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本文引用的文献

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ON THE ACTIVE SITE OF MYOSIN A-ADENOSINE TRIPHOSPHATASE. IV. PROPERTIES OF BINDING OF TRINITROBENZENESULFONATE AND P-CHLOROMERCURIBENZOATE TO MYOSIN A.
Biochim Biophys Acta. 1963 Dec 13;78:698-704. doi: 10.1016/0006-3002(63)91035-7.
2
On the active site of myosin A-adenosine triphosphatase. II. Properties of the trinitrophenyl enzyme and the enzyme free from divalent cations.关于肌球蛋白A - 三磷酸腺苷酶的活性位点。II. 三硝基苯基酶和不含二价阳离子的酶的性质。
J Biol Chem. 1961 Mar;236:902-6.
3
Conformation of myosin interdomain interactions during contraction: deductions from proteins in solution.收缩过程中肌球蛋白结构域间相互作用的构象:来自溶液中蛋白质的推断。
Biochemistry. 2001 Apr 17;40(15):4834-43. doi: 10.1021/bi002388g.
4
Conformation of myosin interdomain interactions during contraction: deductions from muscle fibers using polarized fluorescence.收缩过程中肌球蛋白结构域间相互作用的构象:利用偏振荧光从肌纤维得出的推论。
Biochemistry. 2001 Apr 17;40(15):4821-33. doi: 10.1021/bi002387o.
5
Three conformational states of scallop myosin S1.扇贝肌球蛋白S1的三种构象状态。
Proc Natl Acad Sci U S A. 2000 Oct 10;97(21):11238-43. doi: 10.1073/pnas.200376897.
6
Structural mechanism of muscle contraction.肌肉收缩的结构机制。
Annu Rev Biochem. 1999;68:687-728. doi: 10.1146/annurev.biochem.68.1.687.
7
Trinitrophenylated reactive lysine residue in myosin detects lever arm movement during the consecutive steps of ATP hydrolysis.
Biochemistry. 1999 May 18;38(20):6428-40. doi: 10.1021/bi990149r.
8
Atomic structure of scallop myosin subfragment S1 complexed with MgADP: a novel conformation of the myosin head.与MgADP复合的扇贝肌球蛋白亚片段S1的原子结构:肌球蛋白头部的一种新构象。
Cell. 1999 May 14;97(4):459-70. doi: 10.1016/s0092-8674(00)80756-4.
9
Formation of the myosin.ADP.gallium fluoride complex and its solution structure by small-angle synchrotron X-ray scattering.肌球蛋白-ADP-氟化镓复合物的形成及其通过小角同步加速器X射线散射得到的溶液结构
J Biochem. 1999 Jan;125(1):177-85. doi: 10.1093/oxfordjournals.jbchem.a022257.
10
Crystal structure of a vertebrate smooth muscle myosin motor domain and its complex with the essential light chain: visualization of the pre-power stroke state.脊椎动物平滑肌肌球蛋白运动结构域及其与必需轻链复合物的晶体结构:动力冲程前状态的可视化
Cell. 1998 Sep 4;94(5):559-71. doi: 10.1016/s0092-8674(00)81598-6.

通过阻碍杠杆臂运动,使肌球蛋白收缩循环中ATP酶激活与力产生发生化学解偶联。

Chemical decoupling of ATPase activation and force production from the contractile cycle in myosin by steric hindrance of lever-arm movement.

作者信息

Muhlrad Andras, Peyser Y Michael, Nili Mahta, Ajtai Katalin, Reisler Emil, Burghardt Thomas P

机构信息

Department of Oral Biology, Hebrew University Hadassah School of Dental Medicine, Jerusalem, Israel 91120.

出版信息

Biophys J. 2003 Feb;84(2 Pt 1):1047-56. doi: 10.1016/S0006-3495(03)74921-2.

DOI:10.1016/S0006-3495(03)74921-2
PMID:12547786
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1302682/
Abstract

The myosin motor protein generates force in muscle by hydrolyzing Adenosine 5'-triphosphate (ATP) while interacting transiently with actin. Structural evidence suggests the myosin globular head (subfragment 1 or S1) is articulated with semi-rigid catalytic and lever-arm domains joined by a flexible converter domain. According to the prevailing hypothesis for energy transduction, ATP binding and hydrolysis in the catalytic domain drives the relative movement of the lever arm. Actin binding and reversal of the lever-arm movement (power stroke) applies force to actin. These domains interface at the reactive lysine, Lys84, where trinitrophenylation (TNP-Lys84-S1) was observed in this work to block actin activation of myosin ATPase and in vitro sliding of actin over myosin. TNP-Lys84-S1's properties and interactions with actin were examined to determine how trinitrophenylation causes these effects. Weak and strong actin binding, the rate of mantADP release from actomyosin, and actomyosin dissociation by ATP were equivalent in TNP-Lys84-S1 and native S1. Molecular dynamics calculations indicate that lever-arm movement inhibition during ATP hydrolysis and the power stroke is caused by steric clashes between TNP and the converter or lever-arm domains. Together these findings suggest that TNP uncouples actin activation of myosin ATPase and the power stroke from other steps in the contraction cycle by inhibiting the converter and lever-arm domain movements.

摘要

肌球蛋白运动蛋白通过水解三磷酸腺苷(ATP)在肌肉中产生力,同时与肌动蛋白短暂相互作用。结构证据表明,肌球蛋白球状头部(亚片段1或S1)由半刚性催化结构域和杠杆臂结构域通过柔性转换器结构域连接而成。根据普遍的能量转导假说,催化结构域中的ATP结合和水解驱动杠杆臂的相对运动。肌动蛋白结合和杠杆臂运动的反向(动力冲程)将力施加到肌动蛋白上。这些结构域在反应性赖氨酸Lys84处相互作用,在本研究中观察到三硝基苯化(TNP-Lys84-S1)可阻断肌动蛋白对肌球蛋白ATP酶的激活以及肌动蛋白在肌球蛋白上的体外滑动。研究了TNP-Lys84-S1的特性及其与肌动蛋白的相互作用,以确定三硝基苯化如何引起这些效应。TNP-Lys84-S1与天然S1的弱和强肌动蛋白结合、mantADP从肌动球蛋白释放的速率以及ATP引起的肌动球蛋白解离均相当。分子动力学计算表明,ATP水解和动力冲程期间杠杆臂运动的抑制是由TNP与转换器或杠杆臂结构域之间的空间冲突引起的。这些发现共同表明,TNP通过抑制转换器和杠杆臂结构域的运动,使肌动蛋白对肌球蛋白ATP酶的激活和动力冲程与收缩周期中的其他步骤解偶联。