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慢肌和快肌肌浆网钙释放的比较。

Comparison of calcium release from sarcoplasmic reticulum of slow and fast twitch muscles.

作者信息

Lee Y S, Ondrias K, Duhl A J, Ehrlich B E, Kim D H

机构信息

Department of Medicine, University of Connecticut Health Center, Farmington 06030.

出版信息

J Membr Biol. 1991 Jun;122(2):155-63. doi: 10.1007/BF01872638.

Abstract

The mechanism of Ca2+ release from the sarcoplasmic reticulum (SR) of slow and fast twitch muscle was compared by examining biochemical characteristics, ryanodine binding, Ca2+ efflux, and single Ca2+ channel properties of SR vesicles. Although many features of the Ca2+ release channel were comparable, two functional assays revealed remarkable differences. The comparable properties include: a high molecular weight protein from both types of muscle was immunologically equivalent, and Scatchard analysis of [3H]ryanodine binding to SR showed that the Kd was similar for slow and fast SR. In the flux assay the sensitivity to the agonists caffeine, doxorubicin, and Ca2+ and the antagonists Mg2+, ruthenium red, and tetracaine differed only slightly. When SR vesicles were incorporated into lipid bilayers, the single-channel conductances of the Ca2+ release channels were indistinguishable. The distinguishing properties are: When Ca2+ release from passively 45Ca(2+)-loaded SR were monitored by rapid filtration, the initial rates of Ca2+ release induced by Ca2+ and caffeine were three times lower in slow SR than in fast SR. Similarly, when Ca2+ release channels were incorporated into lipid bilayers, the open probability of the slow SR channel was markedly less, mainly due to a longer mean closed time. Our results indicate that slow and fast muscle have ryanodine receptors that are biochemically analogous, yet functional differences in the Ca2+ release channel may contribute to the different time to peak contraction observed in intact slow and fast muscles.

摘要

通过检测肌浆网(SR)囊泡的生化特性、ryanodine结合、Ca2+流出以及单个Ca2+通道特性,比较了慢肌和快肌肌浆网中Ca2+释放的机制。尽管Ca2+释放通道的许多特征具有可比性,但两项功能测定显示出显著差异。具有可比性的特性包括:两种类型肌肉中的高分子量蛋白质在免疫上是等效的,对[3H]ryanodine与SR结合的Scatchard分析表明,慢肌和快肌SR的Kd相似。在通量测定中,对激动剂咖啡因、阿霉素和Ca2+以及拮抗剂Mg2+、钌红和丁卡因的敏感性仅略有不同。当SR囊泡整合到脂质双层中时,Ca2+释放通道的单通道电导无法区分。显著不同的特性是:当通过快速过滤监测被动加载45Ca(2+)的SR中的Ca2+释放时,Ca2+和咖啡因诱导的Ca2+释放初始速率在慢肌SR中比在快肌SR中低三倍。同样,当Ca2+释放通道整合到脂质双层中时,慢肌SR通道的开放概率明显更低,主要是由于平均关闭时间更长。我们的结果表明,慢肌和快肌具有生化相似的ryanodine受体,但Ca2+释放通道的功能差异可能导致在完整的慢肌和快肌中观察到的收缩峰值时间不同。

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