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αB-crystallin is a sensor for assembly intermediates and for the subunit topology of desmin intermediate filaments

机译:αB-crystallin是用于装配中间体和结蛋白中间体细丝亚基拓扑的传感器

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Mutations in the small heat shock protein chaperone CRYAB (αB-crystallin/HSPB5) and the intermediate filament protein desmin, phenocopy each other causing cardiomyopathies. Whilst the binding sites for desmin on CRYAB have been determined, desmin epitopes responsible for CRYAB binding and also the parameters that determine CRYAB binding to desmin filaments are unknown. Using a combination of co-sedimentation centrifugation, viscometric assays and electron microscopy of negatively stained filaments to analyse the in vitro assembly of desmin filaments, we show that the binding of CRYAB to desmin is subject to its assembly status, to the subunit organization within filaments formed and to the integrity of the C-terminal tail domain of desmin. Our in vitro studies using a rapid assembly protocol, C-terminally truncated desmin and two disease-causing mutants (I451M and R454W) suggest that CRYAB is a sensor for the surface topology of the desmin filament. Our data also suggest that CRYAB performs an assembly chaperone role because the assembling filaments have different CRYAB-binding properties during the maturation process. We suggest that the capability of CRYAB to distinguish between filaments with different surface topologies due either to mutation (R454W) or assembly protocol is important to understanding the pathomechanism(s) of desmin-CRYAB myopathies.
机译:小分子热激蛋白伴侣蛋白CRYAB(αB-crystallin/ HSPB5)和中间丝蛋白desmin的突变,在表型上互相突变,引起心肌病。虽然已经确定了结蛋白在CRYAB上的结合位点,但负责结蛋白CRYAB结合的结蛋白表位以及确定CRYAB与结蛋白细丝结合的参数是未知的。使用共沉淀离心,粘度测定法和电镜观察阴性染色的细丝的组合来分析结蛋白细丝的体外组装,我们表明CRYAB与结蛋白的结合受制于其组装状态以及细丝中亚基的组织形成结蛋白并达到结蛋白C末端尾域的完整性。我们使用快速组装方案,C末端截短的结蛋白和两个致病突变体(I451M和R454W)进行的体外研究表明CRYAB是结蛋白细丝表面拓扑的传感器。我们的数据还表明CRYAB发挥了组装伴侣的作用,因为在成熟过程中,组装的长丝具有不同的CRYAB结合特性。我们建议,CRYAB能够区分由于突变(R454W)或装配规程而具有不同表面拓扑的细丝的能力,对于了解desmin-CRYAB肌病的发病机理非常重要。

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