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β-肌动蛋白的一种翻译后修饰作用导致不可逆性镰状细胞的血影蛋白-蛋白4.1-肌动蛋白复合物的缓慢解离。

A posttranslational modification of beta-actin contributes to the slow dissociation of the spectrin-protein 4.1-actin complex of irreversibly sickled cells.

作者信息

Shartava A, Monteiro C A, Bencsath F A, Schneider K, Chait B T, Gussio R, Casoria-Scott L A, Shah A K, Heuerman C A, Goodman S R

机构信息

Department of Structural and Cellular Biology, University of South Alabama College of Medicine, Mobile 36688.

出版信息

J Cell Biol. 1995 Mar;128(5):805-18. doi: 10.1083/jcb.128.5.805.

DOI:10.1083/jcb.128.5.805
PMID:7876306
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2120399/
Abstract

Irreversibly sickled cells (ISCs) remain sickled even under conditions where they are well oxygenated and hemoglobin is depolymerized. In our studies we demonstrate that triton extracted ISC core skeletons containing only spectrin, protein 4.1, and actin also retain their sickled shape; while reversibly sickled cell (RSC) skeletons remodel to a round or biconcave shape. We also demonstrate that these triton extracted ISC core skeletons dissociate more slowly upon incubation at 37 degrees C than do RSC or control (AA) core skeletons. This observation may supply the basis for the inability of the ISC core skeleton to remodel its shape. Using an in vitro ternary complex dissociation assay, we demonstrate that a modification in beta-actin is the major determinant of the slow dissociation of the spectrin-protein 4.1-actin complex isolated from the ISC core skeleton. We demonstrate that the difference between ISC and control beta-actin is the inaccessibility of two cysteine residues in ISC beta-actin to labeling by thiol reactive reagents; due to the formation of a disulfide bridge between cysteine284 and cysteine373 in ISC beta-actin, or alternatively another modification of cysteine284 and cysteine373 which is reversible with DTT and adds less than 100 D to the molecular weight of beta-actin.

摘要

不可逆镰状细胞(ISC)即使在充分氧合且血红蛋白解聚的条件下仍保持镰状形态。在我们的研究中,我们证明,仅含有血影蛋白、蛋白4.1和肌动蛋白的经曲拉通提取的ISC核心骨架也保持其镰状形态;而可逆镰状细胞(RSC)骨架则重塑为圆形或双凹形。我们还证明,这些经曲拉通提取的ISC核心骨架在37℃孵育时比RSC或对照(AA)核心骨架解离得更慢。这一观察结果可能为ISC核心骨架无法重塑其形状提供了基础。使用体外三元复合物解离试验,我们证明β-肌动蛋白的修饰是从ISC核心骨架分离的血影蛋白-蛋白4.1-肌动蛋白复合物缓慢解离的主要决定因素。我们证明,ISCβ-肌动蛋白与对照β-肌动蛋白之间的差异在于ISCβ-肌动蛋白中的两个半胱氨酸残基无法被硫醇反应试剂标记;这是由于ISCβ-肌动蛋白中半胱氨酸284和半胱氨酸373之间形成了二硫键,或者是半胱氨酸284和半胱氨酸373的另一种修饰,这种修饰可被二硫苏糖醇逆转,且使β-肌动蛋白的分子量增加不到100道尔顿。

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