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Analyzing folding and degradation of metabolically labelled polypeptides by conventional and diagonal sodium dodecyl sulfate-polyacrylamide gel electrophoresis

机译:通过常规和对角十二烷基硫酸钠-聚丙烯酰胺凝胶电泳分析代谢标记多肽的折叠和降解

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Efficient protein folding and quality control are essential for unperturbed cell viability. Defects in these processes may lead to production of aberrant polypeptides that are either degraded leading to “loss-of-function” phenotypes, or deposited in or outside cells leading to “gain-of-toxic-function” phenotypes. Elucidation of molecular mechanisms regulating folding and quality control of newly synthesized polypeptides is therefore of greatest interest. Here we describe protocols for metabolic labelling of transfected/infected mammalian cells with [35S]-methionine and [35S]-cysteine, for immunoisolation from detergent extracts of the selected model proteins and for the investigation of the model polypeptide’s intracellular fate in response to chaperone-deletions or to cell exposure to folding or degradation inhibitors.
机译:有效的蛋白质折叠和质量控制对于稳定的细胞活力至关重要。这些过程中的缺陷可能导致产生异常的多肽,这些多肽要么被降解导致“功能丧失”表型,要么沉积在细胞内或细胞外而导致“毒性功能获得”表型。因此,阐明调节新合成多肽的折叠和质量控制的分子机制是最受关注的。在这里,我们描述了使用[ 35 S]-蛋氨酸和[ 35 S]-半胱氨酸对转染/感染的哺乳动物细胞进行代谢标记的方案,用于从选定的洗涤剂提取物中进行免疫分离模型蛋白,以及用于研究模型多肽在伴侣分子缺失或细胞暴露于折叠或降解抑制剂后的细胞内命运。

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