@phdthesis{Sauer2011, author = {Sauer, Florian}, title = {Structural studies on the association of filamentous proteins in the human M-Bands}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-72410}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2011}, abstract = {Cross-striated muscles enable higher animals to perform directed movements and to create mechanical force. The cells of heart and skeletal muscles consist of myofibrils, serial arrays of the smallest contractile subunits, the sarcomeres. Main components of the sarcomeres are the thin and thick filaments, large protein assemblies consisting of mainly actin (thin filaments) and myosin (thick filaments), whose energy-dependent interaction is responsible for the contraction of sarcomeres and so of the whole muscle. The thin filaments are anchored in the sarcomere bordering Z-discs, while the thick filaments are anchored in the M-bands, traverse structures in the sarcomere center. Electron-microscopic studies revealed that the M-bands consist of regular, lattice-like structures that appear to cross-link the thick filaments. A number of proteins could be identified by immune-fluorescence and biochemical binding studies to be present and interact with each other in the M-bands. These data have been integrated into preliminary models of the M-bands. Detailed knowledge of how these proteins interact with each other in the center of the sarcomeres is, however, largely missing. The current study focuses on the structural characterization of the interactions between the titin, myomesin-1, obscurin and obscurin-like 1 (OBSL1), modular filamentous proteins interacting with each other in the M-bands. The high-resolution crystal structure of the titin M10 - OBSL1 Ig1 complex was solved. The structure and additional biophysical data show that titin and OBSL1 as well as titin and obscurin form stable binary complexes through the formation of a small intermolecular ß-sheet. In contrast to previously characterized intermolecular assemblies of sarcomeric proteins, this sheet is formed between parallel non- homologous ß-strands of the interaction partners. The investigation of disease-related variants of the M10 domain by biophysical methods did not allow to draw unambiguous conclusions on a direct connection between impaired OBSL1/obscurin binding and disease development. Two out of four known M10 variants have effects on the correct domain folding and so interfere with the ability to bind obscurin/OBSL1. The two other known variants displayed however only minor effects on fold and binding affinities. It should therefore be further elucidated whether a direct connection between impaired complex formation and disease development exists. -I- Abstract A direct interaction between titin and myomesin-1 could not be confirmed in vitro. Possible explanations for the different results are discussed. While the consequences of the inability of both proteins to interact are unclear, the further characterization of the putative interacting parts of titin and myomesin-1 led to the discovery of two new potential sites of self-assembly on M-band titin and myomesin-1. The crystal structure of titin M4 showed that this domain can form dimeric assemblies through the formation of a disulfide bridge and an intermolecular metal binding site between residues that are unique to this domain. On myomesin-1, in addition to the described C-terminal interaction site, a potential second site of self-assembly was found in its central Fn3-domain segment. The interacting site was mapped to the predicted Fn3 domain My5. The crystal structure of the domain in its dimeric form showed that the interaction is mediated by a mechanism that has previously not been observed in sarcomeric proteins. Two My5 interact with each other by the mutual exchange of an N-terminal ß-strand which complements the Fn3 fold on the binding partner. This type of interaction can be interpreted as misfolding. However, the position of the interacting domain and its mode of interaction allowed the postulation of a model of how myomesin-1 could be integrated in the M-bands. This model is in good agreement with the electron-microscopic appearance of the M-bands.}, subject = {Muskelkontraktion}, language = {en} } @phdthesis{Joseph2011, author = {Joseph, Julie}, title = {Studying the role of Th17 cells in autoimmune diabetes and generation of a beta cell reporter mouse by lentiviral transgenesis}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-66571}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2011}, abstract = {Type 1 diabetes affects around 0.5\% of the population in developed countries and the incidence rates have been rising over the years. The destruction of beta cells is irreversible and the current therapy available to patients only manages the symptoms and does not prevent the associated pathological manifestations. The patients need lifelong therapy and intensive research is being carried out to identify ways to eliminate autoimmune responses directed against pancreatic beta cells and to replace or regenerate beta cells. The work presented herein aimed at analyzing the role of the Th17 T cell subset, characterized by secretion of the pro- inflammatory cytokine IL-17A, in autoimmune diabetes and also at generating a beta cell reporter mouse line in the NOD background, the most widely- used mouse model for type 1 diabetes. We generated IL- 17A knockdown (KD) NOD mice, using RNAi in combination with lentiviral transgenesis. We analyzed diabetes frequency in IL-17A deficient mice and found that the loss of IL-17A did not protect the transgenic mice from diabetes. Based on these observations, we believe that Th17 cells do not play a critical role in type 1 diabetes through the IL-17A pathway, though they might still be involved in the disease process through alternate pathways. We also generated NOD and NOD-SCID mice with a transgene that drives the beta cell specific expression of a luciferase reporter gene. We used a lentiviral construct, which combined a luciferase sequence and a short- hairpin RNA (shRNA) expression cassette, allowing gene- knockdown under the beta cell specific rat insulin promoter (RIP). These mice will be of use in studying beta cell phenotypes resulting from the knockdown of target genes, using non- invasive bioimaging. We believe that the generation of these reporter mouse lines for diabetes studies will prove valuable in future investigations. Furthermore, the demonstration that the loss of IL-17A does not alter susceptibility to type 1 diabetes should help clarify the controversial involvement of Th17 cells in this disease.}, subject = {Diabetes mellitus}, language = {en} } @article{PhamHelluyKleinschnitzetal.2011, author = {Pham, Mirko and Helluy, Xavier and Kleinschnitz, Christoph and Kraft, Peter and Bartsch, Andreas J. and Jakob, Peter and Nieswandt, Bernhard and Bendszus, Martin and Guido, Stoll}, title = {Sustained Reperfusion after Blockade of Glycoprotein-Receptor-Ib in Focal Cerebral Ischemia: An MRI Study at 17.6 Tesla}, series = {PLoS ONE}, volume = {6}, journal = {PLoS ONE}, number = {4}, doi = {10.1371/journal.pone.0018386}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-142608}, pages = {e18386}, year = {2011}, abstract = {Background: Inhibition of early platelet adhesion by blockade of glycoprotein-IB (GPIb) protects mice from ischemic stroke. To elucidate underlying mechanisms in-vivo, infarct development was followed by ultra-high field MRI at 17.6 Tesla. Methods: Cerebral infarction was induced by transient-middle-cerebral-artery-occlusion (tMCAO) for 1 hour in C57/BL6 control mice (N = 10) and mice treated with 100 mg Fab-fragments of the GPIb blocking antibody p0p/B 1 h after tMCAO (N = 10). To control for the effect of reperfusion, additional mice underwent permanent occlusion and received anti-GPIb treatment (N = 6; pMCAO) or remained without treatment (N = 3; pMCAO). MRI 2 h and 24 h after MCAO measured cerebral-blood-flow (CBF) by continuous arterial-spin labelling, the apparent-diffusion-coefficient (ADC), quantitative-T2 and T2-weighted imaging. All images were registered to a standard mouse brain MRI atlas and statistically analysed voxel-wise, and by cortico-subcortical ROI analysis. Results: Anti-GPIb treatment led to a relative increase of postischemic CBF vs. controls in the cortical territory of the MCA (2 h: 44.2 +/- 6.9 ml/100g/min versus 24 h: 60.5 +/- 8.4; p = 0.0012, F((1,18)) = 14.63) after tMCAO. Subcortical CBF 2 h after tMCAO was higher in anti-GPIb treated animals (45.3 +/- 5.9 vs. controls: 33.6 +/- 4.3; p = 0.04). In both regions, CBF findings were clearly related to a lower probability of infarction (Cortex/Subcortex of treated group: 35\%/65\% vs. controls: 95\%/100\%) and improved quantitative-T2 and ADC. After pMCAO, anti-GPIb treated mice developed similar infarcts preceded by severe irreversible hypoperfusion as controls after tMCAO indicating dependency of stroke protection on reperfusion. Conclusion: Blockade of platelet adhesion by anti-GPIb-Fab-fragments results in substantially improved CBF early during reperfusion. This finding was in exact spatial correspondence with the prevention of cerebral infarction and indicates in-vivo an increased patency of the microcirculation. Thus, progression of infarction during early ischemia and reperfusion can be mitigated by anti-platelet treatment.}, language = {en} } @article{WaldholmWangBrodinetal.2011, author = {Waldholm, Johan and Wang, Zhi and Brodin, David and Tyagi, Anu and Yu, Simei and Theopold, Ulrich and {\"O}stlund Farrants, Ann Kristin and Visa, Neus}, title = {SWI/SNF regulates the alternative processing of a specific subset of pre-mRNAs in \(Drosophila\) \(melanogaster\)}, series = {BMC Molecular Biology}, volume = {12}, journal = {BMC Molecular Biology}, number = {46}, doi = {10.1186/1471-2199-12-46}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-142613}, pages = {1-12}, year = {2011}, abstract = {Background: The SWI/SNF chromatin remodeling factors have the ability to remodel nucleosomes and play essential roles in key developmental processes. SWI/SNF complexes contain one subunit with ATPase activity, which in Drosophila melanogaster is called Brahma (Brm). The regulatory activities of SWI/SNF have been attributed to its influence on chromatin structure and transcription regulation, but recent observations have revealed that the levels of Brm affect the relative abundances of transcripts that are formed by alternative splicing and/or polyadenylation of the same pre-mRNA. Results: We have investigated whether the function of Brm in pre-mRNA processing in Drosophila melanogaster is mediated by Brm alone or by the SWI/SNF complex. We have analyzed the effects of depleting individual SWI/SNF subunits on pre-mRNA processing throughout the genome, and we have identified a subset of transcripts that are affected by depletion of the SWI/SNF core subunits Brm, Snr1 or Mor. The fact that depletion of different subunits targets a subset of common transcripts suggests that the SWI/SNF complex is responsible for the effects observed on pre-mRNA processing when knocking down Brm. We have also depleted Brm in larvae and we have shown that the levels of SWI/SNF affect the pre-mRNA processing outcome in vivo. Conclusions: We have shown that SWI/SNF can modulate alternative pre-mRNA processing, not only in cultured cells but also in vivo. The effect is restricted to and specific for a subset of transcripts. Our results provide novel insights into the mechanisms by which SWI/SNF regulates transcript diversity and proteomic diversity in higher eukaryotes.}, language = {en} } @phdthesis{Subota2011, author = {Subota, Ines}, title = {Switches in trypanosome differentiation: ALBA proteins acting on post-transcriptional mRNA control}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-85707}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2011}, abstract = {Trypanosoma brucei is a digenetic eukaryotic parasite that develops in different tissues of a mammalian host and a tsetse fly. It is responsible for sleeping sickness in sub-saharan Africa. The parasite cycle involves more than nine developmental stages that can be clearly distinguished by their general morphology, their metabolism and the relative positioning of their DNA-containing organelles. During their development, trypanosomes remain exclusively extracellular and encounter changing environments with different physico-chemical properties (nutritional availability, viscosity, temperature, etc.). It has been proposed that trypanosomes use their flagellum as a sensing organelle, in agreement with the established role of structurally-related cilia in metazoa and ciliates. Recognition of environmental triggers is presumed to be at the initiation of differentiation events, leading to the parasite stage that is the best suited to the new environment. These changes are achieved by the modification of gene expression programmes, mostly underlying post-transcriptional control of mRNA transcripts. We first demonstrate that the RNA-binding proteins ALBA3/4 are involved in specific differentiation processes during the parasite development in the fly. They are cytosolic and expressed throughout the parasite cycle with the exception of the stages found in the tsetse fly proventriculus, as shown by both immunofluorescence and live cell analysis upon endogenous tagging with YFP. Knock-down of both proteins in the developmental stage preceding these forms leads to striking modifications: cell elongation, cell cycle arrest and relocalization of the nucleus in a posterior position, all typical of processes acting in parasites found in the proventriculus region. When ALBA3 is over-expressed from an exogenous copy during infection, it interferes with the relocalization of the nucleus in proventricular parasites. This is not observed for ALBA4 over-expression that does not visibly impede differentiation. Both ALBA3/4 proteins react to starvation conditions by accumulating in cytoplasmic stress granules together with DHH1, a recognized RNA-binding protein. ALBA3/4 proteins also partially colocalize with granules formed by polyA+ RNA in these conditions. We propose that ALBA are involved in trypanosome differentiation processes where they control a subset of developmentally regulated transcripts. These processes involving ALBA3/4 are likely to result from the specific activation of sensing pathways. In the second part of the thesis, we identify novel flagellar proteins that could act in sensing mechanisms. Several protein candidates were selected from a proteomic analysis of intact flagella performed in the host laboratory. This work validates their flagellar localization with high success (85\% of the proteins examined) and defines multiple different patterns of protein distribution in the flagellum. Two proteins are analyzed during development, one of them showing down-regulation in proventricular stages. The functional analysis of one novel flagellar membrane protein reveals its rapid dynamics within the flagellum but does not yield a visible phenotype in culture. This is coherent with sensory function that might not be needed in stable culture conditions, but could be required in natural conditions during development. In conclusion, this work adds new pieces to the puzzle of identifying molecular switches involved in developmental mRNA control and environmental sensing in trypanosome stages in the tsetse fly.}, subject = {Trypanosoma brucei}, language = {en} } @phdthesis{Stieb2011, author = {Stieb, Sara Mae}, title = {Synaptic plasticity in visual and olfactory brain centers of the desert ant Cataglyphis}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-85584}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2011}, abstract = {W{\"u}stenameisen der Gattung Cataglyphis wurden zu Modellsystemen bei der Erforschung der Navigationsmechanismen der Insekten. Ein altersabh{\"a}ngiger Polyethismus trennt deren Kolonien in Innendienst-Arbeiterinnen und kurzlebige lichtausgesetzte Fourageure. Nachdem die Ameisen in strukturlosem oder strukturiertem Gel{\"a}nde bis zu mehrere hundert Meter weite Distanzen zur{\"u}ckgelegt haben, k{\"o}nnen sie pr{\"a}zise zu ihrer oft unauff{\"a}lligen Nest{\"o}ffnung zur{\"u}ckzukehren. Um diese enorme Navigationsleistung zu vollbringen, bedienen sich die Ameisen der sogenannten Pfadintegration, welche die Informationen aus einem Polarisationskompass und einem Entfernungsmesser verrechnet; des Weiteren orientieren sie sich an Landmarken und nutzen olfaktorische Signale. Im Fokus dieser Arbeit steht C. fortis, welche in Salzpfannen des westlichen Nordafrikas endemisch ist - einem Gebiet, welches vollst{\"a}ndig von anderen Cataglyphis Arten gemieden wird. Die Tatsache, dass Cataglyphis eine hohe Verhaltensflexibilit{\"a}t aufweist, welche mit sich drastisch {\"a}ndernden sensorischen Anforderungen verbunden ist, macht diese Ameisen zu besonders interessanten Studienobjekten bei der Erforschung synaptischer Plastizit{\"a}t visueller und olfaktorischer Gehirnzentren. Diese Arbeit fokussiert auf plastische {\"A}nderungen in den Pilzk{\"o}rpern (PK) - sensorischen Integrationszentren, die mutmaßlich an Lern- und Erinnerungsprozessen, und auch vermutlich am Prozess des Landmarkenlernens beteiligt sind - und auf plastische {\"A}nderungen in den synaptischen Komplexen des Lateralen Akzessorischen Lobus (LAL) - einer bekannten Relaisstation in der Polarisations-Leitungsbahn. Um die strukturelle synaptische Plastizit{\"a}t der PK in C. fortis zu quantifizieren, wurden mithilfe immunozytochemischer F{\"a}rbungen die pr{\"a}- und postsynaptischen Profile klar ausgepr{\"a}gter synaptischer Komplexe (Mikroglomeruli, MG) der visuellen Region (Kragen) und der olfaktorischen Region (Lippe) der PK-Kelche visualisiert. Die Ergebnisse legen dar, dass eine Volumenzunahme der PK-Kelche w{\"a}hrend des {\"U}bergangs von Innendiensttieren zu Fourageuren von einer Abnahme der MG-Anzahl im Kragen und, mit einem geringeren Anteil, in der Lippe - dieser Effekt wird als Pruning bezeichnet - und einem gleichzeitigen Auswachsen an Dendriten PK-intrinsischer Kenyonzellen begleitet wird. Im Dunkeln gehaltene Tiere unterschiedlichen Alters zeigen nach Lichtaussetzung den gleichen Effekt und im Dunkel gehaltene, den Fourageuren altersm{\"a}ßig angepasste Tiere weisen eine vergleichbare MG-Anzahl im Kragen auf wie Innendiensttiere. Diese Ergebnisse deuten darauf hin, dass die immense strukturelle synaptische Plastizit{\"a}t in der Kragenregion der PK-Kelche haupts{\"a}chlich durch visuelle Erfahrungen ausgel{\"o}st wird und nicht ausschließlich mit Hilfe eines internen Programms abgespielt wird. Ameisen, welche unter Laborbedingungen bis zu einem Jahr alt wurden, zeigen eine vergleichbare Plastizit{\"a}t. Dies deutet darauf hin, dass das System {\"u}ber die ganze Lebensspanne eines Individuums flexibel bleibt. Erfahrene Fourageure wurden in Dunkelheit zur{\"u}ckgef{\"u}hrt, um zu untersuchen, ob die lichtausgel{\"o}ste synaptische Umstrukturierung reversibel ist, doch ihre PK zeigen nur einige die Zur{\"u}ckf{\"u}hrung widerspiegelnde Plastizit{\"a}tsauspr{\"a}gungen, besonders eine {\"A}nderung der pr{\"a}synaptischen Synapsinexprimierung. Mithilfe immunozytochemischer F{\"a}rbungen, konfokaler Mikroskopie und 3D-Rekonstruktionen wurden die pr{\"a}- und postsynaptischen Strukturen synaptischer Komplexe des LAL in C. fortis analysiert und potentielle strukturelle {\"A}nderungen bei Innendiensttieren und Fourageuren quantifiziert. Die Ergebnisse zeigen, dass diese Komplexe aus postsynaptischen, in einer zentralen Region angeordneten Forts{\"a}tzen bestehen, welche umringt sind von einem pr{\"a}synaptischen kelchartigen Profil. Eingehende und ausgehende Trakte wurden durch Farbstoffinjektionen identifiziert: Projektionsneurone des Anterioren Optischen Tuberkels kontaktieren Neurone, welche in den Zentralkomplex ziehen. Der Verhaltens{\"u}bergang wird von einer Zunahme an synaptischen Komplexen um ~13\% begleitet. Dieser Zuwachs suggeriert eine Art Kalibrierungsprozess in diesen potentiell kr{\"a}ftigen synaptischen Kontakten, welche vermutlich eine schnelle und belastbare Signal{\"u}bertragung in der Polarisationsbahn liefern. Die Analyse von im Freiland aufgenommener Verhaltenweisen von C. fortis enth{\"u}llen, dass die Ameisen, bevor sie mit ihrer Fouragiert{\"a}tigkeit anfangen, bis zu zwei Tage lang in unmittelbarer N{\"a}he des Nestes Entdeckungsl{\"a}ufe unternehmen, welche Pirouetten {\"a}hnliche Drehungen beinhalten. W{\"a}hrend dieser Entdeckungsl{\"a}ufe sammeln die Ameisen Lichterfahrung und assoziieren m{\"o}glicherweise den Nesteingang mit spezifischen Landmarken oder werden anderen visuellen Informationen, wie denen des Polarisationsmusters, ausgesetzt und adaptieren begleitend ihre neuronalen Netzwerke an die bevorstehende Herausforderung. Dar{\"u}ber hinaus k{\"o}nnten die Pirouetten einer Stimulation der an der Polarisationsbahn beteiligten neuronalen Netzwerke dienen. Videoanalysen legen dar, dass Lichtaussetzung nach drei Tagen die Bewegungsaktivit{\"a}t der Ameisen heraufsetzt. Die Tatsache, dass die neuronale Umstrukturierung in visuellen Zentren wie auch die Ver{\"a}nderungen im Verhalten im selben Zeitrahmen ablaufen, deutet darauf hin, dass ein Zusammenhang zwischen struktureller synaptischer Plastizit{\"a}t und dem Verhaltens{\"u}bergang von der Innendienst- zur Fouragierphase bestehen k{\"o}nnte. Cataglyphis besitzen hervorragende visuelle Navigationsf{\"a}higkeiten, doch sie nutzen zudem olfaktorische Signale, um das Nest oder die Futterquelle aufzusp{\"u}ren. Mithilfe konfokaler Mikroskopie und 3D-Rekonstruktionen wurden potentielle Anpassungen der prim{\"a}ren olfaktorischen Gehirnzentren untersucht, indem die Anzahl, Gr{\"o}ße und r{\"a}umliche Anordnung olfaktorischer Glomeruli im Antennallobus von C. fortis, C. albicans, C. bicolor, C. rubra, und C. noda verglichen wurde. Arbeiterinnen aller Cataglyphis-Arten haben eine geringere Glomeruli-Anzahl im Vergleich zu denen der mehr olfaktorisch-orientierten Formica Arten - einer Gattung nah verwandt mit Cataglyphis - und denen schon bekannter olfaktorisch-orientierter Ameisenarten. C. fortis hat die geringste Anzahl an Glomeruli im Vergleich zu allen anderen Cataglyphis-Arten und besitzt einen vergr{\"o}ßerten Glomerulus, der nahe dem Eingang des Antennennerves lokalisiert ist. C. fortis M{\"a}nnchen besitzen eine signifikant geringere Glomeruli-Anzahl im Vergleich zu Arbeiterinnen und K{\"o}niginnen und haben einen hervorstechenden M{\"a}nnchen-spezifischen Makroglomerulus, welcher wahrscheinlich an der Pheromon-Kommunikation beteiligt ist. Die Verhaltensrelevanz des vergr{\"o}ßerten Glomerulus der Arbeiterinnen bleibt schwer fassbar. Die Tatsache, dass C. fortis Mikrohabitate bewohnt, welche von allen anderen Cataglyphis Arten gemieden werden, legt nahe, dass extreme {\"o}kologische Bedingungen nicht nur zu Anpassungen der visuellen F{\"a}higkeiten, sondern auch des olfaktorischen Systems gef{\"u}hrt haben. Die vorliegende Arbeit veranschaulicht, dass Cataglyphis ein exzellenter Kandidat ist bei der Erforschung neuronaler Mechanismen, welche Navigationsfunktionalit{\"a}ten zugrundeliegen, und bei der Erforschung neuronaler Plastizit{\"a}t, welche verkn{\"u}pft ist mit der lebenslangen Flexibilit{\"a}t eines individuellen Verhaltensrepertoires.}, subject = {Neuroethologie}, language = {en} } @article{UeceylerHaeuserSommer2011, author = {{\"U}ceyler, Nurcan and H{\"a}user, Winfried and Sommer, Claudia}, title = {Systematic review with meta-analysis: Cytokines in fibromyalgia syndrome}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-69189}, year = {2011}, abstract = {Background: To perform a systematic review and meta-analysis on cytokine levels in patients with fibromyalgia syndrome (FMS). Methods: Through December 2010 we systematically reviewed the databases PubMed, MEDLINE, and PsycINFO and screened the reference lists of 22 review articles for suitable original articles. Original articles investigating cytokines in patients with FMS were included. Data were extracted by two independent authors. Differences of the cytokine levels of FMS patients and controls were summarized by standardized mean differences (SMD) using a random effects model. Study quality was assessed applying methodological scores: modified Center of Evidence Based Medicine, Newcastle-Ottawa-Scale, and W{\"u}rzburg Methodological Quality Score. Results: Twenty-five articles were included investigating 1255 FMS patients and 800 healthy controls. Data of 13/25 studies entered meta-analysis. The overall methodological quality of studies was low. The results of the majority of studies were not comparable because methods, investigated material, and investigated target cytokines differed. Systematic review of the selected 25 articles revealed that FMS patients had higher serum levels of interleukin (IL)-1 receptor antagonist, IL-6, and IL-8, and higher plasma levels of IL-8. Meta-analysis of eligible studies showed that FMS patients had higher plasma IL-6 levels compared to controls (SMD = -0.34 [-0.64, -0.03] 95\% CI; p = 0.03). The majority of investigated cytokines were not different between patients and controls. Conclusions: The pathophysiological role of cytokines in FMS is still unclear. Studies of higher quality and with higher numbers of subjects are needed.}, subject = {Fibromyalgie}, language = {en} } @article{ThormannRaupachWagneretal.2011, author = {Thormann, Birthe and Raupach, Michael J. and Wagner, Thomas and W{\"a}gele, Johann W. and Peters, Marcell K.}, title = {Testing a Short Nuclear Marker for Inferring Staphylinid Beetle Diversity in an African Tropical Rain Forest}, series = {PLoS ONE}, volume = {6}, journal = {PLoS ONE}, number = {3}, doi = {10.1371/journal.pone.0018101}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-142666}, pages = {e18101}, year = {2011}, abstract = {Background: The use of DNA based methods for assessing biodiversity has become increasingly common during the last years. Especially in speciose biomes as tropical rain forests and/or in hyperdiverse or understudied taxa they may efficiently complement morphological approaches. The most successful molecular approach in this field is DNA barcoding based on cytochrome c oxidase I (COI) marker, but other markers are used as well. Whereas most studies aim at identifying or describing species, there are only few attempts to use DNA markers for inventorying all animal species found in environmental samples to describe variations of biodiversity patterns. Methodology/Principal Findings: In this study, an analysis of the nuclear D3 region of the 28S rRNA gene to delimit species-like units is compared to results based on distinction of morphospecies. Data derived from both approaches are used to assess diversity and composition of staphylinid beetle communities of a Guineo-Congolian rain forest in Kenya. Beetles were collected with a standardized sampling design across six transects in primary and secondary forests using pitfall traps. Sequences could be obtained of 99\% of all individuals. In total, 76 molecular operational taxonomic units (MOTUs) were found in contrast to 70 discernible morphospecies. Despite this difference both approaches revealed highly similar biodiversity patterns, with species richness being equal in primary and secondary forests, but with divergent species communities in different habitats. The D3-MOTU approach proved to be an efficient tool for biodiversity analyses. Conclusions/Significance: Our data illustrate that the use of MOTUs as a proxy for species can provide an alternative to morphospecies identification for the analysis of changes in community structure of hyperdiverse insect taxa. The efficient amplification of the D3-marker and the ability of the D3-MOTUs to reveal similar biodiversity patterns as analyses of morphospecies recommend its use in future molecular studies on biodiversity.}, language = {en} } @article{HendriksmaHaertelSteffanDewenter2011, author = {Hendriksma, Harmen P. and H{\"a}rtel, Stephan and Steffan-Dewenter, Ingolf}, title = {Testing Pollen of Single and Stacked Insect-Resistant Bt-Maize on In vitro Reared Honey Bee Larvae}, series = {PLoS One}, volume = {6}, journal = {PLoS One}, number = {12}, doi = {10.1371/journal.pone.0028174}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-137803}, pages = {e28174}, year = {2011}, abstract = {The ecologically and economic important honey bee (Apis mellifera) is a key non-target arthropod species in environmental risk assessment (ERA) of genetically modified (GM) crops. Honey bee larvae are directly exposed to transgenic products by the consumption of GM pollen. But most ERA studies only consider responses of adult bees, although Bt-proteins primarily affect the larval phases of target organisms. We adopted an in vitro larvae rearing system, to assess lethal and sublethal effects of Bt-pollen consumption in a standardized eco-toxicological bioassay. The effects of pollen from two Bt-maize cultivars, one expressing a single and the other a total of three Bt-proteins, on the survival and prepupae weight of honey bee larvae were analyzed. The control treatments included pollen from three non-transgenic maize varieties and of Heliconia rostrata. Three days old larvae were fed the realistic exposure dose of 2 mg pollen within the semi-artificial diet. The larvae were monitored over 120 h, until the prepupal stage, where larvae terminate feeding and growing. Neither single nor stacked Bt-maize pollen showed an adverse effect on larval survival and the prepupal weight. In contrast, feeding of H. rostrata pollen caused significant toxic effects. The results of this study indicate that pollen of the tested Bt-varieties does not harm the development of in vitro reared A. mellifera larvae. To sustain the ecosystem service of pollination, Bt-impact on A. mellifera should always be a crucial part of regulatory biosafety assessments. We suggest that our approach of feeding GM pollen on in vitro reared honey bee larvae is well suited of becoming a standard bioassay in regulatory risk assessments schemes of GM crops.}, language = {en} } @article{WobserGaiglTrautmann2011, author = {Wobser, Marion and Gaigl, Zeno and Trautmann, Axel}, title = {The concept of "compartment allergy": prilocaine injected into different skin layers}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-68679}, year = {2011}, abstract = {We herein present a patient with delayed-type allergic hypersensitivity against prilocaine leading to spreading eczematous dermatitis after subcutaneous injections for local anesthesia with prilocaine. Prilocaine allergy was proven by positive skin testing and subcutaneous provocation, whereas the evaluation of other local anesthetics - among them lidocaine, articaine and mepivacaine - did not exhibit any evidence for cross-reactivity. Interestingly, our patient repeatedly tolerated strictly deep subcutaneous injection of prilocaine in provocation testing while patch and superficial subcutaneous application mounted strong allergic responses. We hypothesize, that lower DC density in deeper cutaneous compartments and/or different DC subsets exhibiting distinct functional immunomodulatory properties in the various layers of the skin may confer to the observed absence of clinical reactivity against prilocaine after deep subcutaneous injection. The term compartment allergy indicates that the route of allergen administration together with the targeted immunologic environment orchestrates on the immunologic outcome: overt T-cell mediated allergy or clinical tolerance.}, subject = {Medizin}, language = {en} }