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肌钙蛋白C与肌球蛋白横桥附着之间的相互偶联。

Reciprocal coupling between troponin C and myosin crossbridge attachment.

作者信息

Zot A S, Potter J D

机构信息

Department of Pharmacology, University of Miami School of Medicine, Florida 33101.

出版信息

Biochemistry. 1989 Aug 8;28(16):6751-6. doi: 10.1021/bi00442a031.

DOI:10.1021/bi00442a031
PMID:2790028
Abstract

The attachment of cycling myosin crossbridges to actin and the resultant muscle contraction are regulated in skeletal muscle by the binding of Ca2+ to the amino-terminal, regulatory sites of the troponin C (TnC) subunit of the thin filament protein troponin. Conversely, the attachment of crossbridges to actin has been shown to alter the affinity of TnC for Ca2+. In this study, fluorescently labeled TnC incorporated into reconstituted thin filaments was used to investigate the relationship between crossbridge attachment to actin and structural changes in the amino-terminal region of TnC. Fluorescence intensity changes were measured under the following conditions: saturating [Ca2+] in the absence of crossbridges, rigor crossbridge attachment in the presence and absence of Ca2+, and cycling crossbridge attachment. The percent of heavy meromyosin crossbridges associated with the thin filaments under these conditions was also determined. The results show that, in addition to the binding of Ca2+ to TnC, the attachment of both rigor and cycling crossbridges to actin alters the structure of TnC near the regulatory, Ca2+-specific sites of the molecule. A differential coupling between weakly versus strongly bound crossbridge states and TnC structure was detected, suggesting a possible differential regulation of these states by conformational changes in TnC. These findings illustrate a reciprocal coupling, via thin filament protein interactions, between structural changes in TnC and the attachment of myosin crossbridges to actin, such that each can influence the other, and indicate that TnC is not simply an on-off switch but may exist in a number of different conformations.

摘要

在骨骼肌中,循环的肌球蛋白横桥与肌动蛋白的附着以及由此产生的肌肉收缩是由钙离子(Ca2+)与细肌丝蛋白肌钙蛋白的肌钙蛋白C(TnC)亚基的氨基末端调节位点结合来调控的。相反,已表明横桥与肌动蛋白的附着会改变TnC对Ca2+的亲和力。在本研究中,将掺入重组细肌丝中的荧光标记TnC用于研究横桥与肌动蛋白的附着和TnC氨基末端区域结构变化之间的关系。在以下条件下测量荧光强度变化:无横桥时的饱和[Ca2+]、有和无Ca2+时的强直横桥附着以及循环横桥附着。还测定了在这些条件下与细肌丝相关的重酶解肌球蛋白横桥的百分比。结果表明,除了Ca2+与TnC的结合外,强直和循环横桥与肌动蛋白的附着都会改变TnC分子中靠近调节性Ca2+特异性位点附近的结构。检测到弱结合与强结合横桥状态和TnC结构之间的差异偶联,表明这些状态可能通过TnC的构象变化受到差异调节。这些发现说明了通过细肌丝蛋白相互作用,TnC的结构变化与肌球蛋白横桥与肌动蛋白的附着之间存在相互偶联,使得它们能够相互影响,并表明TnC不仅仅是一个开关,而是可能以多种不同构象存在。

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