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Hsp40 对鉴定细胞毒性暴露所导致的不稳定蛋白的亲和力。

Hsp40 Affinity to Identify Proteins Destabilized by Cellular Toxicant Exposure.

机构信息

Department of Chemistry, University of California, Riverside, Riverside, California 92521, United States.

出版信息

Anal Chem. 2021 Dec 21;93(50):16940-16946. doi: 10.1021/acs.analchem.1c04230. Epub 2021 Dec 7.

Abstract

Environmental toxins and toxicants can damage proteins and threaten cellular proteostasis. Most current methodologies to identify misfolded proteins in cells survey the entire proteome for sites of changed reactivity. We describe and apply a quantitative proteomics methodology to identify destabilized proteins based on their binding to the human Hsp40 chaperone DNAJB8. These protein targets are validated by an orthogonal limited proteolysis assay using parallel reaction monitoring. We find that a brief exposure of HEK293T cells to meta-arsenite increases the affinity of two dozen proteins to DNAJB8, including known arsenite-sensitive proteins. In particular, arsenite treatment destabilizes both the pyruvate dehydrogenase complex E1 subunit and several RNA-binding proteins. This platform can be used to explore how environmental toxins impact cellular proteostasis and to identify the susceptible proteome.

摘要

环境毒素和有毒物质会破坏蛋白质并威胁细胞内的蛋白质稳态。目前大多数用于鉴定细胞中错误折叠蛋白质的方法都检测整个蛋白质组中发生反应性变化的位点。我们描述并应用了一种定量蛋白质组学方法,根据它们与人类热休克蛋白 40 伴侣 DNAJB8 的结合来鉴定不稳定的蛋白质。这些蛋白质靶标通过使用平行反应监测的正交有限蛋白水解测定法进行验证。我们发现,HEK293T 细胞短暂暴露于偏亚砷酸盐会增加二十几种蛋白质与 DNAJB8 的亲和力,其中包括已知的亚砷酸盐敏感蛋白。特别是,亚砷酸盐处理会使丙酮酸脱氢酶复合物 E1 亚基和几种 RNA 结合蛋白失稳。该平台可用于探索环境毒素如何影响细胞内蛋白质稳态,并鉴定易受影响的蛋白质组。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/97ef/9942771/42b806b7f72f/nihms-1844191-f0001.jpg

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