TY - JOUR A1 - Baum, Petra A1 - Toyka, Klaus V. A1 - Blüher, Matthias A1 - Kosacka, Joanna A1 - Nowicki, Marcin T1 - Inflammatory mechanisms in the pathophysiology of diabetic peripheral neuropathy (DN) — new aspects JF - International Journal of Molecular Sciences N2 - The pathogenesis of diabetic neuropathy is complex, and various pathogenic pathways have been proposed. A better understanding of the pathophysiology is warranted for developing novel therapeutic strategies. Here, we summarize recent evidence from experiments using animal models of type 1 and type 2 diabetes showing that low-grade intraneural inflammation is a facet of diabetic neuropathy. Our experimental data suggest that these mild inflammatory processes are a likely common terminal pathway in diabetic neuropathy associated with the degeneration of intraepidermal nerve fibers. In contrast to earlier reports claiming toxic effects of high-iron content, we found the opposite, i.e., nutritional iron deficiency caused low-grade inflammation and fiber degeneration while in normal or high non-heme iron nutrition no or only extremely mild inflammatory signs were identified in nerve tissue. Obesity and dyslipidemia also appear to trigger mild inflammation of peripheral nerves, associated with neuropathy even in the absence of overt diabetes mellitus. Our finding may be the experimental analog of recent observations identifying systemic proinflammatory activity in human sensorimotor diabetic neuropathy. In a rat model of type 1 diabetes, a mild neuropathy with inflammatory components could be induced by insulin treatment causing an abrupt reduction in HbA1c. This is in line with observations in patients with severe diabetes developing a small fiber neuropathy upon treatment-induced rapid HbA1c reduction. If the inflammatory pathogenesis could be further substantiated by data from human tissues and intervention studies, anti-inflammatory compounds with different modes of action may become candidates for the treatment or prevention of diabetic neuropathy. KW - diabetic neuropathy KW - pathogenesis KW - inflammation KW - iron KW - treatment-induced neuropathy in diabetes (TIND) Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-284556 SN - 1422-0067 VL - 22 IS - 19 ER - TY - JOUR A1 - Svensson, Sarah L. A1 - Sharma, Cynthia M. T1 - Small RNAs that target G-rich sequences are generated by diverse biogenesis pathways in Epsilonproteobacteria JF - Molecular Microbiology N2 - Bacterial small RNAs (sRNAs) are widespread post-transcriptional regulators that control bacterial stress responses and virulence. Nevertheless, little is known about how they arise and evolve. Homologs can be difficult to identify beyond the strain level using sequence-based approaches, and similar functionalities can arise by convergent evolution. Here, we found that the virulence-associated CJnc190 sRNA of the foodborne pathogen Campylobacter jejuni resembles the RepG sRNA from the gastric pathogen Helicobacter pylori. However, while both sRNAs bind G-rich sites in their target mRNAs using a C/U-rich loop, they largely differ in their biogenesis. RepG is transcribed from a stand-alone gene and does not require processing, whereas CJnc190 is transcribed from two promoters as precursors that are processed by RNase III and also has a cis-encoded antagonist, CJnc180. By comparing CJnc190 homologs in diverse Campylobacter species, we show that RNase III-dependent processing of CJnc190 appears to be a conserved feature even outside of C. jejuni. We also demonstrate the CJnc180 antisense partner is expressed in C. coli, yet here might be derived from the 3’UTR (untranslated region) of an upstream flagella-related gene. Our analysis of G-tract targeting sRNAs in Epsilonproteobacteria demonstrates that similar sRNAs can have markedly different biogenesis pathways. KW - sRNA biogenesis KW - Campylobacter jejuni KW - Helicobacter pylori KW - pathogenesis KW - RNase III Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-259602 VL - 117 ER - TY - JOUR A1 - Nattmann, Anja A1 - Breun, Maria A1 - Monoranu, Camelia M. A1 - Matthies, Cordula A1 - Ernestus, Ralf-Ingo A1 - Löhr, Mario A1 - Hagemann, Carsten T1 - Analysis of ADAM9 regulation and function in vestibular schwannoma primary cells JF - BMC Research Notes N2 - Objective Recently, we described a disintegrin and metalloproteinase 9 (ADAM9) overexpression by Schwann cells of vestibular schwannoma (VS) and suggested that it might be a marker for VS tumor growth and invasiveness. This research note provides additional data utilizing a small cohort of VS primary cultures and tissue samples. We examined whether reconstitution of Merlin expression in VS cells regulates ADAM9 protein expression and performed lentiviral ADAM9 knock down to investigate possible effects on VS cells numbers. Moreover, the co-localization of ADAM9 and Integrins α6 and α2β1, respectively, was examined by immunofluorescence double staining. Results ADAM9 expression was not regulated by Merlin in VS. However, ADAM9 knock down led to 58% reduction in cell numbers in VS primary cell cultures (p < 0.0001). While ADAM9 and Integrin α2β1 were co-localized in only 22% (2 of 9) of VS, ADAM9 and Integrin α6 were co-localized in 91% (10 of 11) of VS. Therefore, we provide first observations on possible regulatory functions of ADAM9 expression in VS. KW - vestibular schwannoma KW - pathogenesis KW - ADAM9 KW - knock down KW - integrin KW - immunofuorescence double staining KW - Merlin KW - primary cell culture Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-231213 VL - 13 ER - TY - JOUR A1 - Sbiera, Silviu A1 - Kunz, Meik A1 - Weigand, Isabel A1 - Deutschbein, Timo A1 - Dandekar, Thomas A1 - Fassnacht, Martin T1 - The new genetic landscape of Cushing’s disease: deubiquitinases in the spotlight JF - Cancers N2 - Cushing’s disease (CD) is a rare condition caused by adrenocorticotropic hormone (ACTH)-producing adenomas of the pituitary, which lead to hypercortisolism that is associated with high morbidity and mortality. Treatment options in case of persistent or recurrent disease are limited, but new insights into the pathogenesis of CD are raising hope for new therapeutic avenues. Here, we have performed a meta-analysis of the available sequencing data in CD to create a comprehensive picture of CD’s genetics. Our analyses clearly indicate that somatic mutations in the deubiquitinases are the key drivers in CD, namely USP8 (36.5%) and USP48 (13.3%). While in USP48 only Met415 is affected by mutations, in USP8 there are 26 different mutations described. However, these different mutations are clustering in the same hotspot region (affecting in 94.5% of cases Ser718 and Pro720). In contrast, pathogenic variants classically associated with tumorigenesis in genes like TP53 and BRAF are also present in CD but with low incidence (12.5% and 7%). Importantly, several of these mutations might have therapeutic potential as there are drugs already investigated in preclinical and clinical setting for other diseases. Furthermore, network and pathway analyses of all somatic mutations in CD suggest a rather unified picture hinting towards converging oncogenic pathways. KW - Cushing’s disease KW - pathogenesis KW - somatic mutations KW - deubiquitinases Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-193194 SN - 2072-6694 VL - 11 IS - 11 ER - TY - JOUR A1 - Meyer zu Hörste, Gerd A1 - Cordes, Steffen A1 - Mausberg, Anne K. A1 - Zozulya, Alla L. A1 - Wessig, Carsten A1 - Sparwasser, Tim A1 - Mathys, Christian A1 - Wiendl, Heinz A1 - Hartung, Hans-Peter A1 - Kieseier, Bernd C. T1 - FoxP3+Regulatory T Cells Determine Disease Severity in Rodent Models of Inflammatory Neuropathies JF - PLOS ONE N2 - Inflammatory neuropathies represent disabling human autoimmune disorders with considerable disease variability. Animal models provide insights into defined aspects of their disease pathogenesis. Forkhead box P3 (FoxP3)+ regulatory T lymphocytes (Treg) are anti-inflammatory cells that maintain immune tolerance and counteract tissue damage in a variety of immune-mediated disorders. Dysfunction or a reduced frequency of Tregs have been associated with different human autoimmune disorders. We here analyzed the functional relevance of Tregs in determining disease manifestation and severity in murine models of autoimmune neuropathies. We took advantage of the DEREG mouse system allowing depletion of Treg with high specificity as well as anti-CD25 directed antibodies to deplete Tregs in mice in actively induced experimental autoimmune neuritis (EAN). Furthermore antibody-depletion was performed in an adoptive transfer model of chronic neuritis. Early Treg depletion increased clinical EAN severity both in active and adoptive transfer chronic neuritis. This was accompanied by increased proliferation of myelin specific T cells and histological signs of peripheral nerve inflammation. Late stage Treg depletion after initial disease manifestation however did not exacerbate inflammatory neuropathy symptoms further. We conclude that Tregs determine disease severity in experimental autoimmune neuropathies during the initial priming phase, but have no major disease modifying function after disease manifestation. Potential future therapeutic approaches targeting Tregs should thus be performed early in inflammatory neuropathies. KW - Guillain-Barre-Syndrome KW - regulatory cells KW - C57BL/6 mice KW - demyelinating polyradiculoneuropathy KW - cytokines KW - pathogenesis KW - polyneuropathy KW - enteropathy KW - peptide KW - experimental autoimmune neuritis Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-115239 VL - 9 IS - 10 ER - TY - THES A1 - Hochgräfe, Katja T1 - Cre-loxP based mouse models to study prionpathogenesis in the motor nervous system N2 - Prion diseases such as scrapie in sheep, bovine spongiform encephalopathy (BSE) in cattle or Creutzfeldt-Jakob disease (CJD) in humans are fatal neurodegenerative disorders characterized by brain lesions and the accumulation of a disease-associated protein, designated PrPSc. How prions proceed to damage neurons and whether all or only subsets of neurons have to be affected for the onset of the clinical disease is still elusive. The manifestation of clinical prion disease is characterized by motor dysfunctions, dementia and death. Furthermore loss of motor neurons (MN) in the spinal cord is a constant finding in different mouse models of prion disease, suggesting that MN are vulnerable cells for triggering the onset of clinical symptoms. To determine whether the protection of MN against prion induced dysfunctions is an approach for holding the disease at the sub-clinical level, we established a novel conditional model for Cre-mediated expression of a dominant-negative PrP mutant (PrPQ167R) in the cells of interest. Dominant-negative PrP mutants provide protection of prion induced dysfunctions by inhibiting prion replication. Transgenic mice were generated carrying a floxed LacZ marker gene followed by the coding sequence of PrPQ167R under control of the human ubiquitin C promoter. Two Cre strains have been used to direct PrPQ167R expression either to a subset of MN of the spinal cord (Hb9-Cre) or to various neuronal cell populations of the spinal cord and brain (NF-L-Cre). Transgenic mice were infected with mouse-adapted prions via different inoculation routes (intranerval, intracerebral and intraperitoneal) and monitored for effects on incubation time and pathology. Tg floxed LacZ-PrPQ167R/NF-L-Cre mice showed about 15% prolonged survival upon intraperitoneal low dose prion infection, whereas survival of Tg floxed LacZ-PrPQ167R/Hb9-Cre mice was comparable to control littermates. The results suggest that the protection of spinal MN prolongs the incubation period but is not sufficient to completely inhibit clinical prion disease. In a second approach, Cre was transferred into the hind limb muscles of transgenic mice via a double-stranded adeno-associated virus vector (dsAAV2-Cre). The goal of this strategy was to target a broader cell population and thus to enhance expression levels of protective PrPQ167R in the spinal cord of Tg floxed-LacZ-PrPQ167R mice. After intramuscular (i.m.) application of dsAAV2-Cre, exhibiting a physical titer of 5x1010 GP/ml, recombinant transgenic DNA was detected only in the muscle tissue, pointing out that functional Cre-recombinase was expressed at the side of virus application. However, dsAAV2-Cre did neither induce recombination of transgenic DNA in the spinal cord or brain nor expression of dominant-negative PrPQ167R. In conclusion the dsAAV2-Cre vectors system needs further improvement to achieve efficient transport from muscle tissue to the central nervous system (CNS). 105 7 SUMMARY The lymphoreticular system (LRS) is an early site of prion replication. In splenic tissue prion infectivity is associated with follicular dendritic cells (FDC) as well as with Band T-lymphocytes. However, it is still unknown if those cell types are able to replicate the infectious agent or if other PrP-expressing cell types are engaged. To investigate if neurons and in particular MN are involved, transgenic mice carrying one allele of floxed Prnp (lox2+=��) and either one allele of Hb9-Cre or NF-L-Cre were generated on a Prnp0=0 background. Therefore a conditional PrP knockout was established in a subset of MN of the spinal cord (Hb9-Cre) or in various neuronal populations of the spinal cord and brain (NF-L-Cre). Transgenic mice were inoculated with prions to study the accumulation of PrPSc and prion infectivity in spleen and spinal cord at an early time point after infection. The findings show that PrPSc accumulation in mice with MN-specific PrP depletion (lox2+=��/ Hb9-Cre) was comparable to control littermates, while pan-neuronal PrP deficient mice (lox2+=��/NF-L-Cre) were not able to accumulate PrPSc in splenic tissue until 50 days post inoculation. Moreover spleens of lox2+=��/NF-L-Cre mice exhibited a clearly reduced prion infectivity titer, suggesting that accumulation of prions in the spleen is dependent on PrP expression in the nervous tissue. N2 - Prionenerkrankungen, wie Scrapie beim Schaf, die bovine spongiforme Enzephalopathie (BSE) beim Rind oder die Creutzfeldt-Jakob-Krankheit (CJD) beim Menschen sind letale, neurodegenerative Erkrankungen des zentralen Nervensystems (ZNS). Typische Merkmale der Erkrankung sind neben Neuronenverlust die Akkumulation des mit der Krankheit assoziierten Proteins PrPSc im Gehirn infizierter Individuen. Wie die Akkumulation von Prionen zu Neurodegeneration führt und welche Regionen des ZNS für die klinische Erkrankung verantwortlich sind, ist bisher unbekannt. Charakteristische, klinische Symptome von Prionenkrankheiten sind motorische Störungen sowie Demenz in einem späten Stadium der Erkrankung. Außerdem ist der Verlust von Motoneuronen (MN) im Rückenmark ein konstanter Befund im Tiermodell, was eine Rolle des motorischen Nervensystems bei der Prionpathogenese vermuten lässt. In dieser Arbeit sollte daher untersucht werden, ob der Schutz von MN vor Prionen induzierten Dysfunktionen den Ausbruch der klinischen Erkrankung verzögern kann. Dazu wurde ein konditionales Mausmodell mit Cre-induzierbarer Expression einer dom- inant-negativen PrP-Mutante (PrPQ167R) hergestellt. Dominant-negative PrP Mutanten schützen vor Prionen induzierten Schädigungen, indem sie die Replikation von Prionen inhibieren. Das Transgen besteht aus dem humanen Ubiquitin C Promoter, einem „gefloxten” LacZ Markergen und der kodierenden Sequenz von PrPQ167R. Die Kreuzung von Tg floxed LacZ-PrPQ167R Mäusen mit der Hb9-Cre Linie bewirkt eine MNspezifische Expression von PrPQ167R im Rückenmark, während das Einkreuzen eines NF-L-Cre Allels die Expression von PrPQ167R in den meisten Neuronen des Rückenmarks sowie in verschiedenen motorischen Kerngebieten des Gehirns zur Folge hat. Transgenen Mäuse wurden auf verschiedenen Routen (intranerval, intrazerebral und intraperitoneal) mit Maus-adaptierten Prionen infiziert und der Effekt von PrPQ167R auf die Inkubationszeit und Pathologie der Tiere untersucht. Während Tg floxed LacZPrP Q167R/NF-L-Cre Mäuse eine um 15% verlängerte Inkubationszeit aufwiesen, war bei Tg floxed LacZ-PrPQ167R/Hb9-Cre Mäusen kein Überlebensvorteil zu beobachten. Somit verlängert der Schutz von MN des Rückenmarks zwar die Inkubationszeit, ist aber nicht ausreichend, um den klinischen Ausbruch der Erkrankung zu verhindern. Um eine größere Zellpopulation im Rückenmark von Tg floxed LacZ-PrPQ167R Mäusen und so eine stärkere Expression von PrPQ167R zu erreichen, wurde ein viraler Gentransfer von Cre-Rekombinase durchgeführt. Dazu wurden doppelsträngige, Creexprimierende Adeno-assoziierte Virus Vektoren (dsAAV2-Cre) bilateral in die Muskulatur der Hinterbeine von Tg floxed LacZ-PrPQ167R Mäusen injiziert. Die Applikation von dsAAV2-Cre, mit einem physikalischen Virus-Titer von 5x1010 GP/ml, führte ausschließlich im Muskelgewebe zur Expression von enzymatisch aktiver Cre-Rekombinase und folglich zur Rekombination der transgenen DNA. Im Rücken- 107 8 ZUSAMMENFASSUNG mark oder Gehirn war keine rekombinante DNA detektierbar. Auch auf Protein-Ebene konnte die Expression von PrPQ167R weder im Muskel noch im Rückenmark oder Gehirn nachgewiesen werden. Um den Transport von dsAAV2-Cre vom Applikationsort bis in das ZNS zu gewährleisten und Cre stabil zu exprimieren, ist demnach eine weitere Optimierung des dsAAV2-Cre Vektorsystems notwendig. Prionen replizieren im lymphoretikulären System (LRS) bereits in einem frühen Stadium der Erkrankung. In der Milz ist Prionen-Infektiosität in follikulär dendritischen Zellen (FDC) sowie in B- und T-Lymphozyten lokalisiert. Ob noch andere PrP exprimierende Zellen an der Prionen-Replikation im LRS beteiligt sind, ist unklar. Um die Beteiligung von Neuronen und MN an der Akkumulation von Prionen im LRS zu untersuchen, wurden transgene, neuronal PrP defiziente Mäuse generiert. Ein Neuronen-spezifischer bzw. MN-spezifischer Knockout von PrP wurde durch Kreuzung von transgenen lox2+=�� Mäusen, welche ein „gefloxtes“ Prnp Allel Prnp auf einem Prnp0=0 Hintergrund tragen, mit NF-L-Cre oder Hb9-Cre Mäusen erreicht. Nach Prionen-Infektion von lox2+=��/NF-L-Cre und lox2+=��/Hb9-Cre Mäusen wurde die Akkumulation von PrPSc und Prionen-Infektiosität in der Milz und im Rückenmark am Tag 50 nach der Infektion analysiert. Während die Replikation von PrPSc in der Milz von Mäusen mit MN-spezifischem PrP Knockout (lox2+=��/Hb9-Cre) nicht beeinträchtigt war, war in pan-neuronal PrP defizienten Mäusen (lox2+=��/NF-L-Cre) keine Akkumulation von PrPSc nachweisbar. Zudem war die Prionen-Infektiosität in der Milz von lox2+=��/NF-L-Cre Mäusen deutlich reduziert. Die Ergebnisse weisen darauf hin, dass die Akkumulation von PrPSc und Prionen-Infektiosität in der Milz abhängig von neuronaler PrP Expression ist. KW - Prionkrankheit KW - Pathogenese KW - Maus KW - Motoneuron KW - Prion KW - pathogenesis Y1 - 2009 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-45967 ER -