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过氧亚硝酸盐对大鼠快肌和慢肌纤维收缩蛋白特性的差异影响。

Differential effects of peroxynitrite on contractile protein properties in fast- and slow-twitch skeletal muscle fibers of rat.

机构信息

Dept. of Zoology, La Trobe Univ., Melbourne 3086, Victoria, Australia.

出版信息

J Appl Physiol (1985). 2011 Mar;110(3):705-16. doi: 10.1152/japplphysiol.00739.2010. Epub 2010 Oct 28.

DOI:10.1152/japplphysiol.00739.2010
PMID:21030671
Abstract

Oxidative modification of contractile proteins is thought to be a key factor in muscle weakness observed in many pathophysiological conditions. In particular, peroxynitrite (ONOO(-)), a potent short-lived oxidant, is a likely candidate responsible for this contractile dysfunction. In this study ONOO(-) or 3-morpholinosydnonimine (Sin-1, a ONOO(-) donor) was applied to rat skinned muscle fibers to characterize the effects on contractile properties. Both ONOO(-) and Sin-1 exposure markedly reduced maximum force in slow-twitch fibers but had much less effect in fast-twitch fibers. The rate of isometric force development was also reduced without change in the number of active cross bridges. Sin-1 exposure caused a disproportionately large decrease in Ca(2+) sensitivity, evidently due to coproduction of superoxide, as it was prevented by Tempol, a superoxide dismutase mimetic. The decline in maximum force with Sin-1 and ONOO(-) treatments could be partially reversed by DTT, provided it was applied before the fiber was activated. Reversal by DTT indicates that the decrease in maximum force was due at least in part to oxidation of cysteine residues. Ascorbate caused similar reversal, further suggesting that the cysteine residues had undergone S-nitrosylation. The reduction in Ca(2+) sensitivity, however, was not reversed by either DTT or ascorbate. Western blot analysis showed cross-linking of myosin heavy chain (MHC) I, appearing as larger protein complexes after ONOO(-) exposure. The findings suggest that ONOO(-) initially decreases maximum force primarily by oxidation of cysteine residues on the myosin heads, and that the accompanying decrease in Ca(2+) sensitivity is likely due to other, less reversible actions of hydroxyl or related radicals.

摘要

氧化修饰的收缩蛋白被认为是在许多病理生理条件下观察到的肌肉无力的一个关键因素。特别是过氧亚硝酸盐(ONOO(-)),一种强的短寿命氧化剂,可能是导致这种收缩功能障碍的候选物。在这项研究中,ONOO(-)或 3-吗啉代-sydnonimine(Sin-1,一种 ONOO(-)供体)被应用于大鼠去皮肌纤维,以表征对收缩特性的影响。ONOO(-)和 Sin-1 暴露都显著降低了慢肌纤维的最大力,但对快肌纤维的影响较小。等长力发展的速度也降低了,而活性横桥的数量没有变化。Sin-1 暴露导致 Ca(2+)敏感性明显降低,显然是由于超氧化物的共同产生,因为它被超氧化物歧化酶模拟物 Tempol 所阻止。用 Sin-1 和 ONOO(-)处理后最大力的下降可以部分被 DTT 逆转,如果在纤维被激活之前应用 DTT。DTT 的逆转表明,最大力的下降至少部分是由于半胱氨酸残基的氧化。抗坏血酸也引起了类似的逆转,进一步表明半胱氨酸残基已经经历了 S-亚硝化。然而,Ca(2+)敏感性的降低不能被 DTT 或抗坏血酸逆转。Western blot 分析显示肌球蛋白重链(MHC)I 的交联,在 ONOO(-)暴露后表现为更大的蛋白质复合物。研究结果表明,ONOO(-)最初主要通过肌球蛋白头部半胱氨酸残基的氧化降低最大力,并且伴随的 Ca(2+)敏感性降低可能是由于羟基或相关自由基的其他、不太可逆的作用。

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