TY  - JOUR
A1  - Meyer, Malin Tordis
A1  - Watermann, Christoph
A1  - Dreyer, Thomas
A1  - Ergün, Süleyman
A1  - Karnati, Srikanth
T1  - 2021 update on diagnostic markers and translocation in salivary gland tumors
JF  - International Journal of Molecular Sciences
N2  - Salivary gland tumors are a rare tumor entity within malignant tumors of all tissues. The most common are malignant mucoepidermoid carcinoma, adenoid cystic carcinoma, and acinic cell carcinoma. Pleomorphic adenoma is the most recurrent form of benign salivary gland tumor. Due to their low incidence rates and complex histological patterns, they are difficult to diagnose accurately. Malignant tumors of the salivary glands are challenging in terms of differentiation because of their variability in histochemistry and translocations. Therefore, the primary goal of the study was to review the current literature to identify the recent developments in histochemical diagnostics and translocations for differentiating salivary gland tumors.
KW  - salivary gland tumors
KW  - epithelial salivary gland
KW  - adenoid cystic carcinoma (ACC)
KW  - pleomorphic adenoma
KW  - mucoepidermoid carcinoma
KW  - diagnostic markers
Y1  - 2021
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-261057
SN  - 1422-0067
VL  - 22
IS  - 13
ER  - 
TY  - JOUR
A1  - Grunz, Jan-Peter
A1  - Wenig, Andreas Max
A1  - Kunz, Andreas Steven
A1  - Veyhl-Wichmann, Maike
A1  - Schmitt, Rainer
A1  - Gietzen, Carsten Herbert
A1  - Pennig, Lenhard
A1  - Herz, Stefan
A1  - Ergün, Süleyman
A1  - Bley, Thorsten Alexander
A1  - Gassenmaier, Tobias
T1  - 3D cone-beam CT with a twin robotic x-ray system in elbow imaging: comparison of image quality to high-resolution multidetector CT
JF  - European Radiology Experimental
N2  - Background
Elbow imaging is challenging with conventional multidetector computed tomography (MDCT), while cone-beam CT (CBCT) provides superior options. We compared intra-individually CBCT versus MDCT image quality in cadaveric elbows.

Methods
A twin robotic x-ray system with new CBCT mode and a high-resolution clinical MDCT were compared in 16 cadaveric elbows. Both systems were operated with a dedicated low-dose (LD) protocol (equivalent volume CT dose index [CTDI\(_{vol(16 cm)}\)] = 3.3 mGy) and a regular clinical scan dose (RD) protocol (CTDI\(_{vol(16 cm)}\) = 13.8 mGy). Image quality was evaluated by two radiologists (R1 and R2) on a seven-point Likert scale, and estimation of signal intensity in cancellous bone was conducted. Wilcoxon signed-rank tests and intraclass correlation coefficient (ICC) statistics were used.

Results
The CBCT prototype provided superior subjective image quality compared to MDCT scans (for RD, p ≤ 0.004; for LD, p ≤ 0.001). Image quality was rated very good or excellent in 100% of the cases by both readers for RD CBCT, 100% (R1) and 93.8% (R2) for LD CBCT, 62.6% and 43.8% for RD MDCT, and 0.0% and 0.0% for LD MDCT. Single-measure ICC was 0.95 (95% confidence interval 0.91–0.97; p < 0.001). Software-based assessment supported subjective findings with less “undecided” pixels in CBCT than dose-equivalent MDCT (p < 0.001). No significant difference was found between LD CBCT and RD MDCT.
Conclusions

In cadaveric elbow studies, the tested cone-beam CT prototype delivered superior image quality compared to high-end multidetector CT and showed a potential for considerable dose reduction.
KW  - Cancellous bone
KW  - Cone-beam computed tomography
KW  - Elbow
KW  - Elbow joint
KW  - Multidetector computed tomography
Y1  - 2020
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-229877
VL  - 4
ER  - 
TY  - JOUR
A1  - Schmidt, Sven
A1  - Alt, Yvonne
A1  - Deoghare, Nikita
A1  - Krüger, Sarah
A1  - Kern, Anna
A1  - Rockel, Anna Frederike
A1  - Wagner, Nicole
A1  - Ergün, Süleyman
A1  - Wörsdörfer, Philipp
T1  - A blood vessel organoid model recapitulating aspects of vasculogenesis, angiogenesis and vessel wall maturation
JF  - Organoids
N2  - Blood vessel organoids are an important in vitro model to understand the underlying mechanisms of human blood vessel development and for toxicity testing or high throughput drug screening. Here we present a novel, cost-effective, and easy to manufacture vascular organoid model. To engineer the organoids, a defined number of human induced pluripotent stem cells are seeded in non-adhesive agarose coated wells of a 96-well plate and directed towards a lateral plate mesoderm fate by activation of Wnt and BMP4 signaling. We observe the formation of a circular layer of angioblasts around days 5–6. Induced by VEGF application, CD31\(^+\) vascular endothelial cells appear within this vasculogenic zone at approximately day 7 of organoid culture. These cells arrange to form a primitive vascular plexus from which angiogenic sprouting is observed after 10 days of culture. The differentiation outcome is highly reproducible, and the size of organoids is scalable depending on the number of starting cells. We observe that the initial vascular ring forms at the interface between two cell populations. The inner cellular compartment can be distinguished from the outer by the expression of GATA6, a marker of lateral plate mesoderm. Finally, 14-days-old organoids were transplanted on the chorioallantois membrane of chicken embryos resulting in a functional connection of the human vascular network to the chicken circulation. Perfusion of the vessels leads to vessel wall maturation and remodeling as indicated by the formation of a continuous layer of smooth muscle actin expressing cells enwrapping the endothelium. In summary, our organoid model recapitulates human vasculogenesis, angiogenesis as well as vessel wall maturation and therefore represents an easy and cost-effective tool to study all steps of blood vessel development and maturation directly in the human setting without animal experimentation.
KW  - organoid
KW  - blood vessel
KW  - vasculogenesis
KW  - angiogenesis
KW  - induced pluripotent stem cells
Y1  - 2022
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-284043
SN  - 2674-1172
VL  - 1
IS  - 1
SP  - 41
EP  - 53
ER  - 
TY  - JOUR
A1  - Neuhaus, Winfried
A1  - Burek, Malgorzata
A1  - Djuzenova, Cholpon C
A1  - Thal, Serge C
A1  - Koepsell, Hermann
A1  - Roewer, Norbert
A1  - Förster, Carola Y
T1  - Addition of NMDA-receptor antagonist MK801 during oxygen/glucose deprivation moderately attenuates the up-regulation of glucose uptake after subsequent reoxygenation in brain endothelial cells
N2  - During stroke the blood–brain barrier (BBB) is damaged which can result in vasogenic brain edema and inflammation. The reduced blood supply leads to decreased delivery of oxygen and glucose to affected areas of the brain. Oxygen and glucose deprivation (OGD) can cause upregulation of glucose uptake of brain endothelial cells. In this letter, we investigated the influence of MK801, a non-competitive inhibitor of the NMDA-receptor, on the regulation of the glucose uptake and of the main glucose transporters glut1 and sglt1 in murine BBB cell line cerebEND during OGD. mRNA expression of glut1 was upregulated 68.7- fold after 6 h OGD, which was significantly reduced by 10 μM MK801 to 28.9-fold. Sglt1 mRNA expression decreased during OGD which was further reduced by MK801. Glucose uptake was significantly increased up to 907% after 6 h OGD and was still higher (210%) after the 20 h reoxygenation phase compared to normoxia. Ten micromolar MK801 during OGD was able to reduce upregulated glucose uptake after OGD and reoxygenation significantly. Presence of several NMDAR subunits was proven on the mRNA level in cerebEND cells. Furthermore, it was shown that NMDAR subunit NR1 was upregulated during OGD and that this was inhibitable by MK801. In conclusion, the addition of MK801 during the OGD phase reduced significantly the glucose uptake after the subsequent reoxygenation phase in brain endothelial cells.
KW  - Blut-Hirn-Schranke
KW  - Schlaganfall
KW  - Glucosetransportproteine
KW  - NMDA-Antagonist
KW  - NMDA-Rezeptor
KW  - blood-brain barrier
KW  - MK801
KW  - NMDAR
KW  - stroke
KW  - glut1
KW  - sglt1
Y1  - 2012
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-67241
ER  - 
TY  - JOUR
A1  - Kleefeldt, Florian
A1  - Bömmel, Heike
A1  - Broede, Britta
A1  - Thomsen, Michael
A1  - Pfeiffer, Verena
A1  - Wörsdörfer, Philipp
A1  - Karnati, Srikanth
A1  - Wagner, Nicole
A1  - Rueckschloss, Uwe
A1  - Ergün, Süleyman
T1  - Aging‐related carcinoembryonic antigen‐related cell adhesion molecule 1 signaling promotes vascular dysfunction
JF  - Aging Cell
N2  - Aging is an independent risk factor for cardiovascular diseases and therefore of particular interest for the prevention of cardiovascular events. However, the mechanisms underlying vascular aging are not well understood. Since carcinoembryonic antigen‐related cell adhesion molecule 1 (CEACAM1) is crucially involved in vascular homeostasis, we sought to identify the role of CEACAM1 in vascular aging. Using human internal thoracic artery and murine aorta, we show that CEACAM1 is upregulated in the course of vascular aging. Further analyses demonstrated that TNF‐α is CEACAM1‐dependently upregulated in the aging vasculature. Vice versa, TNF‐α induces CEACAM1 expression. This results in a feed‐forward loop in the aging vasculature that maintains a chronic pro‐inflammatory milieu. Furthermore, we demonstrate that age‐associated vascular alterations, that is, increased oxidative stress and vascular fibrosis, due to increased medial collagen deposition crucially depend on the presence of CEACAM1. Additionally, age‐dependent upregulation of vascular CEACAM1 expression contributes to endothelial barrier impairment, putatively via increased VEGF/VEGFR‐2 signaling. Consequently, aging‐related upregulation of vascular CEACAM1 expression results in endothelial dysfunction that may promote atherosclerotic plaque formation in the presence of additional risk factors. Our data suggest that CEACAM1 might represent an attractive target in order to delay physiological aging and therefore the transition to vascular disorders such as atherosclerosis.
KW  - aging
KW  - anti‐aging
KW  - cytokines
KW  - inflammation
KW  - mouse
KW  - reactive oxygen species
Y1  - 2019
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-201231
VL  - 2019
IS  - 18
ER  - 
TY  - THES
A1  - Fahr, Martin Siegfried
T1  - Akzessorische Gelenke zwischen Basiokziput und Atlas bzw. Dens axis in der Medianebene
T1  - Accessory joints between basiocciput and atlas/axis in the median plane
N2  - Der vordere kraniozervikale Übergang wurde an 99 Kopf-Hals-Präparaten aus dem Präpariersaal mittels MRT, CT und Sägeschnitten untersucht. Weiterhin wurden 110 Schädel, 56 Atlas- und 33 Axispräparate vermessen. Es fand sich in 70% der Präparate das Vorliegen einer Osteoarthrose (Ostheoarthritis) der Art. atlanto-axialis mediana; diese Erkrankung war durch die Bildung von maximalen Osteophyten, Vergrößerung der Gelenkflächen, Verlängerung der Gelenkhöhle und Verminderung des Abstandes zum Hinterhauptsbein charakterisiert. In drei Fällen hatten sich sehr große (giant), nach kranial gerichteten Osteophyten mit knöchernen Kontaktzonen zum Basiokziput gebildet. Die Kontaktzonen waren - wie sich feingeweblich zeigte – echte, erworbene, akzessorische, atlanto-okzipitale Gelenke in der Medianebene. In 11 Fällen lagen - wie die MRT- und CT- Schnittbilder zeigten – Reste des Proatlas bzw. der hypochondralen Spange vor: 3 mal als Condylus occipitalis tertius und knöchernen Kontaktzonen zu Atlas bzw. Axis und 7 mal als freie, überknorpelte Ossikel. Auch hier kann - wie die histologische Kontrolle zeigte – bei den Kontaktzonen von echten, allerdings angeborenen akzessorischen (atlantookzipitalen und odonto-okzipitalen) Gelenken in der Medianebene gesprochen werden. Der Casus mit Vorkommen eines Condylus occipitalis tertius und gleichzeitiger Bildung eines Osteophyten der Densspitze, die zusammen eine knöcherne Kontaktzone und akzessorische Gelenkkammern ausgebildet hatten, kann als „gemischter“ Fall bezeichnet werden.
N2  - To explore the many osseous irregularities that are found in the area between the basiocciput, the anterior arch of the atlas and the tip of the dens axis we studied 99 cadaver specimens using magnetic resonance tomography (MRT), computed tomography (CT), median saw-cut sections, and histological sections. Additionally, dry specimens of the skull (n = 110), atlas (n = 56), and axis (n = 33) were investigated. In the median plane, the dry and cadaver specimens exhibited osteoarthritis-related osseous outgrowths and osteophytes of the articular surfaces of the median atlanto-axial joint (n = 63), and the presence of congenitally developed free ossicles (n = 22) and of third occipital condyles (n = 3). The largest osteophytes (giant osteophytes) (n = 4) of the anterior arch of the atlas formed osseous contact zones with the basiocciput that were visible histologically as real joints and were designated accessory median atlanto-occipital joints. The third occipital condyles also formed osseous contact zones, visible histologically as real joints, with the anterior arch of the atlas or with the tip of the dens, and were designated accessory atlanto-occipital or occipito-odontoid joints. Frequent free ossicles, incorporated into the accessory joint, were found by histological examination to be covered with hyaline cartilage.
KW  - Basiokziput
KW  - Atlas
KW  - Dens axis
KW  - TOC (Condylus occipitale tertius)
KW  - Osteoarthrose
KW  - Basiocciput
KW  - Atlas
KW  - Axis
KW  - TOC (third occipital condyle)
KW  - Osteoarthritis
Y1  - 2005
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-17912
ER  - 
TY  - JOUR
A1  - Agranovsky, A. A.
A1  - Dolya, V. V.
A1  - Gorboulev, Valentin G.
A1  - Kozlov, J. V.
A1  - Atabekov, J. G.
T1  - Aminoacylation of barley stripe mosaic virus RNA: polyadenylate-containing RNA has a 3'-terminal tyrosine-accepting structure
N2  - Barley stripe mosaic virus (BSMV) RNA which was previously reported to contain poly(A) sequences (Agranovsky et al., 1978) can be specifically esterified with tyrosine in vitro in the presence of an aminoacyl-tRNA synthetase fraction from wheat embryos. All the three RNA components of the BSMV strain with a three-component genome (Norwich) and both RNA components of a two-component strain (Russian) can be tyrosylated. The poly(A)-containing (bound to oligo(dT)-cellulose) and poly(A)-deficient(not bound to oligo(dT)-cellulose) fractions of BSMV RNA display a similar amino acidaccepting ability. The nucleotide sequence which accepts tyrosine is coupled with the intact genomic polyadenylated BSMV RNA. The viral RNA isolated after sucrose density gradient centrifugation under drastic denaturing conditions retains its aminoacylating activity, which suggests that this activity is not due to the presence in a BSMV RNA preparation of a tyrosine tRNA associated with BSMV RNA. Inhibition of aminoacylation of the 3’-oxidized (treated with sodium metaperiodate) BSMV RNA suggests that the tyrosine-accepting structure is localized at the 3’ terminus of BSMV RNA molecules. It is shown that segments of different lengths obtained upon random fragmentation can be tyrosylated. The 3’-terminal (tyrosine-accepting) poly(A)+ segments can be isolated. The shortest segments of viral RNA capable of being aminoacylated [i.e., containing both tRNA-like structure and poly(A)] consists of approximately 150-200 nucleotides. The analysis of the oligonucleotides derived from individual BSMV RNA components labeled with 32P at the 3’ end revealed two types of 3’-terminal sequences different from poly(A). It is suggested that a poly(A) sequence is intercalated between a 3’-terminal tyrosineaccepting structure and the 5’-terminal portion of poly(A)+ BSMV RNA.
Y1  - 1981
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-32566
ER  - 
TY  - JOUR
A1  - Simon, Micha
A1  - Ipek, Rojda
A1  - Homola, György A.
A1  - Rovituso, Damiano M.
A1  - Schampel, Andrea
A1  - Kleinschnitz, Christoph
A1  - Kuerten, Stefanie
T1  - Anti-CD52 antibody treatment depletes B cell aggregates in the central nervous system in a mouse model of multiple sclerosis
JF  - Journal of Neuroinflammation
N2  - Background:
Multiple sclerosis (MS) is a chronic autoimmune disease of the central nervous system (CNS) for which several new treatment options were recently introduced. Among them is the monoclonal anti-CD52 antibody alemtuzumab that depletes mainly B cells and T cells in the immune periphery. Considering the ongoing controversy about the involvement of B cells and in particular the formation of B cell aggregates in the brains of progressive MS patients, an in-depth understanding of the effects of anti-CD52 antibody treatment on the B cell compartment in the CNS itself is desirable.

Methods:
We used myelin basic protein (MBP)-proteolipid protein (PLP)-induced experimental autoimmune encephalomyelitis (EAE) in C57BL/6 (B6) mice as B cell-dependent model of MS. Mice were treated intraperitoneally either at the peak of EAE or at 60 days after onset with 200 μg murine anti-CD52 vs. IgG2a isotype control antibody for five consecutive days. Disease was subsequently monitored for 10 days. The antigen-specific B cell/antibody response was measured by ELISPOT and ELISA. Effects on CNS infiltration and B cell aggregation were determined by immunohistochemistry. Neurodegeneration was evaluated by Luxol Fast Blue, SMI-32, and Olig2/APC staining as well as by electron microscopy and phosphorylated heavy neurofilament serum ELISA.

Results:
Treatment with anti-CD52 antibody attenuated EAE only when administered at the peak of disease. While there was no effect on the production of MP4-specific IgG, the treatment almost completely depleted CNS infiltrates and B cell aggregates even when given as late as 60 days after onset. On the ultrastructural level, we observed significantly less axonal damage in the spinal cord and cerebellum in chronic EAE after anti-CD52 treatment.

Conclusion:
Anti-CD52 treatment abrogated B cell infiltration and disrupted existing B cell aggregates in the CNS.
KW  - Alemtuzumab
KW  - B cells
KW  - CD52
KW  - CNS
KW  - EAE
KW  - MS
Y1  - 2018
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-176120
VL  - 15
IS  - 225
ER  - 
TY  - JOUR
A1  - Otto, Christoph
A1  - Friedrich, Alexandra
A1  - Madunić, Ivana Vrhovac
A1  - Baumeier, Christian
A1  - Schwenk, Robert W.
A1  - Karaica, Dean
A1  - Germer, Christoph-Thomas
A1  - Schürmann, Annette
A1  - Sabolić, Ivan
A1  - Koepsell, Hermann, Hermann
T1  - Antidiabetic Effects of a Tripeptide That Decreases Abundance of Na\(^+\)-D-glucose Cotransporter SGLT1 in the Brush-Border Membrane of the Small Intestine
JF  - ACS Omega
N2  - In enterocytes, protein RS1 (RSC1A1) mediates an increase of glucose absorption after ingestion of glucose-rich food via upregulation of Na+-D-glucose cotransporter SGLT1 in the brush-border membrane (BBM). Whereas RS1 decelerates the exocytotic pathway of vesicles containing SGLT1 at low glucose levels between meals, RS1-mediated deceleration is relieved after ingestion of glucose-rich food. Regulation of SGLT1 is mediated by RS1 domain RS1-Reg, in which Gln-Ser-Pro (QSP) is effective. In contrast to QSP and RS1-Reg, Gln-Glu-Pro (QEP) and RS1-Reg with a serine to glutamate exchange in the QSP motif downregulate the abundance of SGLT1 in the BBM at high intracellular glucose concentrations by about 50%. We investigated whether oral application of QEP improves diabetes in db/db mice and affects the induction of diabetes in New Zealand obese (NZO) mice under glucolipotoxic conditions. After 6-day administration of drinking water containing 5 mM QEP to db/db mice, fasting glucose was decreased, increase of blood glucose in the oral glucose tolerance test was blunted, and insulin sensitivity was increased. When QEP was added for several days to a high fat/high carbohydrate diet that induced diabetes in NZO mice, the increase of random plasma glucose was prevented, accompanied by lower plasma insulin levels. QEP is considered a lead compound for development of new antidiabetic drugs with more rapid cellular uptake. In contrast to SGLT1 inhibitors, QEP-based drugs may be applied in combination with insulin for the treatment of type 1 and type 2 diabetes, decreasing the required insulin amount, and thereby may reduce the risk of hypoglycemia.
KW  - chemistry
Y1  - 2020
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-230654
N1  - Lizenz: https://pubs.acs.org/page/policy/authorchoice_termsofuse.html
VL  - 5
IS  - 45
ER  - 
TY  - JOUR
A1  - Chen, Wen
A1  - Gaßner, Birgit
A1  - Börner, Sebastian
A1  - Nikolaev, Viacheslav O.
A1  - Schlegel, Nicolas
A1  - Waschke, Jens
A1  - Steinbronn, Nadine
A1  - Strasser, Ruth
A1  - Kuhn, Michaela
T1  - Atrial natriuretic peptide enhances microvascular albumin permeability by the caveolae-mediated transcellular pathway
JF  - Cardiovascular Research
N2  - Aims 
Cardiac atrial natriuretic peptide (ANP) participates in the maintenance of arterial blood pressure and intravascular volume homeostasis. The hypovolaemic effects of ANP result from coordinated actions in the kidney and systemic microcirculation. Hence, ANP, via its guanylyl cyclase-A (GC-A) receptor and intracellular cyclic GMP as second messenger, stimulates endothelial albumin permeability. Ultimately, this leads to a shift of plasma fluid into interstitial pools. Here we studied the role of caveolae-mediated transendothelial albumin transport in the hyperpermeability effects of ANP.
Methods and results 
Intravital microscopy studies of the mouse cremaster microcirculation showed that ANP stimulates the extravasation of fluorescent albumin from post-capillary venules and causes arteriolar vasodilatation. The hyperpermeability effect was prevented in mice with conditional, endothelial deletion of GC-A (EC GC-A KO) or with deleted caveolin-1 (cav-1), the caveolae scaffold protein. In contrast, the vasodilating effect was preserved. Concomitantly, the acute hypovolaemic action of ANP was abolished in EC GC-A KO and Cav-1−/− mice. In cultured microvascular rat fat pad and mouse lung endothelial cells, ANP stimulated uptake and transendothelial transport of fluorescent albumin without altering endothelial electrical resistance. The stimulatory effect on albumin uptake was prevented in GC-A- or cav-1-deficient pulmonary endothelia. Finally, preparation of caveolin-enriched lipid rafts from mouse lung and western blotting showed that GC-A and cGMP-dependent protein kinase I partly co-localize with Cav-1 in caveolae microdomains.
Conclusion 
ANP enhances transendothelial caveolae-mediated albumin transport via its GC-A receptor. This ANP-mediated cross-talk between the heart and the microcirculation is critically involved in the regulation of intravascular volume.
KW  - caveolin-1
KW  - microvessel permeability
KW  - atrial natriuretic peptide
Y1  - 2012
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-126562
N1  - Lizenzhinweis: The online version of this article has been published under an open access model. Users are entitled to use, reproduce, disseminate, or display the open access version of this article for noncommercial purposes provided that the original authorship is properly and fully attributed; the Journal, Learned Society and Oxford University Press are attributed as the original place of publication with correct citation details given; if an article is subsequently reproduced or disseminated not in its entirety but only in part or as a derivative work this must be clearly indicated.
VL  - 93
IS  - 1
ER  - 
TY  - JOUR
A1  - Kleist, Christian
A1  - Mohr, Elisabeth
A1  - Gaikwad, Sadanand
A1  - Dittmar, Laura
A1  - Kuerten, Stefanie
A1  - Platten, Michael
A1  - Mier, Walter
A1  - Schmitt, Michael
A1  - Opelz, Gerhard
A1  - Terness, Peter
T1  - Autoantigen-specific immunosuppression with tolerogenic peripheral blood cells prevents relapses in a mouse model of relapsing-remitting multiple sclerosis
JF  - Journal of Translational Medicine
N2  - Background: Dendritic cells (DCs) rendered suppressive by treatment with mitomycin C and loaded with the autoantigen myelin basic protein demonstrated earlier their ability to prevent experimental autoimmune encephalomyelitis (EAE), the animal model for multiple sclerosis (MS). This provides an approach for prophylactic vaccination against autoimmune diseases. For clinical application such DCs are difficult to generate and autoantigens hold the risk of exacerbating the disease. 

Methods: We replaced DCs by peripheral mononuclear cells and myelin autoantigens by glatiramer acetate (Copaxone ®), a drug approved for the treatment of MS. Spleen cells were loaded with Copaxone®, incubated with mitomycin C (MICCop) and injected into mice after the first bout of relapsing-remitting EAE. Immunosuppression mediated by MICCop was investigated in vivo by daily assessment of clinical signs of paralysis and in in vitro restimulation assays of peripheral immune cells. Cytokine profiling was performed by enzyme-linked immunosorbent assay (ELISA). Migration of MICCop cells after injection was examined by biodistribution analysis of 111Indium-labelled MICCop. The number and inhibitory activity of CD4+CD25+FoxP3+ regulatory T cells were analysed by histology, flow cytometry and in vitro mixed lymphocyte cultures. In order to assess the specificity of MICCop-induced suppression, treated EAE mice were challenged with the control protein ovalbumin. Humoral and cellular immune responses were then determined by ELISA and in vitro antigen restimulation assay. 

Results: MICCop cells were able to inhibit the harmful autoreactive T-cell response and prevented mice from further relapses without affecting general immune responses. Administered MICCop migrated to various organs leading to an increased infiltration of the spleen and the central nervous system with CD4+CD25+FoxP3+ cells displaying a suppressive cytokine profile and inhibiting T-cell responses. 

Conclusion: We describe a clinically applicable cell therapeutic approach for controlling relapses in autoimmune encephalomyelitis by specifically silencing the deleterious autoimmune response.
KW  - Autoimmunity
KW  - Cell therapy
KW  - Copaxone®
KW  - Immune tolerance
KW  - Mitomycin C
KW  - Relapsing-remitting MS
KW  - Regulatory T cells
Y1  - 2016
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-165787
VL  - 14
IS  - 99
ER  - 
TY  - THES
A1  - Spindler, Volker Bernd
T1  - Bedeutung der Rho-GTPasen für desmosomale Adhäsion und Pemphigus-Pathogenese
T1  - Role of Rho GTPases for desmosomal adhesion and pemphigus pathogenesis
N2  - Die Stabiltät und Integrität der Epidermis beruht zu einem großen Teil auf der intakten Funktion der Desmosomen. Diese fleckförmigen Zellkontakte vermitteln extrazellulär die Haftung zwischen den Keratinozyten durch Desmocadherine und sind intrazellulär über Adaptorproteine im Intermediärfilamentsystem des Zellskeletts verankert. Diese Funktion ist bei der Autoimmunerkrankung Pemphigus gestört, die zu intraepidermaler Blasenbildung durch Akantholyse der Keratinozyten führt. Pemphigus vulgaris (PV) und Pemphigus foliaceus (PF) stellen die beiden Hauptvarianten dar, wobei PV durch Autoantikörper gegen die Desmocadherine Desmoglein (Dsg) 3 und oftmals zusätzlich gegen Dsg 1, PF durch Autoantikörper nur gegen Dsg 1 gekennzeichnet ist. Rho-GTPasen sind zelluläre Regulatorproteine, die das Aktinzytoskelett und verschiedene Zellkontakte beeinflussen. Die vorliegende Arbeit beschäftigte sich mit dem Einfluss von Rho-GTPasen bei der Regulation von desmosomal vermittelter Adhäsion. In einem zweiten Teil wurde die Beteiligung von Rho-GTPasen bei den Pemphigusvarianten PV und PF näher charakterisiert. Für den ersten Abschnitt wurden bakterielle Toxine verwendet, die spezifisch Rho GTPasen aktivieren bzw. inhibieren, während für den zweiten Teil IgG-Fraktionen von PV- und PF-Patienten in Kombination mit aktivierenden Toxinen zur Anwendung kamen. Eine Inhibition der drei Hauptvertreter der Rho-GTPasen in kultivierten Keratinozyten und humaner Epidermis führte zu einer Rarefizierung des Aktinfilamentsystems, zu Verlust von membranständig lokalisiertem Dsg 1 und 3 und zu Zelldissoziation sowie zu verminderter Dsg 1 und 3-vermittelter Haftung von Mikroperlen auf der Oberfläche von Keratinozyten. Die Aktivierung der GTPasen resultierte in vermehrter linearisierter Darstellbarkeit von Aktin und Dsg 3 an den Zellgrenzen und einer verstärkten Dsg-vermittelten Haftung. Pemphigus-IgG führten ebenfalls zu Zelldissoziation und Verlust von Dsg-Immunreaktivität in Keratinozytenkulturen, zu Spaltbildung in humaner Epidermis und zum Verlust der durch Dsg 1 und Dsg 3 vermittelten Adhäsion. Dies ging einher mit einer vermehrten Menge an nicht am Zytoskelett verankerten Dsg 3 und wurde durch eine p38MAPK-abhängige Verminderung der Aktivität von Rho A moduliert. Die Aktivierung von Rho A verhinderte die Ausbildung der Pemphigus-induzierten Effekte nahezu vollständig. Zusammenfassend regulieren Rho-GTPasen die desmosomale Haftung in Keratinozyten. Die Daten zeigen weiterhin, dass Pemphigus-IgG durch eine Inhibition von Rho A diese Regulation beeinträchtigt, was zu Schwächung der Zytoskelettverankerung von Desmogleinen und zu Haftungsverlust und Spaltbildung führt. Somit ist Rho A ein wichtiger Faktor der Pemphigus-Pathogenese und stellt einen Erfolg versprechenden Ansatzpunkt zur Entwicklung neuer Therapieoptionen dar.
N2  - Integrity and stability of human epidermis is based on the correct function of desmosomes. These spot-like cell contacts mediate adhesion of adjacent keratinocytes by desmosomal cadherins and are linked via adapter proteins to the intermediate filament cytoskeleton. This function is impaired in the autoimmune disease pemphigus, resulting in intraepidermal blister formation by akantholysis of keratinocytes. Pemphigus vulgaris (PV) and pemphigus foliaceus (PF) are the main subtypes of pemphigus, with PV being characterized by autoantibodies targeting the desmosomal cadherins Desmoglein (Dsg) 3 and in part Dsg1. PF patients develeop autoantibodies against Dsg1 only. Rho GTPases are regulatory proteins which are known to modulate the actin cytoskeleton and different cell contacts. The aim of this thesis was to evaluate the role of Rho GTPases in the regulation of desmosome-mediated adhesion. The second part addresses the involvement of Rho GTPases in the pathogenesis of PV and PF. Toxins served to activate or inactivate specific GTPases in the first part, whereas in the latter part purified IgG fractions of pemphigus patients were used in combination with Rho activating toxins. An inhibition of the three best characterized GTPases in cultured keratinocytes and human epidermis resulted in rarefication of the actin cytoskeleton, loss and fragmentation of membrane-localized Dsg1 and Dsg3 immunostaining, cell dissociation and reduced adhesion of Dsg1 and Dsg3-coated microbeads on the cell surface of keratinocytes. Activation of GTPases led to linearized immunoreactivity of Dsg3 at the cell membrane, pronounced cortical actin staining and strengthened Dsg-mediated adhesion. Similarily to inhibition of Rho-GTPases, Pemphigus IgG caused cell dissociation and loss of Dsg staining in cultured keratinocytes, blister formation in human epidermis and reduction of Dsg-mediated adhesion. These changes were accompanied by a decrease of cytoskeleton-bound Dsg3 and were modulated by a p38MAPK-dependent reduction of RhoA activity. Activation of RhoA blocked the Pemphigus IgG-induced effects. Taken together, Rho GTPases regulate desmosomal adhesion in keratinocytes. Additionaly, Pemphigus IgG interfere with this regulation by inhibition of RhoA, resulting in reduced cytoskeletal anchorage of desmogleins, reduced intercellular adhesion and gap formation. Thus RhoA is identified as an important factor in pemphigus pathogenesis and might eventually serve as a target of new therapy approaches.
KW  - Zelladhäsion
KW  - Pemphigus
KW  - Rho-Proteine
KW  - Desmosom
KW  - Epidermis
KW  - Desmoglein
KW  - Keratinozyten
KW  - cell adhesion
KW  - desmosome
KW  - rho GTPases
KW  - keratinocytes
KW  - pemphigus
Y1  - 2009
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-38728
ER  - 
TY  - THES
A1  - Hübner, Lisa-Christina
T1  - Bedeutung von neuroendokrinen Zellen für die Signalübertragung an sensorischen Nervenfasern in den Atemwegen
T1  - Importance of neuroendocrine cells in the respiratory tracts of mice which connect to sensory nervous fibers
N2  - Die vorliegende Arbeit hatte zum Ziel, neuroendokrine Zellen in den Atemwegen bei Mäusen zu untersuchen, welche Kontakt zu sensorischen Nervenfasern ausbilden. In vorangegangenen Versuchen konnte bereits die Menge des ausgeschütteten CGRPs nach Stimulation mit Bitterstoffen bestimmt werden. Die Methode zur Messung der Freisetzung von CGRP aus verschiedenen Organen wurde von Prof. Reeh und seiner Arbeitsgruppe etabliert. Ziel der vorliegenden Arbeit war es, zu untersuchen, woher das ausgeschüttete CGRP kommt und ob die Stimulation von Bürstenzellen mit Bitterstoffen zur Ausschüttung von CGRP aus den neuroendokrinen Zellen führt. Anhand der elektronenmikroskopischen Auswertung und der dreidimensionalen Rekonstruktion konnte gezeigt werden, dass es Kontakt zwischen den neuroendokrinen Zellen im Epithel der Trachea und sensorischen Nervenfasern gibt. Die immunhistochemischen Versuche zeigten, dass es nach Stimulation mit Denatonium höchstwahrscheinlich zur Ausschüttung von CGRP durch die intraepithelialen Fasern gekommen ist. Diese Annahme spiegelt sich in der veränderten Morphologie sowie der geringeren Quantität der intraepithelialen Fasern nach Stimulation mit Denatonium deutlich wider. Dass es weder bei der Anzahl der neuroendokrinen Zellen, noch bei der Erscheinung und Anzahl der extraepithelialen Fasern nach Denatoniumstimulation zu einer Veränderung gekommen ist, unterstützt diese Annahme ebenfalls. Im Hinblick auf die durchgeführten Versuche mit den TRPM5-gendefizienten Mäusen zeigte sich, dass die Stimulation mit Denatonium keine Auswirkungen auf die Anzahl der neuroendokrinen Zellen hatte. Dieses Ergebnis unterstützt die Erkenntnisse der vorangegangenen Untersuchungen, welche gezeigt haben, dass das CGRP nicht von den neuroendokrinen Zellen ausgeschüttet wurde. Des Weiteren lässt das Ergebnis darauf schließen, dass die Ausschüttung von CGRP nicht abhängig von der Anwesenheit von Bürstenzellen ist. Insgesamt zeigen die Untersuchungen, dass es nach Stimulation mit Bittersubstanzen zu einer CGRP-Ausschüttung durch die intraepithelialen Fasern gekommen ist. Interessant wäre es weiterhin zu klären, welche Effekte diese Ausschüttung bewirkt und welche Bedeutung der Freisetzung von Substanz P in diesem Zusammenhang zukommt.
N2  - This thesis focused on the objective to investigate the neuroendocrine cells in the respiratory tracts of mice which connect to sensory nervous fibers. In the preceding trials it was possible to determine the amount of the released CGRP after the stimulation with bitter substances. The method of measuring the release of CGRP from a variety of organs was established by Prof. Reeh and his working group. The aim of this work was to investigate where the released CGRP originates from and if the stimulation of brush cells with bitter substances leads to the release of CGRP in the neuroendocrine cells. Based on the electron-microscopic analysis and the three dimensional reconstruction, a correlation between the neuroendocrine cells in the epithelium of mice trachea and the sensory nervous fibers was observed. The immunhistochemical examinations displayed that the stimulation with Denatonium most probably leads to the release of CGRP through intraepithelial fibers. This presumption is reflected in the changed morphology as well as the lower quantity of intraepithelial fibers after the stimulation with Denatonium. Furthermore, the presumption is supported by the fact that neither the number of neuroendocrine cells, nor the appearance and number of extraepithelial fibers led to a change after denationium stimulation. With regards to the executed trials with TRPM5 gene-deficient mice it was observed that the stimulation with Denatonium does not impact the number of neuroendocrine cells. This again supports the finding of the previous trials which showed that CGRP was not released by neuroendocrine cells. Moreover, it can be concluded from this result that the release of CGRP is independent from the existence of brush cells. Overall the trials showed that the release of CGRP through intraepithelial fibers was triggered by the stimulation with bitter substances. Based on these results it would be interesting to investigate the effects of the release and to understand the role of substance P in this correlation.
KW  - Luftröhre
KW  - Luftröhrenschleimhaut
KW  - Signaltransduktion
KW  - Neuroendokrine Zellen
KW  - Signalübertragung
KW  - Trachea
KW  - neuroendocrine cells
KW  - signal transmission
Y1  - 2020
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-207517
ER  - 
TY  - THES
A1  - Semlanski, Christin Martina
T1  - Beeinflussung der Substratbindungsregion des organischen Kationentransporters 1 der Ratte durch Mutation einer intrazellulär gelegenen Aminosäure
T1  - The Influence of the Substrate Binding Region of the rOCT 1 via Mutation of an intracellular Aminoacid
N2  - 1994 wurde von Gründemann et al. der erste organische Kationentransporter, der rOCT1 beschrieben. Es wurden bereits einige Aminosäuren identifiziert, die bei der Bindung kationischer Substanzen beteiligt sind. Hierbei handelt es sich um Phenylalanin 160 der zweiten Transmembrandomäne, Tryptophan 218, Tyrosin 222 und Threonin 226 der vierten Transmembrandomäne, um Arginin 440, Leucin 447, Glutamin 448 der zehnten und um Aspartat 475 der elften Transmembrandomäne. Hintergrund der Versuche dieser Arbeit war das im Jahre 2005 von Sturm et al. identifizierte Cystein 451. Es liegt zwischen der zehnten und elften Transmembrandomäne. Cystein 451 ist wahrscheinlich auf Grund seiner Lage im Strukturmodell nicht direkt an der Bindung von Substraten beteiligt. Es wird vermutet, dass die Mutation des Cysteins 451 die Positionen von Aminosäuren in der Bindungsstelle verändert. Daher wurden die Mutante C451M, die Doppelmutanten L447F/C451M, L447Y/C451M und die Dreifachmutante Y222F/L447F/C451M mittels Tracer-Fluxexperimenten hinsichtlich der Hemmung der Tetraethylammonium-Aufnahme durch Kortikosteron und durch Tetrabutylammonium untersucht. Die Mutation C451M steigert verglichen mit dem rOCT1-Wildtyp die Affinität für Kortikosteron, jedoch sinkt bei dieser Mutante die TBuA-Affinität. Man nimmt nun aufgrund dieser Mutageneseversuche und den bereits zuvor generierten Modellen des rOCT1 an, dass aufgrund seiner Lage Cystein 451 nicht direkt an der Bindung von Substraten beteiligt ist, sondern einen indirekten Effekt auf die Substratbindungsregion des Transporters ausübt. Weiterhin wurde festgestellt, dass die Mutanten L447Y/C451M und L447F/C451M gegensätzliche Affinitäten für TBuA und Kotikosteron haben. Tauscht man das Leucin an Position 447 gegen ein Tyrosin aus, so wird der Transporter weniger affin für Kortikosteron, jedoch steigt die TBuA-Affinität. Tauscht man das Leucin gegen ein Phenylalanin aus, verhält es sich gegensätzlich. Die Position 222 scheint weder an der TBuA-Bindung, noch an der Bindung von Kortikosteron maßgeblich beteiligt zu sein.
N2  - In 1994 Gründemann et al. described the first organic cation transporter, called rOCT1. Several previous studies revealed some amino acids, which are critical for substrate binding. In 2005 Sturm et al. identified the cysteine on position 451. It is located between the tenth and eleventh TMH. Because of its position in the structure model cysteine 451 might not be directly involved in substrate binding. However it is postulated, that mutation of C451 alters the position of amino acids in the substrate binding region. The mutation on C451 is the basis for this work. Concerning the inhibition of the TEA uptake by corticosterone or TBuA the mutants C451M, L447F/C451M, L447Y/C451M and Y222F/L447F/C451M were analyzed by tracer uptake measurements. The TEA uptake measurements showed that the replacement of cysteine 451 by methionine resulted in an increased affinity for corticosterone and a decreased affinity for TBuA. The present work together with the proposed localization of cysteine 451 in the tertiary structure of rOCT1 further support the idea that cysteine 451 is not directly-involved in ligand binding, but it seems to exert an indirect effect on the substrate binding region of the transporter, which alters its affinity for TBuA and corticosterone. The affinity for corticosterone and TBuA of the mutants L447F/C451M and L447Y/C451M was opposed. When L447 was replaced by a tyrosine the affinity for corticosterone was decreased, but the affinity for TBuA was increased. Though, when leucine was replaced by phenylalanine the affinity for corticosterone was increased and the affinity for TBuA was decreased. The position 222 seems to be unimportant concerning the linkage of corticosterone and TBuA
KW  - Cytologie
KW  - Cytologie
Y1  - 2011
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-65672
ER  - 
TY  - JOUR
A1  - Trávníček, Bohumil
A1  - Meierott, Lenz
A1  - Žíla, Vojtĕch
T1  - Beiträge zur Gattung Taraxacum in Bayern
T1  - Contribution to the genus Taraxacum in Bavaria
JF  - Forum Geobotanicum
N2  - Eine Reihe mehrtägiger Suchexkur-sionen / Transekte in verschiedene Regionen Bayerns in den Jahren 2011 bis 2014 waren der Gattung Taraxacum gewidmet. Unter den gesammelten und beobachteten Arten ist Taraxacum broddesonii (sect. Ruderalia / Taraxacum) neu für Deutschland. Neu für Bayern sind Taraxacum fusciflorum, marklundii, spiculatum (sect. Hamata) und Taraxacum acroglossum, atroviride, clarum, floccosum, freticola, glossodon, hemicyclum, homoschistum, infuscatum, intumescens, lacinulatum, leucopodum, lundense, ottonis, pallidipes, praestabile, pseudoretroflexum, pulverulentum, saxonicum, sellandii, sundbergii, uncidentatum, uniforme, violaceinervosum (sect. Ruderalia / Taraxacum). Taraxacum lojoënse wird als ältester und korrekter Name für T. lippertianum und T. matricium und wahrscheinlich auch für T. ampelophytum und T. debrayi angesehen. Seltenere Arten sind abgebildet.
N2  - Several excursions in selected regions of Bavaria were undertaken in the years 2011-2014 to broaden our knowledge of the genus Taraxacum in Bavaria. Among the observed and collected species Taraxacum broddesonii (sect. Ruderalia / Taraxacum) is new for Germany, and the following species are new for Bavaria: Taraxacum fusciflorum, marklundii, spiculatum (sect. Hamata) and Taraxacum acroglossum, atroviride, clarum, floccosum, freticola, glossodon, hemicyclum, homoschistum, infuscatum, intumescens, lacinulatum, leucopodum, lundense, ottonis, pallidipes, praestabile, pseudo-retroflexum, pulverulentum, saxonicum, sellandii, sundbergii, uncidentatum, uniforme, violaceinervosum (sect. Ruderalia / Taraxacum). Taraxacum lojoënse is accepted as the oldest and correct name for T. lippertianum and T. matricium and probably also for T. ampelophytum and T. debrayi. The more remarkable and rare species are depicted by herbarium specimen.
KW  - Taraxacum
KW  - Bayern
KW  - Kuhblume
KW  - Löwenzahn <Taraxacum>
KW  - Kettenblume
KW  - Bayern
KW  - Bavaria
KW  - dandelion
Y1  - 2015
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-126782
UR  - http://www.forum-geobotanicum.net/articles/vol_6-2012/travnicek_taraxacum/Taraxacum-Bayern-FG-6-S20-49-2015.pdf
SN  - 1867-9315
VL  - Vol. VI
ER  - 
TY  - THES
A1  - Schampel, Andrea
T1  - Beneficial therapeutic effects of the L-type calcium channel antagonist nimodipine in experimental autoimmune encephalomyelitis – an animal model for multiple sclerosis
T1  - Günstige therapeutische Effekte des L-Typ-Calciumkanal-Antagonisten Nimodipin in der experimentellen autoimmunen Enzephalomyelitis  ̶  einem Tiermodell der Multiplen Sklerose
N2  - Multiple sclerosis (MS) is the most prevalent neurological disease of the central nervous system (CNS) in young adults and is characterized by inflammation, demyelination and axonal pathology that result in multiple neurological and cognitive deficits. The focus of MS research remains on modulating the immune response, but common therapeutic strategies are only effective in slowing down disease progression and attenuating the symptoms; they cannot cure the disease. Developing an option to prevent neurodegeneration early on would be a valuable addition to the current standard of care for MS. Based on our results we suggest that application of nimodipine could be an effective way to target both neuroinflammation and neurodegeneration. We performed detailed analyses of neurodegeneration in experimental autoimmune encephalomyelitis (EAE), an animal model of MS, and in in vitro experiments regarding the effect of the clinically well-established L-type calcium channel antagonist nimodipine. Nimodipine treatment attenuated the course of EAE and spinal cord histopathology. Furthermore, it promoted remyelination. The latter could be due to the protective effect on oligodendrocytes and oligodendrocyte precursor cells (OPCs) we observed in response to nimodipine treatment. To our surprise, we detected calcium channel-independent effects on microglia, resulting in apoptosis. These effects were cell type-specific and independent of microglia polarization. Apoptosis was accompanied by decreased levels of nitric oxide (NO) and inducible NO synthase (iNOS) in cell culture as well as decreased iNOS expression and reactive oxygen species (ROS) activity in EAE. Overall, application of nimodipine seems to generate a favorable environment for regenerative processes and could therefore be a novel treatment option for MS, combining immunomodulatory effects while promoting neuroregeneration.
N2  - Multiple Sklerose (MS) ist die häufigste neurologische Erkrankung des zentralen Nervensystems (ZNS) von jungen Erwachsenen und charakterisiert durch Inflammation, Demyelinisierung und axonale Pathologie. Diese Prozesse bewirken zahlreiche neurologische und kognitive Defizite. Der Schwerpunkt in der MS-Forschung besteht derzeit vor allem in der Modulation der Immunantwort, jedoch sind herkömmliche Therapiestrategien bislang nur in der Lage die Progression der Erkrankung zu verlangsamen und die Symptome zu lindern, die Krankheit kann jedoch immer noch nicht geheilt werden. Die Möglichkeit, den Prozess der Neurodegeneration früh aufzuhalten, würde eine wertvolle Ergänzung zu herkömmlichen Therapien darstellen. Basierend auf den Ergebnissen dieser Studie schlagen wir vor, dass die Applikation von Nimodipin eine elegante Möglichkeit wäre, um sowohl die Neuroinflammation als auch die -degeneration zu bekämpfen. Um den Effekt des klinisch gut etablierten Calciumkanal-Antagonisten Nimodipin zu untersuchen, haben wir detaillierte Analysen der Degeneration in der experimentellen autoimmunen Enzephalomyelitis (EAE), einem Tiermodell der MS, und in in vitro Untersuchungen durchgeführt. Applikation von Nimodipin verringerte das klinische Erscheinungsbild der EAE sowie die Histopathologie des Rückenmarkes. Außerdem förderte es die Regeneration. Die Ursache für letzteres liegt vermutlich am protektiven Effekt der Behandlung mit Nimodipin auf die Oligodendrozyten und deren Vorläuferzellen. Überraschenderweise, konnten wir Calciumkanal-unspezifische Effekte auf Mikroglia feststellen, die in Apoptose resultierten und sowohl Zelltyp-spezifisch als auch unabhängig von der Polarisierung der Mikrogliazellen waren. Apoptose wurde begleitet von reduzierten Spiegeln an Stickstoffmonoxid (NO) und der induzierbaren NO Synthase (iNOS) in Zellkultur, sowie einer reduzierten Expression von iNOS und dem geringeren Vorkommen von reaktiven oxygenen Spezies (ROS) in der EAE. Zusammenfassend gehen wir davon aus, dass die Applikation von Nimodipin eine günstige Umgebung für regenerative Prozesse schafft. Daher stellt die Applikation dieser Substanz eine neue Behandlungsmöglichkeit für die MS dar, insbesondere da sie Möglichkeiten der Immunmodulation mit der Förderung von Neuroregeneration verbindet.
KW  - Nimodipin
KW  - Multiple Sklerose
KW  - l-type calcium channel antagonist
KW  - experimental autoimmune encephalomyelitis
KW  - L-typ Calciumkanal Antagonist
KW  - experimentelle autoimmune Enzephalomyelitis
KW  - neuroprotection
KW  - multiple sclerosis
Y1  - 2017
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-148952
ER  - 
TY  - THES
A1  - Laymann, Bettina
T1  - Bindung der extrazellulären Domäne von N-Cadherin an den Fibroblastenwachstumsfaktor-Rezeptor FGFR-1
N2  - N-Cadherin, ein Mitglied der klassischen Cadherin Familie vermittelt durch homophile Bindungen der extrazellulären Domänen (EZD) zwischen benachbarten Zellen Zell-Zell-Kontakte. Im Nervensystem kontrolliert es zahlreiche Aufgaben wie beispielsweise die Ausbildung von Synapsen, die synaptische Plastizität, das Auswachsen von Axonen und deren richtungsgezielte Orientierung. In Untersuchungen zum Axonwachstum von cerebellären Körnerzellen konnte von Doherty et al. (1995, 1996) gezeigt werden, dass die isolierte EZDI-V von N-Cadherin über den FGFR-1 (Fibroblastenwachstumsfaktor-Rezeptor-1) ein richtungsvermitteltes Auswachsen von Axonen verursacht. Basierend auf diesen Beobachtungen wurde ein Bindungsmodell erstellt (Doherty et al., 1996). Dieses geht davon aus, dass zwischen transdimeren N-Cadherin-Molekülen, über die Aminosäuren IDPVNGQ der EZD Wechselwirkungen mit den Aminosäuren HAV der EZD von FGFR-1 auftreten (siehe hierzu Abb. 17). Der dadurch dimerisierte FGFR-1 bewirkt innerhalb der Nervenzelle eine intrazelluläre Signaltransduktion, die in einem zielgerichteten Axonwachstum resultiert. Das Ziel der vorliegenden Arbeit war, dieses Bindungsmodell näher zu untersuchen. Ausgehend von den für N-Cadherin und FGFR-1 kodierenden cDNAs und entsprechenden Vektorsystemen wurden in CHO-Zellen stabile Zelllinien erstellt. Das zugrundeliegende Expressionssystem führte zu einem Ausschleusen der für die Experimente notwendigen Fc-Fusionsproteine in den Kulturüberstand. Eine daran anschließende auf Protein A basierende Affinitätschromatographie des Kulturüberstandes ermöglichte die Isolierung und Anreicherung der Fc-Fusionsproteine. Desweiteren wurden Expressionsvektoren verwendet, die für subzelluläre Lokalisationsuntersuchungen verwendet wurden. Zu Beginn der Bindungsstudien wurde Untersuchungen zum Axonwachstum cerebellärer Körnerzellen durchgeführt. Diese dienten zum einen der Überprüfung der von Doherty und Walsh (1996) durchgeführten Experimente zum Längenwachstum cerebellärer Körnerzellen in Gegenwart ausgewählter Zelladhäsionsmoleküle (NCAM, L1 und N-Cadherin), zum anderen dienten sie der Überprüfung der Funktionalität der FGFR-1-und N-Cadherin-spezifischen Peptide (HAV und IDPVNGQ). Wie zu erwarten wurde durch Zugabe von N-Cadherin EZDI-V ein Axonlängenwachstum festgestellt, dass durch Zugabe der HAV- und IDPVNGQ-Peptide inhibiert wurde. Für den Auschluß der Wirkung von Fremdproteinen wurden in der vorliegenden Arbeit direkte Bindungsstudien durchgeführt. Hierzu wurden sowohl ELISA- als auch in Dot-Blot-Experimente durchgeführt. Diese ergaben eine Wechselwirkung der EZD von FGFR-1 und N-Cadherin. Eine von DsRed-FGFR-1 abhängige Lokalisation von GFP-N-Cadherin in CHO-Zellen deutete ebenfalls auf eine Interaktion hin. Nähere Bindungsstudien zeigten, dass die Bindungsmotive IDPVNGQ und HAV für eine Wechselwirkung der FGFR-1- und N-Cadherin-spezifischen EZDs bedeutungslos sind. Auch an der Laserpinzette durchgeführte Untersuchungen ergaben, das Wechselwirkungen zwischen N-Cadherin (auf Mikroperlen immobilisiert) und PC12-Zellen in Gegenwart der inhibierenden IDPVNGQ- und HAV-Peptide nicht verhindert werden konnten. Zusammenfasssend ist es gelungen zum ersten Mal eine direkte Wechselwirkung zwischen N-Cadherin und FGFR-1 nachzuweisen. Allerdings konnte in Kompetitionsexperimenten eine Bedeutung der postulierten Bindungsmotive nicht bestätigt werden.
N2  - N-cadherin, a member of the classic cadherin family, mediates intercellular contacts between neighbouring cells through homophile bonds. In the nervous system, it is involved in numerous functions, such as the formation of synapses, synaptic plasticity, the development of axons and their spatio-controlled orientation. In studies regarding axonal growth of cerebellar granule cells, Doherty et al., (1995, 1996) were able to demonstrate that the isolated extracellular domain I-V (ECDI-V) of N-cadherin together with FGFR-1 (Fibroblast Growth Factor Receptor-1) induces directional development of axons. Based on these observations, a bonding model was derived (Doherty et al., 1996), assuming that ECD-directed interactions with the HAV amino acids of the FGFR-1-ECD occur via the IDPVNGQ amino acids from the ECD of N-cadherin (see Fig. 17). Consequently, dimerized FGFR-1 induce intracellular signalling within the nerve cells, resulting in continuous axonal growth. The aim of this thesis was to examine the bonding model in more detail. In order to conduct studies of interactions between N-cadherin and FGFR-1 respective expression vectors were constructed and used to generate stable cell lines for protein production. Subsequent to expression and secretion of the fusion proteins into the supernatant, purification was performed by protein A-specific affinity chromatography. In addition expression vectors were generated suitable for investigating subcellular localization of N-cadherin-GFP in the presence /absence of FGFR-1-dsRed. Initial binding studies were conducted on cerebellar granule cells, firstly to confirm CAM-dependency of axonal growth as shown by Doherty and Walsh (1996) and secondly functionality of the inhibitory FGFR-1- and N-cadherin-specific peptides (HAV and IDPVNGQ) on N-cadherin binding activity. As expected, addition of N-cadherin EZDI-V to cerebellar granule cells resulted into axonal growth, whereas the presence of the inhibitory HAV- und IDPVNGQ-peptides reduced binding of N-cadherin EZDI-V to cerebellar granule cells significantly. To exclude unspecifity of protein interactions in such complex binding studies, protein-protein interactions were performed by either ELISA- and Dot-Blot-Assays. In both assays interaction between the ECD of N-cadherin and FGFR-1 was detected. FGFR-1-dsRed-dependent localization of N-cadherin-EGFP in CHO-cells additionally indicated interaction between both proteins. Detailed binding studies revealed no effect of the inhibitory binding peptides HAV und IDPVNGQ on the ECD-interaction of N-cadherin and FGFR-1. Supporting these results was the observation, that in laser tweezer experiments binding of N-cadherin EZDI-V (immobilized onto microbeads) to cultured PC-12 cells could not be prevented by the inhibitory binding peptides HAV und IDPVNGQ. In conclusion, this thesis demonstrates for the first time binding of the ECD of N-cadherin to that of FGFR-1. However, the significance of the binding motives HAV und IDPVNGQ for N-cadherin/FGFR- interaction could not be confirmed in competition experiments and remains questionable.
KW  - Cadherine
KW  - Fibroblastenwachstumsfaktor
KW  - Zell-Adhäsionsmolekül
KW  - Nervenzelle
KW  - fibroblastenwachstumsfaktor-rezeptor
KW  - ---
Y1  - 2008
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-26974
ER  - 
TY  - JOUR
A1  - Horder, Hannes
A1  - Guaza Lasheras, Mar
A1  - Grummel, Nadine
A1  - Nadernezhad, Ali
A1  - Herbig, Johannes
A1  - Ergün, Süleyman
A1  - Teßmar, Jörg
A1  - Groll, Jürgen
A1  - Fabry, Ben
A1  - Bauer-Kreisel, Petra
A1  - Blunk, Torsten
T1  - Bioprinting and differentiation of adipose-derived stromal cell spheroids for a 3D breast cancer-adipose tissue model
JF  - Cells
N2  - Biofabrication, including printing technologies, has emerged as a powerful approach to the design of disease models, such as in cancer research. In breast cancer, adipose tissue has been acknowledged as an important part of the tumor microenvironment favoring tumor progression. Therefore, in this study, a 3D-printed breast cancer model for facilitating investigations into cancer cell-adipocyte interaction was developed. First, we focused on the printability of human adipose-derived stromal cell (ASC) spheroids in an extrusion-based bioprinting setup and the adipogenic differentiation within printed spheroids into adipose microtissues. The printing process was optimized in terms of spheroid viability and homogeneous spheroid distribution in a hyaluronic acid-based bioink. Adipogenic differentiation after printing was demonstrated by lipid accumulation, expression of adipogenic marker genes, and an adipogenic ECM profile. Subsequently, a breast cancer cell (MDA-MB-231) compartment was printed onto the adipose tissue constructs. After nine days of co-culture, we observed a cancer cell-induced reduction of the lipid content and a remodeling of the ECM within the adipose tissues, with increased fibronectin, collagen I and collagen VI expression. Together, our data demonstrate that 3D-printed breast cancer-adipose tissue models can recapitulate important aspects of the complex cell–cell and cell–matrix interplay within the tumor-stroma microenvironment
KW  - adipose-derived stromal cells
KW  - adipose tissue
KW  - bioprinting
KW  - breast cancer model
KW  - extracellular matrix
KW  - hyaluronic acid
KW  - spheroids
Y1  - 2021
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-236496
VL  - 10
IS  - 4
ER  - 
TY  - JOUR
A1  - Tsfasman, I. M.
A1  - Nesmeyanova, M. A.
A1  - Gorboulev, Valentin G.
A1  - Rubtsov, P. M.
A1  - Skryabin, K. G.
T1  - Biosynthesis and secretion of bovine growth hormone in Escherichia coli under the control of the secretory vector containing a promoter and signal sequence of alkaline phosphatase gene
N2  - A recombinant plasmid was constructed containing the gene for bovine growth hormone joinea with the regulatory region and the region coding the signal sequence of the Escherichia coli alkaline phosphatase gene. In conditions of phosphorus starvation, which c~s derepression of alkaline phosphatase, expression was shown of the gene for bovine growth hormone, in addition to partial processing and secretion of protein into periplasm.
Y1  - 1989
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-46932
ER  - 
TY  - JOUR
A1  - Göbel, Kerstin
A1  - Pankratz, Susann
A1  - Asaridou, Chloi-Magdalini
A1  - Herrmann, Alexander M.
A1  - Bittner, Stefan
A1  - Merker, Monika
A1  - Ruck, Tobias
A1  - Glumm, Sarah
A1  - Langhauser, Friederike
A1  - Kraft, Peter
A1  - Krug, Thorsten F.
A1  - Breuer, Johanna
A1  - Herold, Martin
A1  - Gross, Catharina C.
A1  - Beckmann, Denise
A1  - Korb-Pap, Adelheid
A1  - Schuhmann, Michael K.
A1  - Kuerten, Stefanie
A1  - Mitroulis, Ioannis
A1  - Ruppert, Clemens
A1  - Nolte, Marc W.
A1  - Panousis, Con
A1  - Klotz, Luisa
A1  - Kehrel, Beate
A1  - Korn, Thomas
A1  - Langer, Harald F.
A1  - Pap, Thomas
A1  - Nieswandt, Bernhard
A1  - Wiendl, Heinz
A1  - Chavakis, Triantafyllos
A1  - Kleinschnitz, Christoph
A1  - Meuth, Sven G.
T1  - Blood coagulation factor XII drives adaptive immunity during neuroinflammation via CD87-mediated modulation of dendritic cells
JF  - Nature Communications
N2  - Aberrant immune responses represent the underlying cause of central nervous system (CNS) autoimmunity, including multiple sclerosis (MS). Recent evidence implicated the crosstalk between coagulation and immunity in CNS autoimmunity. Here we identify coagulation factor XII (FXII), the initiator of the intrinsic coagulation cascade and the kallikrein–kinin system, as a specific immune cell modulator. High levels of FXII activity are present in the plasma of MS patients during relapse. Deficiency or pharmacologic blockade of FXII renders mice less susceptible to experimental autoimmune encephalomyelitis (a model of MS) and is accompanied by reduced numbers of interleukin-17A-producing T cells. Immune activation by FXII is mediated by dendritic cells in a CD87-dependent manner and involves alterations in intracellular cyclic AMP formation. Our study demonstrates that a member of the plasmatic coagulation cascade is a key mediator of autoimmunity. FXII inhibition may provide a strategy to combat MS and other immune-related disorders.
KW  - blood coagulation
KW  - factor XII
KW  - neuroinflammation
KW  - dendric cells
Y1  - 2016
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-165503
VL  - 7
IS  - 11626
ER  - 
TY  - JOUR
A1  - Kleefeldt, Florian
A1  - Upcin, Berin
A1  - Bömmel, Heike
A1  - Schulz, Christian
A1  - Eckner, Georg
A1  - Allmanritter, Jan
A1  - Bauer, Jochen
A1  - Braunger, Barbara
A1  - Rueckschloss, Uwe
A1  - Ergün, Süleyman
T1  - Bone marrow-independent adventitial macrophage progenitor cells contribute to angiogenesis
JF  - Cell Death & Disease
N2  - Pathological angiogenesis promotes tumor growth, metastasis, and atherosclerotic plaque rupture. Macrophages are key players in these processes. However, whether these macrophages differentiate from bone marrow-derived monocytes or from local vascular wall-resident stem and progenitor cells (VW-SCs) is an unresolved issue of angiogenesis. To answer this question, we analyzed vascular sprouting and alterations in aortic cell populations in mouse aortic ring assays (ARA). ARA culture leads to the generation of large numbers of macrophages, especially within the aortic adventitia. Using immunohistochemical fate-mapping and genetic in vivo-labeling approaches we show that 60% of these macrophages differentiate from bone marrow-independent Ly6c\(^{+}\)/Sca-1\(^{+}\) adventitial progenitor cells. Analysis of the NCX\(^{−/-}\) mouse model that genetically lacks embryonic circulation and yolk sac perfusion indicates that at least some of those progenitor cells arise yolk sac-independent. Macrophages represent the main source of VEGF in ARA that vice versa promotes the generation of additional macrophages thereby creating a pro-angiogenetic feedforward loop. Additionally, macrophage-derived VEGF activates CD34\(^{+}\) progenitor cells within the adventitial vasculogenic zone to differentiate into CD31\(^{+}\) endothelial cells. Consequently, depletion of macrophages and VEGFR2 antagonism drastically reduce vascular sprouting activity in ARA. In summary, we show that angiogenic activation induces differentiation of macrophages from bone marrow-derived as well as from bone marrow-independent VW-SCs. The latter ones are at least partially yolk sac-independent, too. Those VW-SC-derived macrophages critically contribute to angiogenesis, making them an attractive target to interfere with pathological angiogenesis in cancer and atherosclerosis as well as with regenerative angiogenesis in ischemic cardiovascular disorders.
KW  - macrophages
KW  - angiogenesis
KW  - bone marrow-derived monocytes
Y1  - 2022
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-299724
VL  - 13
IS  - 3
ER  - 
TY  - JOUR
A1  - Koeniger, Tobias
A1  - Bell, Luisa
A1  - Mifka, Anika
A1  - Enders, Michael
A1  - Hautmann, Valentin
A1  - Mekala, Subba Rao
A1  - Kirchner, Philipp
A1  - Ekici, Arif B.
A1  - Schulz, Christian
A1  - Wörsdörfer, Philipp
A1  - Mencl, Stine
A1  - Kleinschnitz, Christoph
A1  - Ergün, Süleyman
A1  - Kuerten, Stefanie
T1  - Bone marrow‐derived myeloid progenitors in the leptomeninges of adult mice
JF  - Stem Cells
N2  - Although the bone marrow contains most hematopoietic activity during adulthood, hematopoietic stem and progenitor cells can be recovered from various extramedullary sites. Cells with hematopoietic progenitor properties have even been reported in the adult brain under steady‐state conditions, but their nature and localization remain insufficiently defined. Here, we describe a heterogeneous population of myeloid progenitors in the leptomeninges of adult C57BL/6 mice. This cell pool included common myeloid, granulocyte/macrophage, and megakaryocyte/erythrocyte progenitors. Accordingly, it gave rise to all major myelo‐erythroid lineages in clonogenic culture assays. Brain‐associated progenitors persisted after tissue perfusion and were partially inaccessible to intravenous antibodies, suggesting their localization behind continuous blood vessel endothelium such as the blood‐arachnoid barrier. Flt3\(^{Cre}\) lineage tracing and bone marrow transplantation showed that the precursors were derived from adult hematopoietic stem cells and were most likely continuously replaced via cell trafficking. Importantly, their occurrence was tied to the immunologic state of the central nervous system (CNS) and was diminished in the context of neuroinflammation and ischemic stroke. Our findings confirm the presence of myeloid progenitors at the meningeal border of the brain and lay the foundation to unravel their possible functions in CNS surveillance and local immune cell production.
KW  - hematopoietic
KW  - meninges
KW  - mouse
KW  - myeloid
KW  - progenitor
Y1  - 2021
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-224452
VL  - 39
IS  - 2
SP  - 227
EP  - 239
ER  - 
TY  - JOUR
A1  - Pozzi, Nicoló Gabriele
A1  - Bolzoni, Francesco
A1  - Biella, Gabriele Eliseo Mario
A1  - Pezzoli, Gianni
A1  - Ip, Chi Wang
A1  - Volkmann, Jens
A1  - Cavallari, Paolo
A1  - Asan, Esther
A1  - Isaias, Ioannis Ugo
T1  - Brain noradrenergic innervation supports the development of Parkinson’s tremor: a study in a reserpinized rat model
JF  - Cells
N2  - The pathophysiology of tremor in Parkinson’s disease (PD) is evolving towards a complex alteration to monoaminergic innervation, and increasing evidence suggests a key role of the locus coeruleus noradrenergic system (LC-NA). However, the difficulties in imaging LC-NA in patients challenge its direct investigation. To this end, we studied the development of tremor in a reserpinized rat model of PD, with or without a selective lesioning of LC-NA innervation with the neurotoxin DSP-4. Eight male rats (Sprague Dawley) received DSP-4 (50 mg/kg) two weeks prior to reserpine injection (10 mg/kg) (DR-group), while seven male animals received only reserpine treatment (R-group). Tremor, rigidity, hypokinesia, postural flexion and postural immobility were scored before and after 20, 40, 60, 80, 120 and 180 min of reserpine injection. Tremor was assessed visually and with accelerometers. The injection of DSP-4 induced a severe reduction in LC-NA terminal axons (DR-group: 0.024 ± 0.01 vs. R-group: 0.27 ± 0.04 axons/um\(^2\), p < 0.001) and was associated with significantly less tremor, as compared to the R-group (peak tremor score, DR-group: 0.5 ± 0.8 vs. R-group: 1.6 ± 0.5; p < 0.01). Kinematic measurement confirmed the clinical data (tremor consistency (% of tremor during 180 s recording), DR-group: 37.9 ± 35.8 vs. R-group: 69.3 ± 29.6; p < 0.05). Akinetic–rigid symptoms did not differ between the DR- and R-groups. Our results provide preliminary causal evidence for a critical role of LC-NA innervation in the development of PD tremor and foster the development of targeted therapies for PD patients.
KW  - Parkinson’s disease
KW  - tremor
KW  - locus coeruleus
KW  - noradrenaline
KW  - reserpinized rat model
Y1  - 2023
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-357721
SN  - 2073-4409
VL  - 12
IS  - 21
ER  - 
TY  - JOUR
A1  - Ferero, Andrea
A1  - Rivero, Olga
A1  - Wäldchen, Sina
A1  - Ku, Hsing-Ping
A1  - Kiser, Dominik P.
A1  - Gärtner, Yvonne
A1  - Pennington, Laura S.
A1  - Waider, Jonas
A1  - Gaspar, Patricia
A1  - Jansch, Charline
A1  - Edenhofer, Frank
A1  - Resink, Thérèse J.
A1  - Blum, Robert
A1  - Sauer, Markus
A1  - Lesch, Klaus-Peter
T1  - Cadherin-13 Deficiency Increases Dorsal Raphe 5-HT Neuron Density and Prefrontal Cortex Innervation in the Mouse Brain
JF  - Frontiers in Cellular Neuroscience
N2  - Background: During early prenatal stages of brain development, serotonin (5-HT)-specific neurons migrate through somal translocation to form the raphe nuclei and subsequently begin to project to their target regions. The rostral cluster of cells, comprising the median and dorsal raphe (DR), innervates anterior regions of the brain, including the prefrontal cortex. Differential analysis of the mouse 5-HT system transcriptome identified enrichment of cell adhesion molecules in 5-HT neurons of the DR. One of these molecules, cadherin-13 (Cdh13) has been shown to play a role in cell migration, axon pathfinding, and synaptogenesis. This study aimed to investigate the contribution of Cdh13 to the development of the murine brain 5-HT system.

Methods: For detection of Cdh13 and components of the 5-HT system at different embryonic developmental stages of the mouse brain, we employed immunofluorescence protocols and imaging techniques, including epifluorescence, confocal and structured illumination microscopy. The consequence of CDH13 loss-of-function mutations on brain 5-HT system development was explored in a mouse model of Cdh13 deficiency.

Results: Our data show that in murine embryonic brain Cdh13 is strongly expressed on 5-HT specific neurons of the DR and in radial glial cells (RGCs), which are critically involved in regulation of neuronal migration. We observed that 5-HT neurons are intertwined with these RGCs, suggesting that these neurons undergo RGC-guided migration. Cdh13 is present at points of intersection between these two cell types. Compared to wildtype controls, Cdh13-deficient mice display increased cell densities in the DR at embryonic stages E13.5, E17.5, and adulthood, and higher serotonergic innervation of the prefrontal cortex at E17.5.

Conclusion: Our findings provide evidence for a role of CDH13 in the development of the serotonergic system in early embryonic stages. Specifically, we indicate that Cdh13 deficiency affects the cell density of the developing DR and the posterior innervation of the prefrontal cortex (PFC), and therefore might be involved in the migration, axonal outgrowth and terminal target finding of DR 5-HT neurons. Dysregulation of CDH13 expression may thus contribute to alterations in this system of neurotransmission, impacting cognitive function, which is frequently impaired in neurodevelopmental disorders including attention-deficit/hyperactivity and autism spectrum disorders.
KW  - serotonin
KW  - cadherin-13 (CDH13)
KW  - T-cadherin
KW  - neurodevelopment
KW  - psychiatric disorders
KW  - radial glia
KW  - dorsal raphe
KW  - prefrontal cortex
Y1  - 2017
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-170313
VL  - 11
IS  - 307
ER  - 
TY  - JOUR
A1  - Hohnmann, Christopher
A1  - Milles, Bianca
A1  - Schinke, Michael
A1  - Schroeter, Michael
A1  - Ulzheimer, Jochen
A1  - Kraft, Peter
A1  - Kleinschnitz, Christoph
A1  - Lehmann, Paul V.
A1  - Kuerten, Stefanie
T1  - Categorization of multiple sclerosis relapse subtypes by B cell profiling in the blood
JF  - Acta Neuropathologica Communications
N2  - Introduction
B cells are attracting increasing attention in the pathogenesis of multiple sclerosis (MS). B cell-targeted therapies with monoclonal antibodies or plasmapheresis have been shown to be successful in a subset of patients. Here, patients with either relapsing-remitting (n = 24) or secondary progressive (n = 6) MS presenting with an acute clinical relapse were screened for their B cell reactivity to brain antigens and were re-tested three to nine months later. Enzyme-linked immunospot technique (ELISPOT) was used to identify brain-reactive B cells in peripheral blood mononuclear cells (PBMC) directly ex vivo and after 96 h of polyclonal stimulation. Clinical severity of symptoms was determined using the Expanded Disability Status Scale (EDSS).

Results
Nine patients displayed B cells in the blood producing brain-specific antibodies directly ex vivo. Six patients were classified as B cell positive donors only after polyclonal B cell stimulation. In 15 patients a B cell response to brain antigens was absent. Based on the autoreactive B cell response we categorized MS relapses into three different patterns. Patients who displayed brain-reactive B cell responses both directly ex vivo and after polyclonal stimulation (pattern I) were significantly younger than patients in whom only memory B cell responses were detectable or entirely absent (patterns II and III; p = 0.003). In one patient a conversion to a positive B cell response as measured directly ex vivo and subsequently also after polyclonal stimulation was associated with the development of a clinical relapse. The evaluation of the predictive value of a brain antigen-specific B cell response showed that seven of eight patients (87.5%) with a pattern I response encountered a clinical relapse during the observation period of 10 months, compared to two of five patients (40%) with a pattern II and three of 14 patients (21.4%) with a pattern III response (p = 0.0005; hazard ratio 6.08 (95% confidence interval 1.87-19.77).

Conclusions
Our data indicate actively ongoing B cell-mediated immunity against brain antigens in a subset of MS patients that may be causative of clinical relapses and provide new diagnostic and therapeutic options for a subset of patients.
KW  - predictive value
KW  - MS
KW  - ELISPOT
KW  - B cells
KW  - relapse
Y1  - 2014
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-126124
VL  - 2
IS  - 138
ER  - 
TY  - JOUR
A1  - Hohmann, Christopher
A1  - Milles, Bianca
A1  - Schinke, Michael
A1  - Schroeter, Michael
A1  - Ulzheimer, Jochen
A1  - Kraft, Peter
A1  - Kleinschnitz, Christoph
A1  - Lehmann, Paul V.
A1  - Kuerten, Stefanie
T1  - Categorization of multiple sclerosis relapse subtypes by B cell profiling in the blood
JF  - Acta Neuropathologica Communications
N2  - INTRODUCTION:
B cells are attracting increasing attention in the pathogenesis of multiple sclerosis (MS). B cell-targeted therapies with monoclonal antibodies or plasmapheresis have been shown to be successful in a subset of patients. Here, patients with either relapsing-remitting (n = 24) or secondary progressive (n = 6) MS presenting with an acute clinical relapse were screened for their B cell reactivity to brain antigens and were re-tested three to nine months later. Enzyme-linked immunospot technique (ELISPOT) was used to identify brain-reactive B cells in peripheral blood mononuclear cells (PBMC) directly ex vivo and after 96 h of polyclonal stimulation. Clinical severity of symptoms was determined using the Expanded Disability Status Scale (EDSS).

RESULTS:
Nine patients displayed B cells in the blood producing brain-specific antibodies directly ex vivo. Six patients were classified as B cell positive donors only after polyclonal B cell stimulation. In 15 patients a B cell response to brain antigens was absent. Based on the autoreactive B cell response we categorized MS relapses into three different patterns. Patients who displayed brain-reactive B cell responses both directly ex vivo and after polyclonal stimulation (pattern I) were significantly younger than patients in whom only memory B cell responses were detectable or entirely absent (patterns II and III; p = 0.003). In one patient a conversion to a positive B cell response as measured directly ex vivo and subsequently also after polyclonal stimulation was associated with the development of a clinical relapse. The evaluation of the predictive value of a brain antigen-specific B cell response showed that seven of eight patients (87.5%) with a pattern I response encountered a clinical relapse during the observation period of 10 months, compared to two of five patients (40%) with a pattern II and three of 14 patients (21.4%) with a pattern III response (p = 0.0005; hazard ratio 6.08 (95% confidence interval 1.87-19.77).

CONCLUSIONS:
Our data indicate actively ongoing B cell-mediated immunity against brain antigens in a subset of MS patients that may be causative of clinical relapses and provide new diagnostic and therapeutic options for a subset of patients.
KW  - ELISPOT
KW  - MS
KW  - predictive value
KW  - relapse
KW  - B cells
Y1  - 2014
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-120580
SN  - 2051-5960
VL  - 2
IS  - 138
ER  - 
TY  - JOUR
A1  - Rovituso, Damiano M.
A1  - Scheffler, Laura
A1  - Wunsch, Marie
A1  - Kleinschnitz, Christoph
A1  - Dörck, Sebastian
A1  - Ulzheimer, Jochen
A1  - Bayas, Antonios
A1  - Steinman, Lawrence
A1  - Ergün, Süleyman
A1  - Kuerten, Stefanie
T1  - CEACAM1 mediates B cell aggregation in central nervous system autoimmunity
JF  - Scientific Reports
N2  - B cell aggregates in the central nervous system (CNS) have been associated with rapid disease progression in patients with multiple sclerosis (MS). Here we demonstrate a key role of carcinoembryogenic antigen-related cell adhesion molecule1 (CEACAM1) in B cell aggregate formation in MS patients and a B cell-dependent mouse model of MS. CEACAM1 expression was increased on peripheral blood B cells and CEACAM1\(^+\) B cells were present in brain infiltrates of MS patients. Administration of the anti-CEACAM1 antibody T84.1 was efficient in blocking aggregation of B cells derived from MS patients. Along these lines, application of the monoclonal anti-CEACAM1 antibody mCC1 was able to inhibit CNS B cell aggregate formation and significantly attenuated established MS-like disease in mice in the absence of any adverse effects. CEACAM1 was co-expressed with the regulator molecule T cell immunoglobulin and mucin domain −3 (TIM-3) on B cells, a novel molecule that has recently been described to induce anergy in T cells. Interestingly, elevated coexpression on B cells coincided with an autoreactive T helper cell phenotype in MS patients. Overall, these data identify CEACAM1 as a clinically highly interesting target in MS pathogenesis and open new therapeutic avenues for the treatment of the disease.
KW  - autoimmunity
KW  - multiple sclerosis
KW  - neuroimmunology
Y1  - 2016
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-147690
VL  - 6
ER  - 
TY  - JOUR
A1  - Peitz, Michael
A1  - Münst, Bernhard
A1  - Thummer, Rajkumar P.
A1  - Helfen, Martina
A1  - Edenhofer, Frank
T1  - Cell-permeant recombinant Nanog protein promotes pluripotency by inhibiting endodermal specification
JF  - Stem Cell Research
N2  - A comprehensive understanding of the functional network of transcription factors establishing and maintaining pluripotency is key for the development of biomedical applications of stem cells. Nanog plays an important role in early development and is essential to induce natural pluripotency in embryonic stem cells (ESCs). Inducible gain-of-function systems allowing a precise control over time and dosage of Nanog activity would be highly desirable to study its vital role in the establishment and maintenance of pluripotency at molecular level. Here we engineered a recombinant cell permeable version of Nanog by fusing it with the cell penetrating peptide TAT. Nanog-TAT can be readily expressed in and purified from E. coli and binds to a consensus Nanog DNA sequence. At cellular level it enhances proliferation and self-renewal of ESCs in the absence of leukemia inhibitory factor (LIF). Nanog-TAT together with LIF acts synergistically as judged by enhanced clonogenicity and activation of an Oct4-promoter-driven GFP reporter gene. Furthermore Nanog-TAT, in the absence of LIF, promotes pluripotency by inhibiting endodermal specification in a Stat3-independent manner. Our results demonstrate that Nanog protein transduction is an attractive tool allowing control over dose and time of addition to the cells for studying the molecular control of pluripotency without genetic manipulation.
KW  - Nanog protein
Y1  - 2014
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-119740
SN  - 1876-7753
VL  - 12
IS  - 3
ER  - 
TY  - JOUR
A1  - Meierott, Lenz
T1  - Cerastium brachypetalum Desp. ex Pers. und Cerastium tenoreanum Ser. (Caryophyllaceae) in Franken
T1  - Cerastium brachypetalum Desp. ex Pers. and Cerastium tenoreanum Ser. (Caryophyllaceae) in Franconia, Southern Germany
N2  - Für Cerastium tenoreanum Ser. und die Varietäten von Cerastium brachypetalum Desp. ex Pers. werden ihre korrekte Nomenklatur, ihre Unterscheidungsmerkmale und ihre Verbreitung in Süddeutschland und Franken mitgeteilt. Die gegenwärtige Ausbreitungstendenz annueller Cerastien wird diskutiert.
N2  - The present communication on Cerastium tenoreanum Ser. and the varieties of Cerastium brachypetalum Desp. ex Pers. deals with nomenclature and diagnostic features of these taxa and their distribution pattern in Southern Germany. Factors influencing the recent distributional expansion of annual Cerastia are discussed.
KW  - Hornkraut
KW  - Nelkengewächse
KW  - Franken
KW  - Cerastium brachypetalum
KW  - Cerastium tenoreanum
KW  - Caryophyllaceae
KW  - Franconia
Y1  - 2008
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-35354
ER  - 
TY  - JOUR
A1  - Harreither, Eva
A1  - Rydberg, Hanna A.
A1  - Åmand, Helene L.
A1  - Jadhav, Vaibhav
A1  - Fliedl, Lukas
A1  - Benda, Christina
A1  - Esteban, Miguel A.
A1  - Pei, Duanqing
A1  - Borth, Nicole
A1  - Grillari-Voglauer, Regina
A1  - Hommerding, Oliver
A1  - Edenhofer, Frank
A1  - Nordén, Bengt
A1  - Grillari, Johanne
T1  - Characterization of a novel cell penetrating peptide derived from human Oct4
JF  - Cell Regeneration
N2  - BACKGROUND:
Oct4 is a transcription factor that plays a major role for the preservation of the pluripotent state in embryonic stem cells as well as for efficient reprogramming of somatic cells to induced pluripotent stem cells (iPSC) or other progenitors. Protein-based reprogramming methods mainly rely on the addition of a fused cell penetrating peptide. This study describes that Oct4 inherently carries a protein transduction domain, which can translocate into human and mouse cells.

RESULTS:
A 16 amino acid peptide representing the third helix of the human Oct4 homeodomain, referred to as Oct4 protein transduction domain (Oct4-PTD), can internalize in mammalian cells upon conjugation to a fluorescence moiety thereby acting as a cell penetrating peptide (CPP). The cellular distribution of Oct4-PTD shows diffuse cytosolic and nuclear staining, whereas penetratin is strictly localized to a punctuate pattern in the cytoplasm. By using a Cre/loxP-based reporter system, we show that this peptide also drives translocation of a functionally active Oct4-PTD-Cre-fusion protein. We further provide evidence for translocation of full length Oct4 into human and mouse cell lines without the addition of any kind of cationic fusion tag. Finally, physico-chemical properties of the novel CPP are characterized, showing that in contrast to penetratin a helical structure of Oct4-PTD is only observed if the FITC label is present on the N-terminus of the peptide.

CONCLUSIONS:
Oct4 is a key transcription factor in stem cell research and cellular reprogramming. Since it has been shown that recombinant Oct4 fused to a cationic fusion tag can drive generation of iPSCs, our finding might contribute to further development of protein-based methods to generate iPSCs. Moreover, our data support the idea that transcription factors might be part of an alternative paracrine signalling pathway, where the proteins are transferred to neighbouring cells thereby actively changing the behaviour of the recipient cell.
KW  - penetratin
KW  - reprogramming
KW  - cell penetrating peptides
KW  - cellular internalization
KW  - homeodomain transcription factors
KW  - Oct4
Y1  - 2014
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-120999
SN  - 2045-9769
VL  - 3
IS  - 2
ER  - 
TY  - JOUR
A1  - Wunsch, Marie
A1  - Zhang, Wenji
A1  - Hanson, Jodi
A1  - Caspell, Richard
A1  - Karulin, Alexey Y.
A1  - Recks, Mascha S.
A1  - Kuerten, Stefanie
A1  - Sundararaman, Srividya
A1  - Lehmann, Paul V.
T1  - Characterization of the HCMV-Specific CD4 T Cell Responses that Are Associated with Protective Immunity
JF  - Viruses
N2  - Most humans become infected with human cytomegalovirus (HCMV). Typically, the immune system controls the infection, but the virus persists and can reactivate in states of immunodeficiency. While substantial information is available on the contribution of CD8 T cells and antibodies to anti-HCMV immunity, studies of the T\(_{H}\)1, T\(_{H}\)2, and T\(_{H}\)17 subsets have been limited by the low frequency of HCMV-specific CD4 T cells in peripheral blood mononuclear cell (PBMC). Using the enzyme-linked Immunospot\(^{®}\) assay (ELISPOT) that excels in low frequency measurements, we have established these in a sizable cohort of healthy HCMV controllers. Cytokine recall responses were seen in all seropositive donors. Specifically, interferon (IFN)-\({\gamma}\) and/or interleukin (IL)-17 were seen in isolation or with IL-4 in all test subjects. IL-4 recall did not occur in isolation. While the ratios of T\(_{H}\)1, T\(_{H}\)2, and T\(_{H}\)17 cells exhibited substantial variations between different individuals these ratios and the frequencies were relatively stable when tested in samples drawn up to five years apart. IFN-\({\gamma}\) and IL-2 co-expressing polyfunctional cells were seen in most subjects. Around half of the HCMV-specific CD4 cells were in a reversible state of exhaustion. The data provided here established the T\(_{H}\)1, T\(_{H}\)2, and T\(_{H}\)17 characteristic of the CD4 cells that convey immune protection for successful immune surveillance against which reactivity can be compared when the immune surveillance of HCMV fails.
KW  - memory cells
KW  - hcv infection
KW  - signature
KW  - Enzyme-Linked Immunospot assay (ELISPOT)
KW  - cytokine secretion kinetics
KW  - chronic viral infection
KW  - HCMV infection
KW  - CD4 T cells
KW  - exhaustion
KW  - activation
KW  - human cytomegalovirus (HCMV)
KW  - B cells
KW  - cytomegalovirus
KW  - elispot
Y1  - 2015
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-151462
VL  - 7
SP  - 4414
EP  - 4437
ER  - 
TY  - THES
A1  - Arbeiter, Anja Katrin
T1  - Charakterisierung der Bindung des Stressproteins Alpha-B-Crystallin an kardiale Myofibrillen unter Ischämie
T1  - Characterization of the binding of the stress protein Alpha-B-crystallin to cardiac myofibrils under ischemia
N2  - Prolongierte Isch&auml;mieperioden des Herzens f&uuml;hren zu struktureller Sch&auml;digung der Kardiomyozyten, d.h. einer Desorganisation und Zerst&ouml;rung des kontraktilen und plasmalemmalen Zytoskeletts, welche sich final durch Verlust an Kontraktilit&auml;t und Ruptur der Plasmamembran manifestieren. Stressproteine k&ouml;nnen an die Komponenten des Zytoskelettes binden und durch Konformationsschutz der isch&auml;mischen Sch&auml;digung entgegenwirken. In vorangegangenen Untersuchungen wurde gezeigt, dass es unter Isch&auml;mie zu einer Translokation des konstitutiv in hoher Konzentration vorkommenden kardialen Stressproteins aB-Crystallin vom Zytosol an die Myofibrillen kommt. Dabei f&uuml;hren bereits kurzdauernde Isch&auml;mieperioden zu einer kompletten Umverteilung von aB-Crystallin in die Z/I-Region des Sarkomers. Es war das Ziel dieser Arbeit, diese Bindung von aB-Crystallin an Strukturproteine im Z/I-Banden Bereich n&auml;her zu charakterisieren und aB-Crystallin ultrastrukturell zu lokalisieren. Durch Immunogoldmarkierung konnte aB-Crystallin ultrastrukturell im Herzen unter globaler Isch&auml;mie in einer Linie parallel zur Z-Scheibe etwa in der Mitte der halben I-Bande lokalisiert werden. Diese Zone entspricht dem Bereich, der als N-Linie bezeichnet wird. In der Frage der in vivo-Bindungspartner von aB-Crystallin waren daher in erster Linie Komponenten der I-Bande, d.h. Aktin und Titin in Betracht zu ziehen. Z-Scheiben Proteine wie a-Actinin treten dagegen in den Hintergrund. Um Anhaltspunkte &uuml;ber die Bindungsst&auml;rke des Stressproteins aB-Crystallin an kardiale Myofibrillen unter Isch&auml;mie zu erhalten, wurden isch&auml;mische Myofibrillen aus dem Rattenherz mit hochmolaren Salzl&ouml;sungen und chaotropen Substanzen behandelt. Dabei konnte eine sehr hohe Bindungsaffinit&auml;t von aB-Crystallin an die Myofibrillen festgestellt werden. Die myofibrill&auml;re Bindung zeigte sich resistent gegen&uuml;ber 1M KCl, 1M NaSCN und 2M Harnstoff, erst 2M NaSCN und 4M Harnstoff, die eine Zerst&ouml;rung der myofibrill&auml;ren Integrit&auml;t bewirken, verm&ouml;gen die aB-Crystallin-Bindung zu l&ouml;sen. Aktin dagegen lie&szlig; sich bereits durch 0,5M NaSCN-L&ouml;sung von den Myofibrillen extrahieren, Bedingungen, unter denen aB-Crystallin noch fest an die Myofibrillen gebunden blieb. Aktin scheidet somit als in vivo-Bindungspartner von aB-Crystallin aus. Dieses Ergebnis immunhistochemischer Untersuchungen konnte auch mit biochemischer Methodik (Immunreplikanalyse) verifiziert werden. Titin zeigte sich wie aB-Crystallin resistent gegen&uuml;ber den meisten der oben aufgef&uuml;hrten Salzl&ouml;sungen. Eine deutliche Extraktion von Titin aus den Myofibrillen konnte erst durch Behandlung mit 2M NaSCN sowie 4M Harnstoffl&ouml;sung beobachtet werden, das Extraktionsverhalten entsprach somit dem von aB-Crystallin. Einen Hinweis auf eine Assoziation von aB-Crystallin mit Titin lieferte der Nachweis von aB-Crystallin in isolierten Titinfraktionen aus isch&auml;mischen Herzen. Der direkte Beweis f&uuml;r eine aB-Crystallin-Titin-Interaktion konnte im Rahmen dieser Arbeit jedoch nicht erbracht werden. Bindungsstudien, die zwischen ausgew&auml;hlten nativen, in vitro translatierten Titindom&auml;nen und aus der Linse isoliertem aB-Crystallin durchgef&uuml;hrt wurden, waren negativ. Dies ist m&ouml;glicherweise dadurch bedingt, dass aB-Crystallin erst unter Isch&auml;mie mit Titin interagiert und in vitro Kofaktoren ben&ouml;tigt werden. Durch eine Bindung an I-Banden Abschnitte des Titinmolek&uuml;ls k&ouml;nnte aB-Crystallin eine kardioprotektive Funktion erf&uuml;llen, indem es unter Isch&auml;mie stabilisierend auf das Filamentsystem einwirkt.
N2  - Prolonged ischemic periods of the heart lead to structural damage of the cardiomyocytes, i.e. disorganization and destruction of the cellular cytoskeleton with final loss of contractility and rupture of the plasma membrane. Stress proteins can bind to components of the cellular cytoskeleton and play a protective role during various kinds of stresses. Previous studies showed a translocation of the cardiac stress protein áB crystallin from the cytosol, there occurring in constitutive high concentrations, to the myofibrils under ischemia. Already short ischemic periods lead to a complete translocation of áB crystallin into the Z/I region of the myofibrils. The purpose of the present study was to identify the localization of áB crystallin during ischemia at the ultrastructural level and to obtain further information about myofibrillar components that may serve as binding sites for áB crystallin during ischemia. Under global ischemia áB crystallin could be located by immunogold-labelling in the heart in a narrow zone of the I-band parallel to the Z-disk (area of the N2-line).The restriction of áB crystallin to this N2-line indicates binding of áB crystallin to either titin or components of actin filaments. Actin filaments and actin associated proteins such as tropomyosin or troponin complex are not likely candidates for áB crystallin binding because actin became completely extracted of the myofibrils after treatment of cryostat sections of ischemic rat myocardium with 0,5M NaSCN, conditions where áB crystallin and titin remained unchanged.The myofibrillaric binding of áB crystallin and titin resisted extraction with 1M KCl, 1M NaSCN and 2M urea, only 2M NaSCN and 4M urea, which cause a destruction of the myofibrillaric integrity, were able to disrupt the áB crystallin binding. These results of immunocytochemistry could be verified biochemically (immunoblotting). They indicate association of áB crystallin with titin the only remaining non-actin or actin-binding cytoskeletal component of I-bands outside Z-disks. Further evidence for binding of áB crystallin to titin was obtained by dot-blot assays in which biotinylated áB crystallin was demonstrated to bind to a titin-enriched fraction of pig myocardium immobilized on nitrocellulose. Furthermore this titin-enriched fraction was shown to copurify with áB crystallin. However dot-blot binding studies between several in-vitro translated titin domains and purified áB crystallin did not show any detectable binding. These negative results obtained by in vitro binding studies do not exclude interaction between titin fragments and áB crystallin in vivo. The absence of in vitro interaction is possibly due to a different three dimensional structure of the in vitro expressed titin fragments or to the absence of specific ischemia-induced cofactors. Binding of áB crystallin to titin during cardiac ischemia could serve to stabilize titin against denaturation and might provide an endogenous mechanism to delay ischemic damage by stabilizing this critical I-band region of titin with its elastic properties.
KW  - aB-Crystallin
KW  - Titin
KW  - Stressprotein
KW  - Ischämie
KW  - Myokard
KW  - aB-crystallin
KW  - titin
KW  - stress protein
KW  - ischemia
KW  - myocardium
Y1  - 2001
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-4337
ER  - 
TY  - THES
A1  - Redel, Andreas
T1  - Charakterisierung der kardialen Funktion des Stressproteins alpha-B-Crystallin am isolierten Papillarmuskel der Maus
T1  - Characterisation of the cardiac function of the stress protein alpha-B-Crystallin in isolated murine papillary muscles
N2  - Eine familiäre Myopathie und Kardiomyopathie, der eine Missense-Mutation des alpha-B-Crystallin-Gens zugrunde liegt, weist auf eine wichtige Bedeutung des Stressproteins alpha-B-Crystallin im Herzen hin. Die chaperone-ähnlichen Eigenschaften von alpha-B-Crystallin und die unter kardialer Ischämie zu beobachtende schnelle Translokation vom Zytosol an das elastische Titin-Filamentsystem lassen eine protektive Rolle von alpha-B-Crystallin unter Stressbedingungen vermuten. Ziel der vorliegenden Arbeit war es, eine eventuelle kardioprotektive Funktion von alphaB-Crystallin durch die Charakterisierung alpha-B-Crystallin gendeletierter Mäuse nachzuweisen. Wir etablierten hierfür ein Versuchssystem zur Untersuchung der Kontraktilität isolierter Papillarmuskeln im Organbad. Im Rahmen des Aufbaus unseres Versuchssystems untersuchten wir zunächst den Einfluss der Ca2+-Konzentration, der Temperatur und der Kontraktionsbedingungen (Auxotonie vs. Isometrie) auf die Kraft-Frequenz-Beziehung von murinem Myokard. Wir konnten zeigen, dass die Kraft-Frequenz-Beziehung von Myokardpräparaten der Maus von den genannten Versuchsbedingungen abhängig ist. Bei niedrigen Ca2+-Konzentrationen und Temperaturen ([Ca2+] = 1,0 mM, Temp. = 27 °C) ist sie positiv, flacht bei zunehmender Ca2+-Konzentration und Temperatur ab und ist für [Ca2+] = 5,0 mM, Temp. = 37 °C negativ. Auxotone Kontraktionsbedingungen führen im Vergleich zu isometrischen bei gleichen Ca2+-Konzentrationen und Temperaturen zu einem flacheren Verlauf der Kraft-Frequenz-Beziehung. Unter annähernd physiologischen Bedingungen verläuft die Kraft-Frequenz-Beziehung des Mäuse-Myokards flach bis leicht positiv. Im Gegensatz zum Menschen scheinen somit bei der Maus für eine Steigerung des Herz-Zeit-Volumens andere Mechanismen als eine positive Kraft-Frequenz-Beziehung von Bedeutung zu sein. Hierbei ist insbesondere der Frank-Starling-Mechanismus und die sympathoadrenerge Innervation des Herzens zu erwähnen. Zur Charakterisierung der kardialen Funktion von alphaB-Crystallin untersuchten wir die Kontraktilität isolierter Papillarmuskeln von Wildtyp- und alpha-B-Crystallin gendeletierten Mäusen unter simulierter Ischämie (Glucose- und Sauerstoffentzug) und Reperfusion im Organbad. Unter Kontrollbedingungen zeigten sich zwischen wt- und alpha-B-/- Muskeln keine Unterschiede in der Zuckungskraft, der Geschwindigkeit der Kraftentwicklung und der Relaxationszeit. Die während der 20-minütigen simulierten Ischämie entwickelte Kontraktur setzte jedoch bei den alpha-B-/- Muskeln signifikant früher ein und verlief signifikant stärker als bei wt-Muskeln. Nach einer 60-minütigen Reperfusionsphase blieb die Kontraktur der alpha-B-/- Muskeln im Vergleich zu wt-Muskeln signifikant erhöht. Bezüglich Zuckungskraft, Geschwindigkeit der Kraftentwicklung und Relaxationszeit zeigten sich weder während noch nach simulierter Ischämie deutliche Unterschiede zwischen den Muskeln beider Mäusestämme. Diese Ergebnisse lassen darauf schließen, dass das Fehlen von alpha-B-Crystallin am Gesamtherz nicht zu einer Störung der systolischen Herzfunktion, sondern zu einer eingeschränkten myokardialen Relaxationsfähigkeit unter Ischämie und Reperfusion führen würde. Da alpha-B-Crystallin unter kardialer Ischämie an das elastische Titin-Filamentsystem bindet, könnten die elastischen Eigenschaften des Myokards unter Ischämie durch einen Mangel an alpha-B-Crystallin derart beeinträchtigt werden, dass es zu einer höheren Rigidität der Muskulatur kommt. Eine Funktion von alpha-B-Crystallin im Herzen ist somit möglicherweise die Aufrechterhaltung der elastischen Eigenschaften des Myokards unter kardialer Ischämie und Reperfusion.
N2  - Missense mutations of the alpha-B-Crystallin gene have been shown to cause familial myopathy and cardiomyopathy suggesting an important role of the stress protein alpha-B-Crystallin in cardiac function. The aim of this study was to investigate if alpha-B-Crystallin may play a cardioprotective role during cardiac ischemia/reperfusion using alpha-B-Crystallin-deficient (alpha-B-/-) mice. For this purpose we established an ischemia/reperfusion model of isolated perfused murine papillary muscles and first investigated the influence of Ca2+, temperature and contraction type (auxotonic vs. isometric) on the force-frequency-relation (FFR) of murine myocardium defining optimal experimental conditions for isolated murine papillary muscle preparations. Under isometric conditions low Ca2+ (1.0 mM) and low temperature (27°C) lead to a positive FFR, while at high Ca2+ and temperature (5,0 mM, 37°C) the FFR turned negative. Auxotonic contractions resulted in flattening of the FFR compared to isometric concentrations. Thus, under conditions mimicking the physiological situation best ([Ca2+] = 1,5 mM, 32°C, auxotony) the FFR of murine heart is flat indicating that in contrast to the human heart in the mouse heart in vivo a positive inotropic effect by increasing heart frequency does not contribute significantly to increase cardiac output. To characterise cardiac function of alpha-B-Crystallin papillary muscles from alpha-B-/- and wildtype mice were exposed to 20 min of simulated ischemia (withdrawal of glucose and oxygen) and 60 min of reperfusion. Under physiological conditions no differences in contractility of alpha-B-/- and wildtype mice were observed. However, during simulated ischemia the development of ischemic contracture started earlier and reached a significant higher value in alpha-B-/- than in wildtype muscles. The recovery of the contracture during simulated reperfusion was also significantly attenuated. Interestingly, twitch force was neither during ischemia nor during the reperfusion period significantly altered. This suggests that during ischemia alpha-B-Crystallin may rather serve to protect cardiac relaxation (diastolic function) than contraction itself. The molecular mechanisms underlying this pronounced pathological behaviour remain to be determined. Since alpha-B-Crystallin is known to bind to the elastic titin filament system during ischemia we propose that increased ischemia-induced cardiac muscle stiffness in alpha-B-/- mice result from reduced elastic properties of titin in the absence of alpha-B-Crystallin. Thus, one possible function of alpha-B-Crystallin in the heart might be to preserve myofibrillar elastic properties during ischemia/reperfusion.
KW  - alpha-B-Crystallin
KW  - Hitzeschockprotein
KW  - Ischämie-Reperfusions-Schaden
KW  - Kraft-Frequenz-Beziehung
KW  - Präkonditionierung
KW  - alpha-B-Crystallin
KW  - heat shock protein
KW  - ischemia reperfusion injury
KW  - force frequency relationship
KW  - preconditioning
Y1  - 2004
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-11984
ER  - 
TY  - THES
A1  - Silwedel, Christine
T1  - Charakterisierung immortalisierter Maus-Hirnendothelzelllinien als in vitro-Modelle der Blut-Hirn-Schranke
T1  - Characterization of immortalized murine brain capillary endothelial cells as an in vitro model of the blood brain barrier
N2  - Die Blut-Hirn-Schranke reguliert den Transport von Molekülen aus dem Blut in das Gehirn und aus dem Hirngewebe in das Blut. Die Grundlage dieser für den Erhalt der Homöostase im Gehirn wichtigen Schranke bilden zwischen Endothelzellen der Gehirnkapillaren (BCECs) entwickelte, besonders dichte Zonulae Occludentes (Tight Junctions). Viele Krankheiten, zum Beispiel die Multiple Sklerose, gehen mit einer Dysfunktion der BBB einher, die molekularen Grundlagen verschiedener Störungen und damit die Therapiemöglichkeiten sind bisher jedoch oftmals noch unbekannt. Ein grundlegendes Problem der Forschung an der BBB war bislang das Fehlen eines geeigneten immortalisierten in vitro-Modelles zum Verständnis der Differenzierung und Regulierung der Schrankenfunktion. Es gelang nun erstmals, aus murinen BCECs ein solches in vitro-Modell der BBB zu entwickeln, welches wichtige Charakteristika der BBB in vivo aufweist. Zu den Eigenschaften der BBB in vivo zählen allgemein ein hoher transendothelialer elektrischer Widerstand (TER) von bis zu 2000 &#61527; x cm², die Expression der TJ-Proteine Occludin, Claudin-1, Claudin-3 und Claudin-5 sowie eine geringe Rate transzellulärer Transportvorgänge. Die Entwicklung einer immortalisierten Zelllinie als in vitro-Modell der BBB beinhaltete das Bereitstellen einer möglichst natürlichen Umgebung für die Endothelzellen. Durch Zugabe von Wachstums- und Differenzierungsfaktoren sowie Serumreduktion im Differenzierungsmedium konnte eine dichte Schrankenfunktion induziert werden, welche sich anhand von TER-Messungen nachweisen ließ. Mittels immuncytochemischen und molekularbiologischen Methoden wurde außerdem die Expression verschiedener TJ-Proteine in den immortalisierten BCECs gezeigt. Die Permeabilität der BBB wird durch eine Reihe von Faktoren beeinflusst. So war zu erkennen, dass Glucocorticoide und Insulin die Barrierenfunktion der BBB induzieren und die Zugabe dieser Faktoren die in vitro-Kultivierung von BCECs ermöglicht, ohne dass diese dabei für die BBB in vivo wesentliche Charakteristika verlieren. Diese Ergebnisse stimmen überein mit anderen Studien, denenzufolge für die Induktion und Aufrechterhaltung komplexer Tight Junctions bei kultivierten Endothelzellen Glucocorticoide förderlich sind. Auch klinisch wird dieser Einfluss von Glucocorticoiden bereits genutzt: so konnten im Falle der Multiplen Sklerose Therapieerfolge durch die Gabe von Corticosteroiden erzielt werden.
N2  - The blood brain barrier is responsible for regulation of transport between blood and brain, thus keeping up the brain's homeostasis. Tight Junctions in between brain capillary endothelial cells are the basis for barrier properties. Many diseases are going hand in hand with or are caused by a leakage within the blood brain barrier. Research was often limited by the lack of a proper in vitro model of the blood brain barrier. Aim of this study was to establish an in vitro model of the blood brain barrier and investigate regulation mechanisms. After cell isolation from murine brains certain growth- and differentiation supplements were added, cells were afterwards investigated regarding typical blood brain barrier properties. These are certain tight junction proteins (e.g. occludine, claudins), a high transendothelial electrical resistance as well as a low rate of transcellular transport. Our results showed the isolated brain capillary endothelial cells to be displaying those properties, thus building a valid in vitro model of the blood brain barrier.
KW  - Blut-Hirn-Schranke
KW  - Occludin
KW  - Hirnendothelzellen
KW  - zerebrale Mikrovaskulatur
KW  - blood brain barrier
KW  - cerebral microvasculature
KW  - brain capillary endothelial cells
Y1  - 2008
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-34946
ER  - 
TY  - THES
A1  - Müller, Jonathan
T1  - Charakterisierung von CEACAM1 in der Retina und Choroidea am Mausmodell
T1  - Characterization of CEACAM1 in retina and choroid in mouse model
N2  - Carcinoembryonic antigen-related cell adhesion molecule 1 (CEACAM1) ist ein multifunktionales Zell-Zell Adhäsionsprotein, das in eine Vielzahl an zellulären Prozessen involviert ist, wie zum Beispiel der Differenzierung von Geweben, der Tumorsuppression, Metastasierung, Angiogenese und Apoptose. Außerdem hat es modulierende Eigenschaften auf die angeborene und erworbene Immunantwort. In der vorliegenden Arbeit charakterisierte ich initial die Lokalisation und die CEACAM1-exprimierenden Zelltypen im Auge und bestimmte quantitativ die Expression von Ceacam1 in der Retina und Choroidea zu unterschiedlichen Zeitpunkten. 
Es zeigte sich hierbei, dass Ceacam1 zu allen untersuchten Zeitpunkten, sowohl während der Entwicklung als auch im adulten retinalen und choroidalen Gewebe nachweisbar war. Mittels Immunhistochemie konnte die Expression von CEACAM1 im Corneaepithel, den Gefäßen der Iris und des Ziliarkörpers, im nicht-pigmentierten Epithel des Ziliarkörpers, sowie in den retinalen und choroidalen Gefäßen nachgewiesen werden. Durch Doppelfärbung mit Kollagen IV konnte die endotheliale Expression von CEACAM1 in den Endothelzellen der Gefäße bestätigt werden. 
Im zweiten Teil meiner Arbeit untersuchte ich die Funktion von CEACAM1 im Auge und verglich dazu wildtypische Retinae mit Cc1-/--Retinae. Es zeigten sich keine offensichtlichen morphologischen Veränderungen der retinalen Schichten und die anschließend durchgeführten morphometrischen Analysen der Schichtdicken der retinalen Neurone zeigte keine Anzeichen einer Neurodegeneration. Allerdings waren in Cc1-/--Retinae kleine Zysten und IBA1 positive, phagozytisch aktive Zellen im subneuroretinalen Raum, also dem Bereich zwischen RPE und den Außensegmenten der Photorezeptoren zu erkennen. Die anschließend durchgeführten Expressionsanalysen immunmodulierender Faktoren und von Mitgliedern des TGF-β-Signalwegs in retinalen und choroidealen Proben wildtypischer und Cc1-/--Mäusen zeigten keine veränderte Expression für Iba1, Ccl2 sowie Tnf-α. Jedoch konnten signifikant erhöhte Werte für TGF-β1 in der Gruppe der 2-4 als auch der Gruppe der 9 Monate alten Cc1-/--Retinae im Vergleich zu wildtypischen Retinae nachgewiesen werden. Basierend auf den Daten der vorliegenden Arbeit kann geschlussfolgert werden, dass die Deletion von CEACAM1 unter physiologischen Bedingungen die Struktur der Retina und Choroidea nicht offensichtlich beeinflusst. Allerdings führt die Deletion zu erhöhten Tgfβ1 Spiegeln in der Retina und zur Aktivierung und Akkumulation von IBA1 positiven Zellen im subneuroretinalen Raum.
N2  - Carcinoembryonic antigen-related cell adhesion molecule 1 (Ceacam1, Cc1) is a multi-functional cell–
cell adhesion protein, involved in the differentiation and arrangement of tissue three-dimensional
structure, tumor suppression, metastasis, angiogenesis and apoptosis. Moreover, it has been shown
to modulate innate and adaptive immune responses. Amongst others, it is expressed in vascular
endothelial cells during vascular development and in adult blood vessels that are activated by
angiogenic processes. In this study, we aimed to learn about the function of Ceacam1 in the eye.
We therefore characterized the cell type specific expression of Ceacam1 in the ocular tissues, analyzed
its retinal and choroidal expression at different developmental time points and studied the ocular
morphology of Ceacam1- knockout (Cc1-/-) mice. Finally, we analyzed the molecular expression levels
of immune modulating factors and members of the TGF-β signaling family in retinal and choroidal
tissues of Cc1-/- mice.
Our data show that Ceacam1 is expressed in developing and mature retinal and choroidal endothelial
cells. Furthermore, its deletion promotes the accumulation of phagocytic active and Iba1-positive cells
in the subretinal space and significant upregulated TGF-β1 expression levels in the retina.
KW  - Angiogenese
KW  - Vaskularisation
KW  - Netzhaut
KW  - Aderhaut
KW  - CEACAM1
KW  - Retina
KW  - Choroidea
Y1  - 2023
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-305546
ER  - 
TY  - JOUR
A1  - Schütz, Burkhard
A1  - Jurastow, Innokentij
A1  - Bader, Sandra
A1  - Ringer, Cornelia
A1  - Engelhardt, Jakob von
A1  - Chubanov, Vladimir
A1  - Gudermann, Thomas
A1  - Diener, Martin
A1  - Kummer, Wolfgang
A1  - Krasteva-Christ, Gabriela
A1  - Weihe, Eberhard
T1  - Chemical coding and chemosensory properties of cholinergic brush cells in the mouse gastrointestinal and biliary tract
JF  - Frontiers in Physiology
N2  - The mouse gastro-intestinal and biliary tract mucosal epithelia harbor choline acetyltransferase (ChAT)-positive brush cells with taste cell-like traits. With the aid of two transgenic mouse lines that express green fluorescent protein (EGFP) under the control of the ChAT promoter (EGFP\(^{ChAT}\)) and by using in situ hybridization and immunohistochemistry we found that EGFP\(^{ChAT}\) cells were clustered in the epithelium lining the gastric groove. EGFP\(^{ChAT}\) cells were numerous in the gall bladder and bile duct, and found scattered as solitary cells along the small and large intestine. While all EGFP\(^{ChAT}\) cells were also ChAT-positive, expression of the high-affinity choline transporter (ChT1) was never detected. Except for the proximal colon, EGFP\(^{ChAT}\) cells also lacked detectable expression of the vesicular acetylcholine transporter (VAChT). EGFP\(^{ChAT}\) cells were found to be separate from enteroendocrine cells, however they were all immunoreactive for cytokeratin 18 (CK18), transient receptor potential melastatin-like subtype 5 channel (TRPM5), and for cyclooxygenases 1 (COX1) and 2 (COX2). The ex vivo stimulation of colonic EGFP\(^{ChAT}\) cells with the bitter substance denatonium resulted in a strong increase in intracellular calcium, while in other epithelial cells such an increase was significantly weaker and also timely delayed. Subsequent stimulation with cycloheximide was ineffective in both cell populations. Given their chemical coding and chemosensory properties, EGFP\(^{ChAT}\) brush cells thus may have integrative functions and participate in induction of protective reflexes and inflammatory events by utilizing ACh and prostaglandins for paracrine signaling.
KW  - vesicular acetylcholine transporter
KW  - nonneuronal acetylcholine
KW  - nervous system
KW  - functional characterization
KW  - cholinergic
KW  - taste receptor cells
KW  - enteroendocrine cells
KW  - gene locus
KW  - tuft cells
KW  - transgenic mice
KW  - expression
KW  - brush cell
KW  - ChAT
KW  - VAChT
KW  - ChT1
KW  - intestine
KW  - gall bladder
KW  - bile duct
Y1  - 2015
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-143550
VL  - 6
IS  - 87
ER  - 
TY  - JOUR
A1  - Karnati, Srikanth
A1  - Seimetz, Michael
A1  - Kleefeldt, Florian
A1  - Sonawane, Avinash
A1  - Madhusudhan, Thati
A1  - Bachhuka, Akash
A1  - Kosanovic, Djuro
A1  - Weissmann, Norbert
A1  - Krüger, Karsten
A1  - Ergün, Süleyman
T1  - Chronic Obstructive Pulmonary Disease and the Cardiovascular System: Vascular Repair and Regeneration as a Therapeutic Target
JF  - Frontiers in Cardiovascular Medicine
N2  - Chronic obstructive pulmonary disease (COPD) is a major cause of morbidity and mortality worldwide and encompasses chronic bronchitis and emphysema. It has been shown that vascular wall remodeling and pulmonary hypertension (PH) can occur not only in patients with COPD but also in smokers with normal lung function, suggesting a causal role for vascular alterations in the development of emphysema. Mechanistically, abnormalities in the vasculature, such as inflammation, endothelial dysfunction, imbalances in cellular apoptosis/proliferation, and increased oxidative/nitrosative stress promote development of PH, cor pulmonale, and most probably pulmonary emphysema. Hypoxemia in the pulmonary chamber modulates the activation of key transcription factors and signaling cascades, which propagates inflammation and infiltration of neutrophils, resulting in vascular remodeling. Endothelial progenitor cells have angiogenesis capabilities, resulting in transdifferentiation of the smooth muscle cells via aberrant activation of several cytokines, growth factors, and chemokines. The vascular endothelium influences the balance between vaso-constriction and -dilation in the heart. Targeting key players affecting the vasculature might help in the development of new treatment strategies for both PH and COPD. The present review aims to summarize current knowledge about vascular alterations and production of reactive oxygen species in COPD. The present review emphasizes on the importance of the vasculature for the usually parenchyma-focused view of the pathobiology of COPD.
KW  - COPD
KW  - emphysema
KW  - pulmonary hypertension
KW  - hypoxia
KW  - oxidative stress
Y1  - 2021
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-235631
SN  - 2297-055X
VL  - 8
ER  - 
TY  - THES
A1  - Langenhan, Tobias
T1  - Ciliary neurotrophic factor (CNTF) im olfaktorischen System von Ratten und Mäusen
T1  - Ciliary neurotrophic factor (CNTF) in the olfactory system of rats and mice
N2  - Das olfaktorische System ist aufgrund seiner lebenslangen regenerativen Kapazität, seines Reichtums an neurotrophen Faktoren und der relativ guten Zugänglichkeit für Manipulationen ein attraktiver Gegenstand neurobiologischer Forschung. In der vorliegenden Arbeit wurde die Lokalisation und mögliche Funktion des ziliären neurotrophen Faktors (CNTF) in der primären Geruchsbahn mit Hilfe immunhistochemischer Methoden untersucht. Es konnte gezeigt werden, dass die CNTF-Ir bei Ratten und Mäusen in den olfaktorischen Gliazellen (Ensheathingzellen) lokalisiert ist. Elektronenmikroskopische Aufnahmen belegten ein zytoplasmatisches und nukleäres Vorkommen der CNTF-Ir innerhalb der EC. Ein neues und überraschendes Ergebnis der Arbeit ist, dass CNTF in individuellen olfaktorischen Neuronen vorkommt. Bislang wurde CNTF lediglich in Gliazellen des zentralen und peripheren Nervensystems nachgewiesen. Die weitere Charakterisierung der epithelialen CNTF-ir Neurone kennzeichnete diese als reife olfaktorische Nervenzellen. Die CNTF-Ir war mit dem olfaktorischen Markerprotein (OMP) kolokalisiert, einem Marker ausschließlich reifer ON und wies keine Kolokalisation mit dem Growth associated protein 43 (GAP-43) auf, dessen Expression unreife Riechsinneszellen kennzeichnet. CNTF könnte einerseits an lebenslang fortwährenden De- und/oder Regenerationsvorgängen des olfaktorischen Epithels beteiligt sein. Die Exposition der Riechschleimhaut gegenüber infektiösen, physikalischen und chemischen Noxen bedingt den ständigen Verlust olfaktorischer Neurone und deren lebenslange Regeneration aus neuronalen Vorläuferzellen im olfaktorischen Epithel. Die Zellkerne CNTF-ir ON wiesen in der Mehrzahl keine degenerativen Veränderungen wie Kondensierung und Fragmentierung auf, wie es bei geschädigten und untergehenden Zellen beobachtet wird. Im olfaktorischen Epithel zeigte sich des weiteren keine neuronale Kolokalisation von CNTF mit der aktivierten Caspase-3, einem Exekutorenzym der Apoptose, wie man es bei apoptotisch degenerierenden Neuronen findet. Nach Läsionen des olfaktorischen Epithels von Mäusen, die nekrotische Zelluntergänge auslösen, konnte kein gesteigertes Vorkommen von CNTF-ir ON gezeigt werden. Eine Einbindung von CNTF in die Mechanismen neuronaler Degeneration erscheint nach den Ergebnissen verschiedener Experimente wenig wahrscheinlich. Eine zweite Erklärung für das individuelle neuronale Auftreten der CNTF-Ir bot die Annahme, dass CNTF mit der Expression olfaktorischer Rezeptorproteine vergesellschaftet sein könnte. Dreidimensionale Rekonstruktionen von Paaren von BO bei Ratten und Mäusen zeigte, dass die Axone CNTF-ir ON in Glomeruli olfactorii projizierten, die bilateralsymmetrisch in beiden BO eines Tieres lokalisiert waren. Diese Symmetrie findet man ebenfalls bei den Projektionen der ON, die das gleiche olfaktorische Rezeptorprotein exprimieren. Die Lokalisation der CNTF-ir innervierten Glomeruli war interindividuell ähnlich, ihre Anzahl wies jedoch erhebliche Unterschiede auf. Dieses Phänomen lässt sich mit Befunden vergleichen, die im Rahmen von olfaktorischen Aktivitätsstudien bei Mäusen und Ratten erhoben wurden. Dabei beobachtete man eine Erhöhung der Anzahl aktivierter Glomeruli mit steigenden Geruchsstoffkonzentrationen. Auffallend war eine deutliche Übereinstimmung des Verteilungsmusters der CNTF-ir Glomeruli mit dem in der Literatur dargestellten Verteilungsmuster von Glomeruli, die durch Uringerüche aktiviert werden. Die räumliche Rekonstruktion der BO und die Darstellung der Position der CNTF-ir innervierten Glomeruli legt demnach eine neue mögliche Funktion von CNTF im olfaktorischen System nah: dessen Einbindung in Phänomene der Aktivität olfaktorischer Nervenzellen und plastischer Prozesse, die an der ersten Synapse der Geruchsbahn stattfinden. In der vorliegenden Arbeit konnte durch die Anwendung von klassischen Methoden der anatomisch-histologischen Forschung die Lokalisation von CNTF in der primären Geruchsbahn geklärt werden. Die Befunde führten zu weiteren Hypothesen hinsichtlich seiner funktionellen Einbindung in die olfaktorische Informationsverarbeitung, denen in zukünftigen Studien nachgegangen werden wird.
N2  - The olfactory system is bestowed with a set of remarkable features that render it an intriguing object for neurobiological research. It possesses the livelong capacity to regenerate, it displays an extraordinary wealth of neurotrophic factors and it is easily accessible to experimental manipulations. The current study aimed to deliver a comprehensive description of the localization and possible function of ciliary neurotrophic factor (CNTF) in the primary olfactory pathway by means of immunohistochemical methods. It could be shown that CNTF-immunoreactivity in rats and mice was localized in olfactory glia cells (ensheathing cells); using electron microscopy it was demonstrated that CNTF-immunoreactivity occurred both in the cytoplasm and the nucleus of ensheathing cells. Additionally, it was shown that CNTF can be also found in individual olfactory sensory neurons (OSN). Thus far, CNTF was known to be localized in peripheral and central glial cells only. Further characterization of neuroepithelial CNTF-occurrence revealed that CNTF-immunoreactive OSN are mature neurons displaying colocalization with the olfactory marker protein (OMP), a distinct marker protein for mature OSN. This was in line with absent colocalization of CNTF with Growth associated protein 43 (GAP-43) immunoreactivity, a marker of maturing OSN. CNTF could be implicated in the ongoing processes and neurode- and regeneration that take place in the olfactory epithelium. The olfactory mucosa is constantly exposed to the outer environment including noxious substances such as infectious agents, and extreme physical or chemical conditions. Hence, a permanent loss of OSN occurs which is counterbalanced with constant regeneration of neurons from neural precursor cells residing in the epithelium. Nuclei of CNTF-immunoreactive OSN did not display degenerative signs such as condensation or fragmentation that mark harmed degenerating cells. In addition to that no colocalization of CNTF and the apoptotic executor enzyme activated capsase-3 could be found in the olfactory epithelium. Even after chemical lesions of the olfactory epithelium of mice that cause necrotic cell death no enhanced incidence of CNTF-immunoreactive OSN was noted. Therefore, an implication of CNTF in neuronal degenerative processes in the olfactory mucosa seems unlikely. An alternative explanation for the individual neuronal localization of CNTF-immunoreactivity relied on the assumption that CNTF could be associated with the expression of olfactory receptor proteins (ORP). Three-dimensional reconstructions of rat and mice olfactory bulb pairs demonstrated the axonal projections of CNTF-immunoreactive OSN in olfactory glomeruli, which where found to be located at bilaterally symmetrical positions. This symmetry is also notable for OSN that express the identical ORP. The localization of CNTF-immunoreactive glomeruli was interindividually similar although they substantially differed in their numbers between animals. This phenomenon is reminiscent of results from olfactory activity studies obtained from rats and mice. It was observed that an increasing number of olfactory glomeruli is recruited due to an elevation of the odour concentration that the animals was exposed to. The distribution pattern of CNTF-immunoreactive glomeruli was comparable to glomerular activity maps elicited by urine odours. Hence, the three-dimensional reconstruction of olfactory bulbs and the localization of CNTF-immunoreactive glomeruli indicate a possible role for CNTF in activity-dependent processes of OSN and in neuroplastic mechanisms that occur at the first synapse of the primary olfactory pathway. In the current dissertation the localization of CNTF in the primary olfactory pathway was untangled by means of classical anatomical-histological techniques. The results yielded further hypotheses regarding the functional relationship of CNTF with olfactory information processing, which will be followed by future investigations.
KW  - CNTF
KW  - neurotrophe Faktoren
KW  - Neuroregeneration
KW  - Olfaktion
KW  - Geruchssystem
KW  - CNTF
KW  - neurotrophic facors
KW  - neuroregeneration
KW  - olfaction
KW  - olfactory system
Y1  - 2004
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-16009
ER  - 
TY  - JOUR
A1  - Gredic, Marija
A1  - Karnati, Srikanth
A1  - Ruppert, Clemens
A1  - Guenther, Andreas
A1  - Avdeev, Sergey N.
A1  - Kosanovic, Djuro
T1  - Combined pulmonary fibrosis and emphysema: when Scylla and Charybdis ally
JF  - Cells
N2  - Combined pulmonary fibrosis and emphysema (CPFE) is a recently recognized syndrome that, as its name indicates, involves the existence of both interstitial lung fibrosis and emphysema in one individual, and is often accompanied by pulmonary hypertension. This debilitating, progressive condition is most often encountered in males with an extensive smoking history, and is presented by dyspnea, preserved lung volumes, and contrastingly impaired gas exchange capacity. The diagnosis of the disease is based on computed tomography imaging, demonstrating the coexistence of emphysema and interstitial fibrosis in the lungs, which might be of various types and extents, in different areas of the lung and several relative positions to each other. CPFE bears high mortality and to date, specific and efficient treatment options do not exist. In this review, we will summarize current knowledge about the clinical attributes and manifestations of CPFE. Moreover, we will focus on pathophysiological and pathohistological lung phenomena and suspected etiological factors of this disease. Finally, since there is a paucity of preclinical research performed for this particular lung pathology, we will review existing animal studies and provide suggestions for the development of additional in vivo models of CPFE syndrome.
KW  - CPFE
KW  - lung fibrosis
KW  - emphysema
KW  - animal models
Y1  - 2023
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-313571
SN  - 2073-4409
VL  - 12
IS  - 9
ER  - 
TY  - JOUR
A1  - Artyukova, E. V.
A1  - Gorboulev, Valentin G.
A1  - Rodionova, N. P.
A1  - Krylov, A. V.
A1  - Atabekov, J. G.
T1  - Comparative study of structural peculiarities and translation of potexvirus RNAs
N2  - Structural peculiarities of the S'-end segments of genomic RNA were studied in F potato virus (F-PV) and white clover mosaic virus (WCMV). The methods of affinity chromatography on oligo(dT) cellulose and oligonucleotide mapping revealed a prolonged (up to 210 nucleotides) polyadenyl sequence at the 3'-end of F-PV RNA. A polyadenyl sequence is missing at the 3'end of WCMV RNA. A study of the translation products of WCMV and F-PV RNAs in a oe11-free protein-synthesizing system derived from rabbit reticulocytes showed that polypeptides electrophoretically comigrating with a structural protein of either virus were synthesized alongside high-molecular-weight polypeptides (M\(_r\)\(\approx\) 180-150 kdaltons).
Y1  - 1985
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-46985
ER  - 
TY  - JOUR
A1  - Gruschwitz, Philipp
A1  - Hartung, Viktor
A1  - Ergün, Süleyman
A1  - Peter, Dominik
A1  - Lichthardt, Sven
A1  - Huflage, Henner
A1  - Hendel, Robin
A1  - Pannenbecker, Pauline
A1  - Augustin, Anne Marie
A1  - Kunz, Andreas Steven
A1  - Feldle, Philipp
A1  - Bley, Thorsten Alexander
A1  - Grunz, Jan-Peter
T1  - Comparison of ultrahigh and standard resolution photon-counting CT angiography of the femoral arteries in a continuously perfused in vitro model
JF  - European Radiology Experimental
N2  - Background
With the emergence of photon-counting CT, ultrahigh-resolution (UHR) imaging can be performed without dose penalty. This study aims to directly compare the image quality of UHR and standard resolution (SR) scan mode in femoral artery angiographies.

Methods
After establishing continuous extracorporeal perfusion in four fresh-frozen cadaveric specimens, photon-counting CT angiographies were performed with a radiation dose of 5 mGy and tube voltage of 120 kV in both SR and UHR mode. Images were reconstructed with dedicated convolution kernels (soft: Body-vascular (Bv)48; sharp: Bv60; ultrasharp: Bv76). Six radiologists evaluated the image quality by means of a pairwise forced-choice comparison tool. Kendall’s concordance coefficient (W) was calculated to quantify interrater agreement. Image quality was further assessed by measuring intraluminal attenuation and image noise as well as by calculating signal-to-noise ratio (SNR) and contrast-to-noise ratios (CNR).

Results
UHR yielded lower noise than SR for identical reconstructions with kernels ≥ Bv60 (p < 0.001). UHR scans exhibited lower intraluminal attenuation compared to SR (Bv60: 406.4 ± 25.1 versus 418.1 ± 30.1 HU; p < 0.001). Irrespective of scan mode, SNR and CNR decreased while noise increased with sharper kernels but UHR scans were objectively superior to SR nonetheless (Bv60: SNR 25.9 ± 6.4 versus 20.9 ± 5.3; CNR 22.7 ± 5.8 versus 18.4 ± 4.8; p < 0.001). Notably, UHR scans were preferred in subjective assessment when images were reconstructed with the ultrasharp Bv76 kernel, whereas SR was rated superior for Bv60. Interrater agreement was high (W = 0.935).

Conclusions
Combinations of UHR scan mode and ultrasharp convolution kernel are able to exploit the full image quality potential in photon-counting CT angiography of the femoral arteries.

Relevance statement
The UHR scan mode offers improved image quality and may increase diagnostic accuracy in CT angiography of the peripheral arterial runoff when optimized reconstruction parameters are chosen.

Key points
• UHR photon-counting CT improves image quality in combination with ultrasharp convolution kernels.

• UHR datasets display lower image noise compared with identically reconstructed standard resolution scans.

• Scans in UHR mode show decreased intraluminal attenuation compared with standard resolution imaging.
KW  - CT angiography
KW  - femoral arteries
KW  - photon-counting computed tomography (CT)
KW  - small pixel effect
KW  - ultrahigh resolution
Y1  - 2023
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-357905
VL  - 7
ER  - 
TY  - JOUR
A1  - Gruschwitz, Philipp
A1  - Hartung, Viktor
A1  - Kleefeldt, Florian
A1  - Peter, Dominik
A1  - Lichthardt, Sven
A1  - Huflage, Henner
A1  - Grunz, Jan-Peter
A1  - Augustin, Anne Marie
A1  - Ergün, Süleyman
A1  - Bley, Thorsten Alexander
A1  - Petritsch, Bernhard
T1  - Continuous extracorporeal femoral perfusion model for intravascular ultrasound, computed tomography and digital subtraction angiography
JF  - PLoS One
N2  - Objectives
We developed a novel human cadaveric perfusion model with continuous extracorporeal femoral perfusion suitable for performing intra-individual comparison studies, training of interventional procedures and preclinical testing of endovascular devices. Objective of this study was to introduce the techniques and evaluate the feasibility for realistic computed tomography angiography (CTA), digital subtraction angiography (DSA) including vascular interventions, and intravascular ultrasound (IVUS).

Methods
The establishment of the extracorporeal perfusion was attempted using one formalin-fixed and five fresh-frozen human cadavers. In all specimens, the common femoral and popliteal arteries were prepared, introducer sheaths inserted, and perfusion established by a peristaltic pump. Subsequently, we performed CTA and bilateral DSA in five cadavers and IVUS on both legs of four donors. Examination time without unintentional interruption was measured both with and without non-contrast planning CT. Percutaneous transluminal angioplasty and stenting was performed by two interventional radiologists on nine extremities (five donors) using a broad spectrum of different intravascular devices.

Results
The perfusion of the upper leg arteries was successfully established in all fresh-frozen but not in the formalin-fixed cadaver. The experimental setup generated a stable circulation in each procedure (ten upper legs) for a period of more than six hours. Images acquired with CT, DSA and IVUS offered a realistic impression and enabled the sufficient visualization of all examined vessel segments. Arterial cannulating, percutaneous transluminal angioplasty as well as stent deployment were feasible in a way that is comparable to a vascular intervention in vivo. The perfusion model allowed for introduction and testing of previously not used devices.

Conclusions
The continuous femoral perfusion model can be established with moderate effort, works stable, and is utilizable for medical imaging of the peripheral arterial system using CTA, DSA and IVUS. Therefore, it appears suitable for research studies, developing skills in interventional procedures and testing of new or unfamiliar vascular devices.
KW  - continuous extracorporeal femoral perfusion model
KW  - novel human cadaveric perfusion model
KW  - computed tomography angiography (CTA)
KW  - digital subtraction angiography (DSA)
KW  - intravascular ultrasound (IVUS)
Y1  - 2023
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-350136
SN  - 1932-6203
VL  - 18
IS  - 5
ER  - 
TY  - JOUR
A1  - Upcin, Berin
A1  - Henke, Erik
A1  - Kleefeldt, Florian
A1  - Hoffmann, Helene
A1  - Rosenwald, Andreas
A1  - Irmak-Sav, Ster
A1  - Aktas, Huseyin Bertal
A1  - Rückschloß, Uwe
A1  - Ergün, Süleyman
T1  - Contribution of adventitia-derived stem and progenitor cells to new vessel formation in tumors
JF  - Cells
N2  - Blocking tumor vascularization has not yet come to fruition to the extent it was hoped for, as angiogenesis inhibitors have shown only partial success in the clinic. We hypothesized that under- appreciated vascular wall-resident stem and progenitor cells (VW-SPCs) might be involved in tumor vascularization and influence effectiveness of anti-angiogenic therapy. Indeed, in patient samples, we observed that vascular adventitia-resident CD34\(^+\) VW-SPCs are recruited to tumors in situ from co-opted vessels. To elucidate this in detail, we established an ex vivo model using concomitant embedding of multi-cellular tumor spheroids (MCTS) and mouse aortic rings (ARs) into collagen
gels, similar to the so-called aortic ring assay (ARA). Moreover, ARA was modified by removing the ARs’ adventitia that harbors VW-SPCs. Thus, this model enabled distinguishing the contribution of VW-SPCs from that of mature endothelial cells (ECs) to new vessel formation. Our results show that the formation of capillary-like sprouts is considerably delayed, and their number and network formation were significantly reduced by removing the adventitia. Substituting iPSC-derived neural spheroids for MCTS resulted in distinct sprouting patterns that were also strongly influenced by the
presence or absence of VW-SPCs, also underlying the involvement of these cells in non-pathological vascularization. Our data suggest that more comprehensive approaches are needed in order to block all of the mechanisms contributing to tumor vascularization.
KW  - vascularization model
KW  - tumor spheroids
KW  - vascular wall stem and progenitor cells
KW  - aortic adventitia
KW  - vasculogenesis
KW  - tumor-vessel wall-interface model
Y1  - 2021
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-242577
VL  - 10
IS  - 7
ER  - 
TY  - THES
A1  - Upcin, Berin
T1  - Contribution of vascular adventitia-resident progenitor cells to new vessel formation in \(ex\) \(vivo\) 3D models
T1  - Der Beitrag der Gefäßwandadventitia-residenten Vorläuferzellen zur Neovaskularisation in \(ex\) \(vivo\) 3D Modellen
N2  - Ongoing research to fight cancer, one of the dominant diseases of the 21st century has led to big progress especially when it comes to understanding the tumor growth and metastasis. This includes the discovery of the molecular mechanisms of tumor vascularization, which is critically required for establishment of tumor metastasis. 
Formation of new blood vessels is the first step in tumor vascularization. Therefore, understanding the molecular and cellular basis of tumor vascularization attracted a significant effort studying in biomedical research. The blood vessels for supplying tumor can be formed by sprouting from pre-existing vessels, a process called angiogenesis, or by vasculogenesis, that is de novo formation of blood vessels from not fully differentiated progenitor cell populations. Vasculogenic endothelial progenitor cells (EPCs) can either be activated from populations in the bone marrow reaching the pathological region via the circulation or they can be recruited from local reservoirs. Neovessel formation influences tumor progression, hence therapeutic response model systems of angiogenesis/vasculogenesis are necessary to study the underlying mechanisms. Although, initially the research in this area focused more on angiogenesis, it is now well understood that both angiogenesis and postnatal vasculogenesis contribute to neovessel formation in adult under both most pathological as well as physiological conditions. Studies in the last two decades demonstrate that in addition to the intimal layer of fully differentiated mature endothelial cells (ECs) and various smaller supplying vessels (vasa vasorum) that can serve as a source for new vessels by angiogenesis, especially the adventitia of large and medium size blood vessels harbors various vascular wall-resident stem and progenitor cells (VW-SPCs) populations that serve as a source for new vessels by postnatal vasculogenesis. However, little is known about the potential role of VW-SPCs in tumor vascularization. 
 To this end, the present work started first to establish a modified aortic ring assay (ARA) using mouse aorta in order to study the contribution of vascular adventitia-resident VW-SPCs to neovascularization in general and in presence of tumor cells. ARA is already established an ex vivo model for neovascularization allows to study the morphogenetic events of complex new vessel formation that includes all layers of mature blood vessels, a significant advantage over the assays that employ monolayer endothelial cell cultures. Moreover, in contrast to assays employing endothelial cells monocultures, both angiogenic and vasculogenic events take place during new vessel formation in ARA although the exact contribution of these two processes to new vessel formation cannot be easily distinguished in conventional ARA. Thus, in this study, a modified protocol for the ARA (mdARA) was established by either removing or keeping the aortic adventitia in place. The mdARA allows to distinguish the role of VW-SPCs from those of other aortic layers. The present data show that angiogenic sprouting from mature aortic endothelium was markedly delayed when the adventitial layer was removed. Furthermore, the network between the capillary-like sprouts was significantly reduced in absence of aortic adventitia. Moreover, the stabilization of new sprouts by assembling the NG2+ pericyte-like cells that enwrapped the endothelial sprouts from the outside was improved when the adventitial layer remained in place. 
Next, mimicking the tumor-vessel adventitia-interaction, multicellular tumor spheroids (MCTS) and aortic rings (ARs) with or without adventitia of C57BL/6-Tg (UBC-GFP) mice were confronted within the collagen gel and cultured ex vivo. This 3D model enabled analysis of the mobilization, migration and capillary-like sprouts formation by VW-SPCs within tumor-vessel wall-interface in comparison to tumor-free side of the ARs. Interestingly, while MCTS preferred the uptake of single vascular adventitia-derived cells, neural spheroids were directly penetrated by capillary-like structures that were sprouted from the aortic adventitia. In summary, the model established in this work allows to study new vessel formation by both postnatal vasculogenesis and angiogenesis under same conditions. It can be applied in various mouse models including reporter mouse models, e.g. Cxcr1 CreER+/mTmG+/- mice, in which GFP-marked macrophages of the vessel wall were directly observed as they mobilized from their niche and migrated into collagen gel. Another benefit of the model is that it can be used for testing different factors such as small molecules, growth factors, cytokines, and drugs with both pro- and anti-angiogenic/vasculogenic effects.
N2  - Die Forschungsarbeiten der letzten Jahrzehnte zur Bekämpfung der Krebserkrankung, einer der dominierenden Krankheiten des 21. Jahrhunderts, haben zu großen Fortschritten, insbesondere im Verständnis bezüglich der Tumormetastasierung geführt. Dies schließt die Prozesse der Tumorvaskularisierung als einen der initialen Schritte der Metastasierung mit ein, die nach wie vor nicht ausreichend geklärt sind. 
Die Blutgefäßbildung zur Versorgung des Tumorgewebes kann durch die Anagiogenese, die als Einsprießen neuer Gefäße aus den bereits vorhandenen Blutgefäßen definiert wird, oder durch die Vaskulogenese, die als Gefäßneubildung aus Stamm- und Vorläuferzellen beschrieben wird, sichergestellt werden. Noch nicht vollständig ausdifferenzierte endotheliale Vorläuferzellen (EPCs) werden dabei nach dem bisherigen Kenntnistand aus dem Knochenmark rekrutiert und erreichen die Regionen der Gefäßneubildung über die Blutzirkulation und können dort zur de novo Formierung neuer Blutgefäße auch beim Erwachsenen beitragen. Untersuchungen der letzten zwei Dekaden haben gezeigt, dass solche Vorläuferzellen auch aus lokalen Reservoiren, wie z.B. aus der Gefäßwandadventitia der bereits existierenden Blutgefäße mobilisiert werden. Da die Bildung neuer Gefäße einen direkten Einfluss auf die Tumorprogression hat, sind entsprechende Modellsysteme notwendig, um die zugrundeliegenden Mechanismen möglichst präzise zu untersuchen. Obwohl sich die Forschung der Tumorvaskularisierung zunächst auf Prozesse der Angiogenese konzentrierte, ist es mittlerweile ausreichend belegt, dass auch die Vaskulogenese zur Tumorvaskularisierung beiträgt und somit die Tumorprogression beeinflusst. 
Anhand einer Vielzahl an Studien der letzten zwei Jahrzehnte konnte demonstriert werden, dass sich, neben der Intimaschicht, die vollständig differenzierte Endothelzellen (ECs) enthält und kleineren Gefäßwand-versorgenden Blutgefäßen, der sogenannten Vasa vasorum in der Adventitia der großen Gefäße, auch Populationen gefäßwandresidenter Stamm- und Vorläuferzellen (VW-SPCs) in der äußeren Gefäßwandschicht, nämlich der Adventitia fast aller Gefäßabschnitte nachweisen lassen. Obwohl diese als Quelle neuer Gefäße in der postnatalen Vaskulogenese beschrieben sind, ist nach wie vor wenig über die potenzielle Rolle von VW-SPCs in der Tumorvaskularisation bekannt. 
Daher wurde im Rahmen dieser Arbeit zuerst ein modifiziertes Aortic Ringassay (ARA) unter Verwendung der Mausaorta etabliert, um den Beitrag der VW-SPCs zur Neovaskularisierung im Allgemeinen und zur Tumorvaskularisierung im Speziellen ex vivo untersuchen zu können. ARA ist ein bereits seit einigen Jahrzehnten etabliertes ex vivo Modell zur Untersuchung der Gefäßneubildung durch Angiogenese. Mittels ARA kann die Bildung komplexer vaskulärer Strukturen in Präsenz aller Wandschichten reifer Blutgefäße untersucht werden, was einen wesentlichen Vorteil gegenüber der Verwendung von Endothelzellkulturen in Monolayer bedeutet. Hierbei ist jedoch anzumerken, dass in ARA sowohl angiogene als auch vaskulogene Prozesse zur Gefäßbildung beitragen, aber der genaue Beitrag beider Prozesse schwer oder kaum voneinander unterscheidbar ist. Daher wurde im Rahmen dieser Arbeit ein modifiziertes ARA-Protokoll etabliert (mdARA), in welchem die aortale Adventitia vor dem Beginn des ARA entweder entfernt oder belassen wurde und somit die Rolle der VW-SPCs bei der Gefäßsprossung von den Zellen anderer Aortenwandschichten differenziert studiert werden konnte. Die dabei generierten Daten zeigen, dass sich die angiogene Aussprossung aus dem reifen Aortenendothel nach Entfernung der adventitialen Schicht deutlich verzögerte. Darüber hinaus war das Netzwerk zwischen den kapillarartigen Sprossen in Abwesenheit der Aortenadventitia signifikant reduziert. Mehr noch, das Belassen der adventitialen Wandstruktur führte zu einer verbesserten Stabilisierung neuer Gefäßsprossen. Als sichtbares Korrelat hierfür zeigte sich eine stärkere und bessere Anlagerung der NG2+ Perizyten-ähnlichen Zellen zu den endothelialen Kapillar-ähnlichen Aussprossungen von außen, wie Perizyten an der Kapillarwand in situ.
Als nächstes wurden die Aortenringe (ARs) von C57BL/6-Tg (UBC-GFP)-Mäusen mit multizellulären Tumor-Sphäroiden (MCTS) in Kollagengel ko-kultiviert, um die Interaktion zwischen Tumor und Gefäßwand-Adventitia ex vivo nachzuahmen. Dieses 3D Modell ermöglichte die Analyse der Mobilisierung und Migration der VW-SPCs von der aortalen Adventitia sowohl zu der Tumorseite in den Tumor-Gefäßwand-Interfaces als auch zu der tumorfreien Seite der Aortenringe. Interessanterweise wurde die Kapillarsprossung im Tumor-Gefäßwand-Interface an der Grenze zum MCTS gestoppt und die VW-SPCs als Einzelzellen in die MCTS aufgenommen. Demgegenüber wurde auf der tumor-freien Seite der Aortenringe eine deutlich längere Kapillaraussprossung beobachtet. Im Gegensatz zu MCTS resultierte die Ko-Kultivierung der ARs mit neuronalen Spheroiden darin, dass die aus der aortalen Adventitia aussprossenden Kapillar-ähnlichen Strukturen direkt in die neuronalen Spheroide penetrierten. Zusammenfassend berücksichtigt dieses neuartige in vitro 3D-Modell sowohl Angiogenese als auch Vaskulogenese und bietet vielfältige Vorteile, wie zum Beispiel die Kompatibilität zu verschiedenen Mausmodellen einschließlich der Reporter-Mausmodelle, wie z.B. die in dieser Arbeit gezeigte Verwendung der Aorta von Cxcr1 CreER+/mTmG+/- um die GFP-markierten Makrophagen aus der Gefäßwand bei der Gefäßaussprossung studieren zu können. Des Weiteren ist dieses Model auch für Testung unterschiedlicher Faktoren und Therapeutika einschließlich der anti-angiogenen und -vasculogenen Substanzen unter ex vivo Bedingungen geeignet.  
KW  - Progenitor
KW  - Adventitia
Y1  - 2022
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-255070
ER  - 
TY  - JOUR
A1  - Arndt, Andreas
A1  - Hoffacker, Peter
A1  - Zellmer, Konstantin
A1  - Goecer, Oktay
A1  - Recks, Mascha S.
A1  - Kuerten, Stefanie
T1  - Conventional Housing Conditions Attenuate the Development of Experimental Autoimmune Encephalomyelitis
JF  - PLoS ONE
N2  - BACKGROUND:
The etiology of multiple sclerosis (MS) has remained unclear, but a causative contribution of factors outside the central nervous system (CNS) is conceivable. It was recently suggested that gut bacteria trigger the activation of CNS-reactive T cells and the development of demyelinative disease.
METHODS:
C57BL/6 (B6) mice were kept either under specific pathogen free or conventional housing conditions, immunized with the myelin basic protein (MBP)-proteolipid protein (PLP) fusion protein MP4 and the development of EAE was clinically monitored. The germinal center size of the Peyer's patches was determined by immunohistochemistry in addition to the level of total IgG secretion which was assessed by ELISPOT. ELISPOT assays were also used to measure MP4-specific T cell and B cell responses in the Peyer's patches and the spleen. Ear swelling assays were performed to determine the extent of delayed-type hypersensitivity reactions in specific pathogen free and conventionally housed mice.
RESULTS:
In B6 mice that were actively immunized with MP4 and kept under conventional housing conditions clinical disease was significantly attenuated compared to specific pathogen free mice. Conventionally housed mice displayed increased levels of IgG secretion in the Peyer's patches, while the germinal center formation in the gut and the MP4-specific TH17 response in the spleen were diminished after immunization. Accordingly, these mice displayed an attenuated delayed type hypersensitivity (DTH) reaction in ear swelling assays.
CONCLUSIONS:
The data corroborate the notion that housing conditions play a substantial role in the induction of murine EAE and suggest that the presence of gut bacteria might be associated with a decreased immune response to antigens of lower affinity. This concept could be of importance for MS and calls for caution when considering the therapeutic approach to treat patients with antibiotics."
KW  - B cells
KW  - secretion
KW  - multiple sclerosis
KW  - enzyme-linked immunoassays
KW  - Peyer's patches
KW  - gut bacteria
KW  - T cells
KW  - immune response
Y1  - 2014
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-119603
VL  - 9
IS  - 6
ER  - 
TY  - JOUR
A1  - Janz, Anna
A1  - Zink, Miriam
A1  - Cirnu, Alexandra
A1  - Hartleb, Annika
A1  - Albrecht, Christina
A1  - Rost, Simone
A1  - Klopocki, Eva
A1  - Günther, Katharina
A1  - Edenhofer, Frank
A1  - Ergün, Süleyman
A1  - Gerull, Brenda
T1  - CRISPR/Cas9-edited PKP2 knock-out (JMUi001-A-2) and DSG2 knock-out (JMUi001-A-3) iPSC lines as an isogenic human model system for arrhythmogenic cardiomyopathy (ACM)
JF  - Stem Cell Research
N2  - Arrhythmogenic cardiomyopathy (ACM) is characterized by fibro-fatty replacement of the myocardium, heart failure and life-threatening ventricular arrhythmias. Causal mutations were identified in genes encoding for proteins of the desmosomes, predominantly plakophilin-2 (PKP2) and desmoglein-2 (DSG2). We generated gene-edited knock-out iPSC lines for PKP2 (JMUi001-A-2) and DSG2 (JMUi001-A-3) using the CRISPR/Cas9 system in a healthy control iPSC background (JMUi001A). Stem cell-like morphology, robust expression of pluripotency markers, embryoid body formation and normal karyotypes confirmed the generation of high quality iPSCs to provide a novel isogenic human in vitro model system mimicking ACM when differentiated into cardiomyocytes.
KW  - mutations
Y1  - 2021
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-259846
VL  - 53
ER  - 
TY  - JOUR
A1  - Wagner, Nicole
A1  - Mott, Kristina
A1  - Upcin, Berin
A1  - Stegner, David
A1  - Schulze, Harald
A1  - Ergün, Süleyman
T1  - CXCL12-abundant reticular (CAR) cells direct megakaryocyte protrusions across the bone marrow sinusoid wall
JF  - Cells
N2  - Megakaryocytes (MKs) release platelets into the lumen of bone marrow (BM) sinusoids while remaining to reside within the BM. The morphogenetic events of this complex process are still not fully understood. We combined confocal laser scanning microscopy with transmission and serial block-face scanning electron microscopy followed by 3D-reconstruction on mouse BM tissue sections. These analyses revealed that MKs in close vicinity to BM sinusoid (BMS) wall first induce the lateral retraction of CXCL12-abundant reticular (CAR) cells (CAR), followed by basal lamina (BL) degradation enabling direct MK-sinusoidal endothelial cells (SECs) interaction. Subsequently, an endothelial engulfment starts that contains a large MK protrusion. Then, MK protrusions penetrate the SEC, transmigrate into the BMS lumen and form proplatelets that are in direct contact to the SEC surface. Furthermore, such processes are induced on several sites, as observed by 3D reconstructions. Our data demonstrate that MKs in interaction with CAR-cells actively induce BMS wall alterations, including CAR-cell retraction, BL degradation, and SEC engulfment containing a large MK protrusion. This results in SEC penetration enabling the migration of MK protrusion into the BMS lumen where proplatelets that are adherent to the luminal SEC surface are formed and contribute to platelet release into the blood circulation.
KW  - megakaryocytes
KW  - microvasculature
KW  - CXCL12-abundant reticular (CAR)-cells
Y1  - 2021
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-234180
SN  - 2073-4409
VL  - 10
IS  - 4
ER  - 
TY  - JOUR
A1  - Schampel, Andrea
A1  - Kuerten, Stefanie
T1  - Danger: high voltage - the role of voltage-gated calcium channels in central nervous system pathology
JF  - Cells
N2  - Voltage-gated calcium channels (VGCCs) are widely distributed within the central nervous system (CNS) and presumed to play an important role in the pathophysiology of a broad spectrum of CNS disorders including Alzheimer’s and Parkinson’s disease as well as multiple sclerosis. Several calcium channel blockers have been in clinical practice for many years so that their toxicity and side effects are well studied. However, these drugs are primarily used for the treatment of cardiovascular diseases and most if not all effects on brain functions are secondary to peripheral effects on blood pressure and circulation. While the use of calcium channel antagonists for the treatment of CNS diseases therefore still heavily depends on the development of novel strategies to specifically target different channels and channel subunits, this review is meant to provide an impulse to further emphasize the importance of future research towards this goal.
KW  - cells
KW  - calcium
KW  - calcium channel antagonists
KW  - CNS
KW  - EAE
KW  - neurodegeneration
KW  - MS
KW  - regeneration
KW  - remyelination
Y1  - 2017
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-172653
VL  - 6
IS  - 4
ER  - 
TY  - THES
A1  - Wunsch, Marie
T1  - Das enterische Nervensystem als mögliche Zielstruktur der Autoimmunreaktion in der Multiplen Sklerose
T1  - The enteric nervous system is a potential autoimmune target in multiple sclerosis
N2  - Bei der Multiplen Sklerose (MS) handelt es sich um eine Autoimmunerkrankung des zentralen Nervensystems (ZNS). Abhängig von der betroffenen ZNS-Region kann es zu vielfältigen Symptomen kommen. Neben neurologischen Symptomen verursacht durch ZNS-Läsionen leidet ein Großteil der MS-Patienten auch unter gastrointestinalen Funktionsstörungen. Diese gastrointestinalen Symptome wurden bisher eher auf Läsionen im Rückenmark zurückgeführt und nicht direkt in Verbindung mit der autoimmunen Ätiologie der Erkrankung gebracht.
In dieser Studie wurde das enterische Nervensystem (ENS) in einem B-Zell- und Antikörper-abhängigen Mausmodell der MS untersucht. Dafür wurde der Autoimmunprozess durch Immunisierung mit MP4, einem Fusionsprotein aus dem Myelin-Basischen-Protein (MBP) und dem Proteolipid-Protein (PLP), ausgelöst. Das ZNS und ENS wurden in den unterschiedlichen Erkrankungsstadien immunhistochemisch und elektronenmikroskopisch analysiert. Neben der Immunpathologie des ZNS konnte dabei eine Degeneration des ENS schon vor dem Einsetzen der ersten neurologischen Defizite nachgewiesen werden. Die ENS-Pathologie war antikörper-mediiert und ging einher mit einer verringerten gastrointestinalen Motilität sowie mit einer Gliose und Neurodegeneration des ENS.
Mithilfe von Immunpräzipitation und Massenspektrometrie konnten im ENS vier mögliche Zielstrukturen des Autoimmunprozesses identifiziert werden, was auf sog. epitope spreading hindeutet. Auch im Plasma von MS-Patienten konnten Antikörper gegen drei dieser Antigene nachgewiesen werden. Des Weiteren zeigten sich in Kolon-Resektaten von MS-Patienten erste Ansätze einer Neurodegeneration und Gliose des ENS. 
In dieser Studie wurde zum ersten Mal ein direkter Zusammenhang zwischen der Autoimmunreaktion gegen das ZNS und einer simultanen Reaktion gegen das ENS gezeigt. Dies kann einen Paradigmenwechsel im Verständnis der Immunpathogenese der MS anstoßen und neue therapeutische und diagnostische Ansätze initiieren.
N2  - Multiple sclerosis (MS) is a chronic autoimmune disease, in which the immune system attacks the central nervous system (CNS). Clinical symptoms and the course of the disease can vary among patients, depending on the region of the brain primarily affected. Besides the neurological symptoms caused by CNS lesions, a great amount of MS patients display functional gastrointestinal impairments. Gastrointestinal symptoms were previously explained by the presence of spinal cord lesions rather than being linked to the autoimmune pathomechanisms of the disease. 
Here, the enteric nervous system (ENS) was studied in a B cell- and antibody-dependent mouse model of MS, in which the myelin basic protein (MBP) - proteolipid protein (PLP) fusion protein MP4 was used to initiate the autoimmune attack. Immunohistochemistry and electron microscopy were performed at different stages of the disease. We noted that in addition to the immune pathology in the CNS itself, the ENS also showed signs of degeneration. ENS degeneration was evident prior to the manifestation of CNS lesions and to the onset of neurological deficits in mice. ENS pathology was antibody-mediated and accompanied by impaired gastrointestinal motility, ENS gliosis and neurodegeneration. Using immunoprecipitation and mass spectrometry, four autoimmune targets expressed by enteric glia and/or neurons could be identified suggesting that epitope spreading to antigens of the ENS had occurred. MS patients displayed plasma antibodies against three of the ENS autoantigens. Studying human colon resectates provided preliminary evidence for gliosis and neurodegeneration of the ENS in MS patients, which was absent in non-MS controls.
Overall, this study establishes a pathomechanistic link between the well-established autoimmune attack on the CNS and a simultaneous attack on the ENS that has not been described so far. These findings can initiate a paradigm shift in the current understanding of the pathomechanism of MS with diagnostic and therapeutic implications.
KW  - Multiple Sklerose
KW  - Autoantikörper
KW  - Enterisches Nervensystem
KW  - Experimentelle Autoimmune Enzephalomyelitis
KW  - Darmwandnervensystem
KW  - Autoimmunität
Y1  - 2019
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-175888
ER  - 
TY  - JOUR
A1  - Bielmeier, Christina B.
A1  - Schmitt, Sabrina I.
A1  - Kleefeldt, Nikolai
A1  - Boneva, Stefaniya K.
A1  - Schlecht, Anja
A1  - Vallon, Mario
A1  - Tamm, Ernst R.
A1  - Hillenkamp, Jost
A1  - Ergün, Süleyman
A1  - Neueder, Andreas
A1  - Braunger, Barbara M.
T1  - Deficiency in retinal TGFβ signaling aggravates neurodegeneration by modulating pro-apoptotic and MAP kinase pathways
JF  - International Journal of Molecular Sciences
N2  - Transforming growth factor β (TGFβ) signaling has manifold functions such as regulation of cell growth, differentiation, migration, and apoptosis. Moreover, there is increasing evidence that it also acts in a neuroprotective manner. We recently showed that TGFβ receptor type 2 (Tgfbr2) is upregulated in retinal neurons and Müller cells during retinal degeneration. In this study we investigated if this upregulation of TGFβ signaling would have functional consequences in protecting retinal neurons. To this end, we analyzed the impact of TGFβ signaling on photoreceptor viability using mice with cell type-specific deletion of Tgfbr2 in retinal neurons and Müller cells (Tgfbr2\(_{ΔOC}\)) in combination with a genetic model of photoreceptor degeneration (VPP). We examined retinal morphology and the degree of photoreceptor degeneration, as well as alterations of the retinal transcriptome. In summary, retinal morphology was not altered due to TGFβ signaling deficiency. In contrast, VPP-induced photoreceptor degeneration was drastically exacerbated in double mutant mice (Tgfbr2\(_{ΔOC}\); VPP) by induction of pro-apoptotic genes and dysregulation of the MAP kinase pathway. Therefore, TGFβ signaling in retinal neurons and Müller cells exhibits a neuroprotective effect and might pose promising therapeutic options to attenuate photoreceptor degeneration in humans.
KW  - TGFβ signaling
KW  - retina
KW  - retinitis pigmentosa
KW  - neuro-/photoreceptor degeneration
KW  - MAP kinase pathway
KW  - ferroptosis
Y1  - 2022
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-283971
SN  - 1422-0067
VL  - 23
IS  - 5
ER  -