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Detection of Intracellular Reduced (Catalytically Active) SHP-1 and Analyses of Catalytically Inactive SHP-1 after Oxidation by Pervanadate or H2O2

机译:过氧钒酸盐或过氧化氢氧化后细胞内还原型(催化活性)SHP-1的检测和催化活性SHP-1的分析

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摘要

Oxidative inactivation of cysteine-dependent Protein Tyrosine Phosphatases (PTPs) by cellular reactive oxygen species (ROS) plays a critical role in regulating signal transduction in multiple cell types. The phosphatase activity of most PTPs depends upon a ‘signature’ cysteine residue within the catalytic domain that is maintained in the de-protonated state at physiological pH rendering it susceptible to ROS-mediated oxidation. Direct and indirect techniques for detection of PTP oxidation have been developed (). To detect catalytically active PTPs, cell lysates are treated with iodoacetyl-polyethylene glycol-biotin (IAP-biotin), which irreversibly binds to reduced (S-) cysteine thiols. Irreversible oxidation of SHP-1 after treatment of cells with pervanadate or H2O2 is detected with antibodies specific for the sulfonic acid (SO3H) form of the conserved active site cysteine of PTPs. In this protocol, we describe a method for the detection of the reduced (S-; active) or irreversibly oxidized (SO3H; inactive) form of the hematopoietic PTP SHP-1 in thymocytes, although this method is applicable to any cysteine-dependent PTP in any cell type.
机译:细胞活性氧(ROS)对半胱氨酸依赖性蛋白酪氨酸磷酸酶(PTP)的氧化失活在调节多种细胞类型的信号转导中起关键作用。大多数PTP的磷酸酶活性取决于催化域中的“签名”半胱氨酸残基,该残基在生理pH下保持去质子化状态,使其易于受到ROS介导的氧化作用。已经开发了用于检测PTP氧化的直接和间接技术()。为了检测具有催化活性的PTP,用碘乙酰基-聚乙二醇-生物素(IAP-生物素)处理细胞裂解液,该碘不可逆地与还原的(S -)半胱氨酸硫醇结合。用对PTP保守的活性位点半胱氨酸的磺酸(SO3H)形式具有特异性的抗体,检测到用过钒酸盐或过氧化氢处理细胞后SHP-1的不可逆氧化。在此协议中,我们描述了一种检测胸腺细胞中造血PTP SHP-1的还原(S -;活性)或不可逆氧化(SO3H;失活)形式的方法,尽管该方法是适用于任何细胞类型的任何半胱氨酸依赖性PTP。

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