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在细胞中定量评估蛋白酪氨酸磷酸酶内源性可逆氧化状态的体外活性测定。

In Vitro Activity Assays to Quantitatively Assess the Endogenous Reversible Oxidation State of Protein Tyrosine Phosphatases in Cells.

机构信息

Department of Nanobioscience, SUNY Polytechnic Institute, Albany, New York.

出版信息

Curr Protoc Chem Biol. 2020 Sep;12(3):e84. doi: 10.1002/cpch.84.

Abstract

The reversible oxidation of protein tyrosine phosphatases (PTPs) impairs their ability to dephosphorylate substrates in vivo. This transient inactivation of PTPs occurs as their conserved catalytic cysteine residue reacts with cellular oxidants thereby abolishing the ability of this reactive cysteine to attack the phosphate of the target substrate. Hence, in vivo, the inhibition of specific PTPs in response to regulated and localized rises in cellular oxidants enables phospho-dependent signaling. We present assays that measure the endogenous activity of specific PTPs that become transiently inactivated in cells exposed to growth factors. Here, we describe the methods and highlight the pitfalls to avoid post-lysis oxidation of PTPs in order to assess the inactivation and the reactivation of PTPs targeted by cellular oxidants in signal transduction. © 2020 Wiley Periodicals LLC. Basic Protocol 1: Cell transfection (optional) Support Protocol: Preparation of degassed lysis buffers Basic Protocol 2: Cellular extraction in anaerobic conditions Basic Protocol 3: Enrichment and activity assay of specific PTPs Alternate Protocol: Measurement of active PTPs via direct cysteinyl labeling.

摘要

蛋白质酪氨酸磷酸酶(PTPs)的可逆氧化会损害其在体内将底物去磷酸化的能力。这种 PTP 瞬时失活是由于其保守的催化半胱氨酸残基与细胞氧化剂反应,从而使该反应性半胱氨酸攻击靶底物磷酸基团的能力丧失。因此,在体内,针对细胞氧化剂的调节和局部升高,特异性 PTP 的抑制作用使磷酸化依赖性信号得以发生。我们提出了测定暴露于生长因子的细胞中内源性特定 PTP 活性的测定方法,这些 PTP 会被瞬时失活。在这里,我们描述了方法并强调了要避免的陷阱,以避免 PTP 在裂解后发生氧化,从而评估细胞氧化剂在信号转导中靶向的 PTP 的失活和再激活。© 2020 威立出版社有限公司。基本方案 1:细胞转染(可选)支持方案:脱气裂解缓冲液的制备基本方案 2:在厌氧条件下进行细胞提取基本方案 3:特定 PTP 的富集和活性测定备选方案:通过直接半胱氨酸标记测量活性 PTPs。

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本文引用的文献

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Cold Spring Harb Perspect Biol. 2014 May 1;6(5):a020644. doi: 10.1101/cshperspect.a020644.

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