der Lebensstationen wie die Zeit als Mitglied der Celler Hofkapelle, aber auch sein Wirken als Ratsmusikant in Hamburg lassen auf zahlreiche Verbindungen zu anderen Künstlern seiner Zeit schließen. Beckers Wirken als Komponist zeigt sich in Sonaten und Suiten für Streicherensembles sowie in geistlichen Werken; vor allem die Überlieferungsgeschichte weist wiederum auf das dichte Beziehungsgeflecht hin, innerhalb dessen sich Becker bewegte. Im Anhang finden sich das Werkverzeichnis, Dokumente zur Biographie Beckers sowie alle erhaltenen Kompositionen.
While beneficial sponge-microbe associations have received much attention in recent years, less effort has been undertaken to investigate the interactions of sponges with potentially pathogenic microorganisms. Thus, the aim of this study was to examine two selected Caribbean disease conditions, termed “Sponge Orange Band” and “Sponge White Patch”, via ecological and molecular methods. Sponge Orange Band (SOB) disease affects the prominent Caribbean barrel sponge Xestospongia muta that is counted among the high-microbial-abundance (HMA) sponges, whereas Sponge White Patch (SWP) disease affects the abundant rope sponge Amphimedon compressa that belongs to the low-microbial-abundance (LMA) sponges. I have documented for both Caribbean sponge diseases a disease progression going along with massive tissue destruction as well as loss of the characteristic microbial signatures. Even though new bacteria were shown to colonize the bleached areas, the infection trials revealed in both cases no indication for the involvement of a microbial pathogen as an etiologic agent of disease leaving us still in the dark about the cause of Sponge Orange Band as well as Sponge White Patch disease.
LIM and SH3 protein 1 (LASP1) is a nucleocytoplasmic scaffolding protein. LASP1 interacts with various cytoskeletal proteins via its domain structure and is known to participate in physiological processes of cells. In the present study, a detailed investigation of the expression pattern of LASP1 protein in normal skin, melanocytic nevi and melanoma was carried out and the melanocyte–specific function of LASP1 was analyzed. LASP1 protein was identified in stratum basale of skin epidermis and a very high level was detected in nevi, the benign tumor of melanocyte. In the highly proliferative basal cells, an additional distinct nuclear localization of the protein was noted. In different tumor entities, an elevated LASP1 expression and nuclear localization, correlated positively with malignancy and tumor grade. However, LASP1 level was determined to be very low in melanoma and even reduced in metastases. Melanoma is distinguished as the first tumor tested to date – that displayed an absence of elevated LASP1 expression. In addition no significant relation was observed between LASP1 protein expression and clinicopathological parameters in melanoma.
The epidermal melanin unit of skin comprises of melanocytes and keratinocytes. Melanocytes are specialized cells that synthesize the photo protective coloring pigment, melanin inside unique organelles called melanosomes. The presence of LASP1 in melanocytes is reported for the first time through this study and the existence was confirmed by immunoblotting analysis in cultured normal human epidermal melanocyte (NHEM) and in melanoma cell lines, along with the immunohistostaining imaging in normal skin and in melanocytic nevi. LASP1 depletion in MaMel2 cells revealed a moderate increase in the intracellular melanin level independently of de novo melanogenesis, pointing to a partial hindrance in melanin release. Immunofluorescence images of NHEM and MaMel2 cells visualized co-localization of LASP1 with dynamin and tyrosinase concomitant with melanosomes at the dendrite tips of the cells. Melanosome isolation experiments by sucrose density gradient centrifugation clearly demonstrated the presence of LASP1 and the melanosome specific markers tyrosinase and TRP1 in late stage melanosomes.
The study identified LASP1 and dynamin as novel binding partners in melanocytes and provides first evidence for the existence of LASP1 and dynamin (a protein well–known for its involvement in vesicle formation and budding) in melanosomes. Co-localization of LASP1 and dynamin along the dendrites and at the tips of the melanocytes indicates a potential participation of the two proteins in the membrane vesicle fission at the plasma membrane.
In summary, a possible involvement of LASP1 in the actin–dynamin mediated membrane fission and exocytosis of melanin laden melanosome vesicles into the extracellular matrix is suggested.
New experimental methods have drastically accelerated the pace and quantity at which biological data is generated. High-throughput DNA sequencing is one of the pivotal new technologies. It offers a number of novel applications in various fields of biology, including ecology, evolution, and genomics. However, together with those opportunities many new challenges arise. Specialized algorithms and software are required to cope with the amount of data, often requiring substantial training in bioinformatic methods. Another way to make those data accessible to non-bioinformaticians is the development of programs with intuitive user interfaces.
In my thesis I developed analyses and programs to tackle current problems with high-throughput data in biology. In the field of ecology this covers the establishment of the bioinformatic workflow for pollen DNA meta-barcoding. Furthermore, I developed an application that facilitates the analysis of ecological communities in the context of their traits. Information from multiple public databases have been aggregated and can now be mapped automatically to existing community tables for interactive inspection. In evolution the new data are used to reconstruct phylogenetic trees from multiple genes. I developed the tool bcgTree to automate this process for bacteria. Many plant genomes have been sequenced in current years. Sequencing reads of those projects also contain data from the chloroplasts. The tool chloroExtractor supports the targeted extraction and analysis of the chloroplast genome. To compare the structure of multiple genomes specialized software is required for calculation and visualization of the relationships. I developed AliTV to address this. In contrast to existing programs for this task it allows interactive adjustments of produced graphics. Thus, facilitating the discovery of biologically relevant information. Another application I developed helps to analyze transcriptomes even if no reference genome is present. This is achieved by aggregating the different pieces of information, like functional annotation and expression level, for each transcript in a web platform. Scientists can then search, filter, subset, and visualize the transcriptome.
Together the methods and tools expedite insights into biological systems that were not possible before.
In der vorliegenden prospektiven Pilotstudie wurden die Hypothesen überprüft, dass es durch die nicht-invasive aurikuläre Vagusnervstimulation, jedoch nicht durch eine Kontrollstimulation am Ohrläppchen, zu einer Steigerung der Befindlichkeit, einer Verbesserung der Kognition und einem positiven Effekt auf die Herzratenvariabilität kommt.
Zusammenfassend konnten dabei in dieser Studie geringe Effekte der t-VNS auf einen kognitiven Parameter (F%-Wert des d2-Tests) sowie einen einzelnen HRV-Parameter (pNN50) gezeigt werden, wobei es Hinweise auf eine Intensitätsabhängigkeit der einzelnen Effekte gab. Auf die übrigen erfassten kognitiven Parameter und die weiteren gemessenen HRV-Parameter sowie die Befindlichkeit konnte kein Einfluss der t-VNS nachgewiesen werden. Bestätigt werden konnte das gute Sicherheitsprofil und die gute Tolerabilität der t-VNS.
Der Ausbau der regenerativen Energiequellen führt vermehrt zu unvorhersehbaren Schwankungen der erzeugten Leistung, da Windkraft und Photovoltaik von natürlichen Bedingungen abhängen. Gerade Kurzzeitfluktuationen im Sekunden- bis Minutenbereich, die bei Solarzellen durch die Verschattung von vorüberziehenden Wolken zustande kommen, wird bislang wenig Beachtung geschenkt. Kurzzeitspeicher müssen eine hohe Zyklenstabilität aufweisen, um zur Glättung dieser Leistungsfluktuationen in Frage zu kommen. Im Rahmen der vorliegenden Dissertation wurden elektrochemische Doppelschichtkondensatoren für die Kopplung mit Siliziumsolarzellen und organischen Solarmodulen mit Hilfe von Simulationen und Messungen untersucht. Zusätzlich wurden grundlegende Fragestellungen zur Prozessierung und Alterung von Doppelschichtkondensatoren im Hinblick auf ein in der Literatur bereits diskutiertes System betrachtet, das beide Komponenten in einem Bauteil integriert - den sogenannten photocapacitor.
Um die Druckbarkeit des gesamten elektrochemischen Doppelschichtkondensators zu ermöglichen, wurde der konventionell verwendete Flüssigelektrolyt durch einen Polymer-Gel-Elektrolyten auf Basis von Polyvinylalkohol und einer Säure ersetzt. Durch eine Verbesserung der Prozessierung konnte ein größerer Anteil der spezifischen Fläche der porösen Kohlenstoffelektroden vom Elektrolyten benetzt und somit zur Speicherung genutzt werden. Die Untersuchungen zeigen, dass mit Polymer-Gel-Elektrolyten ähnliche Kapazitäten erreicht werden wie mit Flüssigelektrolyten. Im Hinblick auf die Anwendung im gekoppelten System muss der elektrochemische Doppelschichtkondensator den gleichen Umweltbedingungen hinsichtlich Temperatur und Luftfeuchte standhalten wie die Solarzelle. Hierzu wurden umfangreiche Alterungstests durchgeführt und festgestellt, dass die Kapazität zwar bei Austrocknung des wasserhaltigen Polymer-Gel-Elektrolyten sinkt, bei einer Wiederbefeuchtung aber auch eine Regeneration des Speichers erfolgt.
Zur passenden Auslegung des elektrochemischen Doppelschichtkondensators wurde eine detaillierte Analyse der Leistungsfluktuationen durchgeführt, die mit einem eigens entwickelten MPP-Messgerät an organischen Solarmodulen gemessen wurden. Anhand der Daten wurde analysiert, welche Energiemengen für welche Zeit im Kurzzeitspeicher zwischengespeichert werden müssen, um eine effiziente Glättung der ins Netz einzuspeisenden Leistung zu erreichen. Aus der Statistik der Fluktuationen wurde eine Kapazität berechnet, die als Richtwert in die Simulationen einging und dann mit anderen Kapazitäten verglichen wurde. Neben einem idealen MPP-Tracking für verschiedene Arten von Solarzellen und Beleuchtungsprofilen konnte die Simulation auch die Kopplung aus Solarzelle und elektrochemischem Doppelschichtkondensator mit zwei verschiedenen Betriebsstrategien nachbilden. Zum einen wurde ein fester Lastwiderstand genutzt, zum anderen eine Zielspannung für den Kurzzeitspeicher und somit auch die Solarzelle vorgegeben und der Lastwiderstand variabel so angepasst, dass die Zielspannung gehalten wird. Beide Betriebsmethoden haben einen Energieverlust gegenüber der MPP-getrackten Solarzelle zu verzeichnen, führen aber zu einer Glättung der Leistung des gekoppelten Systems. Die Simulation konnte für Siliziumsolarzellen mit einem Demonstratorversuch im Labor und für organische Solarzellen unter realen Bedingungen validiert werden.
Insgesamt ergibt sich eine vielversprechende Glättung der Leistungsfluktuationen von Solarzellen durch den Einsatz von elektrochemischen Doppelschichtkondensatoren.
In vorausgegangenen Experimenten unseres Labors war bereits gezeigt worden, dass die Applikation von Glutamat zur transienten Erhöhung der cytosolischen Calciumkonzentration sowie zu einer Depolarisation der Plasmamembran von Mesophyllzellen führt. Pharmakologische Studien weisen auf mögliche Orthologe tierischer ionotroper Glutamatrezeptoren (iGLuRs) hin. Ziel dieser Arbeit war eine vertiefte molekulare und funktionelle Analyse der Glutamatrezeptoren (GLRs) aus Arabidopsis thaliana. Dabei konnten folgende Erkenntnisse gewonnen werden: i. Zugabe von extrazellulärem Glutamat in Kombination mit Glycin führt in Abhängigkeit der extrazellulären ATP-Konzentration (eATP) zu einer transienten Erhöhung der Calciumkonzentration in Mesophyllzellen. ii. Die Reaktion von Mesophyllprotoplasten auf die Applikation von Glutamat und Glycin ist im Vergleich zum intakten Blatt stark reduziert, kann jedoch in Gegenwart von eATP oder Glucose signifikant gesteigert werden. iii. Diese Responsibilität von Mesophyllprotoplasten ist zum Zeitpunkt des Einsetzens der Zellwandsynthese (48h) am höchsten. iv. In Patch-Clamp Experimenten führt die photolytische Freisetzung von extrazellulärem caged-Glutamat bei 34 % der gemessenen A. thaliana Mesophyllprotoplasten zu einem verstärkten Kationentransport über die Plasmamembran. Dieser Kationenstrom kann durch gleichzeitige Anwesenheit von extrazellulärem ATP noch verstärkt werden und ist durch einen Desensitivierungsprozess gekennzeichnet. Die Empfindlichkeit dieser Ströme gegenüber Antagonisten tierischer iGluRs stellt eine Verbindung zu der Genfamilie der AtGLRs dar. v. Coexpressionexperimente ausgewählter AtGLRs geben erste Hinweise auf eine Homo- bzw. eine Heteromerbildung von AtGLR1.1 und AtGLR1.4. Aufgrund fehlender Kanalaktivität konnten einzelne, in Oozyten exprimierte AtGLRs bislang nicht funktionell charakterisiert werden. vi. Studien zur transienten und stabilen Überexpression im homologen Expressionssystem zeigen einen cytotoxischen Effekt bei funktioneller Überexpression ausgewählter AtGLRs. vii. Die Analyse der Stellung des Glutamatrezeptors 3.4 in kälteregulierten Signalnetzwerken via Microarrays weist auf ein überlappendes Aufgabenspektrum der Familie der AtGLRs hin. viii. Im Rahmen von Microarray Transkriptionsanalysen an der glr3.4-1 Mutante konnte ein bisher nicht charakterisiertes, co-reguliertes Protein identifiziert werden. Dieses Protein ist durch den Besitz einer transmembranen Region sowie einer ATP-Bindedomäne charakterisiert und könnte einen möglichen Regulator des AtGLR3.4-Kanals darstellen. ix. Die Überprüfung einer möglichen Beteiligung der pflanzlichen Glutamatrezeptoren an der Generierung der glutamatabhängigen Ca2+-Signale sowie die Suche nach Regulatoren bzw. fehlenden Untereinheiten erfolgte mithilfe Mutanten-„Sreenings“. Die Analyse der bis dato identifizierten, Glutamat-insensitiven Mutanten konnte im Rahmen dieser Arbeit nicht abgeschlossen werden.
Part 1 of this work describes the development of accurate physically grounded force fields for
intermolecular Cation-π interactions based on SAPT energy decomposition analysis.
The presented results demonstrate the benefits of the used DFT-SAPT method to describe non-bonding
interactions. First of all, this method is able to reproduce the high level CCSD(T) energy values
but using much less computational time. Second it provides the possibility to separate the total
intermolecular interaction energy into several physically meaningful contributions. The relative
contributions of the dimers investigated can be seen in Fig. 6.16. In Tab. 6.3 the percentage
contribution of the attractive energy parts to the stabilization energy is shown. The polarization
energy is important for the NH+...C6H6 interaction, whereas it becomes less crucial
considering other dimers. The dispersion energy contribution is large in the case of
the C6H6...H2O dimers, whereas it is relatively less important for the NH+...C6H6
interaction. The electrostatic energy contributes a large amount of stabilizing energy
in all considered dimer interactions. ...
Cyclic adenosine monophosphate (cAMP), the ubiquitous second messenger produced upon stimulation of GPCRs which couple to the stimulatory GS protein, orchestrates an array of physiological processes including cardiac function, neuronal plasticity, immune responses, cellular proliferation and apoptosis. By interacting with various effector proteins, among others protein kinase A (PKA) and exchange proteins directly activated by cAMP (Epac), it triggers signaling cascades for the cellular response. Although the functional outcomes of GSPCR-activation are very diverse depending on the extracellular stimulus, they are all mediated exclusively by this single second messenger. Thus, the question arises how specificity in such responses may be attained. A hypothesis to explain signaling specificity is that cellular signaling architecture, and thus precise operation of cAMP in space and time would appear to be essential to achieve signaling specificity. Compartments with elevated cAMP levels would allow specific signal relay from receptors to effectors within a micro- or nanometer range, setting the molecular basis for signaling specificity. Although the paradigm of signaling compartmentation gains continuous recognition and is thoroughly being investigated, the molecular composition of such compartments and how they are maintained remains to be elucidated. In addition, such compartments would require very restricted diffusion of cAMP, but all direct measurements have indicated that it can diffuse in cells almost freely.
In this work, we present the identification and characterize of a cAMP signaling compartment at a GSPCR. We created a Förster resonance energy transfer (FRET)-based receptor-sensor conjugate, allowing us to study cAMP dynamics in direct vicinity of the human glucagone-like peptide 1 receptor (hGLP1R). Additional targeting of analogous sensors to the plasma membrane and the cytosol enables assessment of cAMP dynamics in different subcellular regions. We compare both basal and stimulated cAMP levels and study cAMP crosstalk of different receptors. With the design of novel receptor nanorulers up to 60nm in length, which allow mapping cAMP levels in nanometer distance from the hGLP1R, we identify a cAMP nanodomain surrounding it. Further, we show that phosphodiesterases (PDEs), the only enzymes known to degrade cAMP, are decisive in constraining cAMP diffusion into the cytosol thereby maintaining a cAMP gradient. Following the discovery of this nanodomain, we sought to investigate whether downstream effectors such as PKA are present and active within the domain, additionally studying the role of A-kinase anchoring proteins (AKAPs) in targeting PKA to the receptor compartment. We demonstrate that GLP1-produced cAMP signals translate into local nanodomain-restricted PKA phosphorylation and determine that AKAP-tethering is essential for nanodomain PKA.
Taken together, our results provide evidence for the existence of a dynamic, receptor associated cAMP nanodomain and give prospect for which key proteins are likely to be involved in its formation. These conditions would allow cAMP to exert its function in a spatially and temporally restricted manner, setting the basis for a cell to achieve signaling specificity. Understanding the molecular mechanism of cAMP signaling would allow modulation and thus regulation of GPCR signaling, taking advantage of it for pharmacological treatment.