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使用新型高速采集系统,测定野生型、mdx型和转基因微肌营养不良蛋白小鼠的电压钳制完整骨骼肌纤维的无负荷缩短速度。

Unloaded speed of shortening in voltage-clamped intact skeletal muscle fibers from wt, mdx, and transgenic minidystrophin mice using a novel high-speed acquisition system.

作者信息

Friedrich O, Weber C, von Wegner F, Chamberlain J S, Fink R H A

机构信息

Medical Biophysics, Department of Systems Physiology, Institute of Physiology and Pathophysiology, Ruprecht-Karls-University, Heidelberg, Germany.

出版信息

Biophys J. 2008 Jun;94(12):4751-65. doi: 10.1529/biophysj.107.126557. Epub 2008 Apr 18.

Abstract

Skeletal muscle unloaded shortening has been indirectly determined in the past. Here, we present a novel high-speed optical tracking technique that allows recording of unloaded shortening in single intact, voltage-clamped mammalian skeletal muscle fibers with 2-ms time resolution. L-type Ca(2+) currents were simultaneously recorded. The time course of shortening was biexponential: a fast initial phase, tau(1), and a slower successive phase, tau(2,) with activation energies of 59 kJ/mol and 47 kJ/mol. Maximum unloaded shortening speed, v(u,max), was faster than that derived using other techniques, e.g., approximately 14.0 L(0) s(-1) at 30 degrees C. Our technique also allowed direct determination of shortening acceleration. We applied our technique to single fibers from C57 wild-type, dystrophic mdx, and minidystrophin-expressing mice to test whether unloaded shortening was affected in the pathophysiological mechanism of Duchenne muscular dystrophy. v(u,max) and a(u,max) values were not significantly different in the three strains, whereas tau(1) and tau(2) were increased in mdx fibers. The results were complemented by myosin heavy and light chain (MLC) determinations that showed the same myosin heavy chain IIA profiles in the interossei muscles from the different strains. In mdx muscle, MLC-1f was significantly increased and MLC-2f and MLC-3f somewhat reduced. Fast initial active shortening seems almost unaffected in mdx muscle.

摘要

过去,骨骼肌无负荷缩短情况是通过间接方法测定的。在此,我们介绍一种新型高速光学跟踪技术,该技术能够以2毫秒的时间分辨率记录单个完整的、电压钳制的哺乳动物骨骼肌纤维的无负荷缩短情况。同时记录L型钙电流。缩短过程呈双指数形式:一个快速的初始阶段,时间常数为tau(1),以及一个较慢的后续阶段,时间常数为tau(2),其活化能分别为59千焦/摩尔和47千焦/摩尔。最大无负荷缩短速度v(u,max)比使用其他技术得出的速度更快,例如在30摄氏度时约为14.0 L(0) s(-1)。我们的技术还能直接测定缩短加速度。我们将该技术应用于C57野生型、营养不良的mdx型以及表达微小抗肌萎缩蛋白的小鼠的单根纤维,以测试在杜兴氏肌营养不良的病理生理机制中无负荷缩短是否受到影响。在这三种品系中,v(u,max)和a(u,max)值没有显著差异,而mdx纤维中的tau(1)和tau(2)增加。肌球蛋白重链和轻链(MLC)测定结果补充了上述结果,这些结果表明不同品系的指间肌中肌球蛋白重链IIA谱相同。在mdx肌肉中,MLC - 1f显著增加,MLC - 2f和MLC - 3f略有降低。mdx肌肉中快速的初始主动缩短似乎几乎未受影响。

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