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大鼠快肌和慢肌骨骼肌纤维电刺激后钙瞬变的衰减

Decay of calcium transients after electrical stimulation in rat fast- and slow-twitch skeletal muscle fibres.

作者信息

Carroll S L, Klein M G, Schneider M F

机构信息

University of Maryland, School of Medicine, Department of Biochemistry and Molecular Biology, Baltimore 21201, USA.

出版信息

J Physiol. 1997 Jun 15;501 ( Pt 3)(Pt 3):573-88. doi: 10.1111/j.1469-7793.1997.573bm.x.

Abstract
  1. Calcium transients were calculated from fura-2 fluorescence signals (corrected for kinetic delays in the Ca(2+)-fura-2 reaction) from single rat skeletal muscle fibres, either fully dissociated from the fast-twitch flexor digitorum brevis (FDB) muscle or in small bundles from the slow-twitch soleus muscle. Fibres or bundles were embedded in agarose gel to inhibit movement and stimulated by single or trains of 1-2 ms electrical pulses (100 Hz, 2-400 ms train duration). 2. The rate constant of decay of [Ca2+] determined from single-exponential fits to the final decay phase of [Ca2+] after a single action potential was considerably faster in FDB fibres than in soleus fibres. As the stimulation duration increased, the rate constant of [Ca2+] decay decreased for both the FDB and soleus fibres, but the effect was greater in FDB than in soleus fibres. 3. Using the magnitude of the decline in the rate constant of [Ca2+] decay with increasing stimulation duration as an index of relative contribution of the saturable Ca2+ binding sites on parvalbumin, subpopulations termed 'high', 'medium' and 'low', referring to estimated parvalbumin content, were determined within each group of FDB and soleus fibres. In fibres assigned to the 'high' and 'medium' groups, parvalbumin was the major contributor (50-73%) to the [Ca2+] decay rate constant after a single action potential. In fibres in the 'low' group, parvalbumin contributed only 0-28% to the rate constant of [Ca2+] decay. 4. Fluorescence recordings using mag-fura-2, a lower-affinity Ca2+ indicator expected to be in equilibrium with myoplasmic Ca2+, gave similar values for both the [Ca2+] decay rate constant after a single action potential and the decrease in this rate constant with increased stimulation duration, as found for the fura-2 [Ca2+] transients from FDB and soleus fibres. Thus, the observed differences in decay rate of Ca2+ were not introduced by kinetic correction of the fura-2 recordings, but are attributed to differences in the Ca2+ binding and transport properties of fast- and slow-twitch mammalian fibres.
摘要
  1. 钙瞬变是根据来自单个大鼠骨骼肌纤维的fura - 2荧光信号计算得出的(已针对Ca(2 +)-fura - 2反应中的动力学延迟进行校正),这些纤维要么完全解离自快肌趾短屈肌(FDB),要么成小束取自慢肌比目鱼肌。将纤维或纤维束嵌入琼脂糖凝胶中以抑制其移动,并通过单个或一串1 - 2毫秒的电脉冲(100赫兹,串持续时间2 - 400毫秒)进行刺激。2. 从单个动作电位后[Ca2 +]最终衰减阶段的单指数拟合确定的[Ca2 +]衰减速率常数,在FDB纤维中比在比目鱼肌纤维中快得多。随着刺激持续时间增加,FDB和比目鱼肌纤维的[Ca2 +]衰减速率常数均降低,但FDB纤维中的这种效应比在比目鱼肌纤维中更大。3. 以[Ca2 +]衰减速率常数随刺激持续时间增加而下降的幅度作为小清蛋白上可饱和Ca2 +结合位点相对贡献的指标,在每组FDB和比目鱼肌纤维中确定了称为“高”、“中”和“低”的亚群,这是指估计的小清蛋白含量。在归入“高”和“中”组的纤维中,小清蛋白是单个动作电位后[Ca2 +]衰减速率常数的主要贡献者(50 - 73%)。在“低”组的纤维中,小清蛋白对[Ca2 +]衰减速率常数的贡献仅为0 - 28%。4. 使用mag - fura - 2进行的荧光记录,mag - fura - 2是一种预期与肌浆Ca2 +处于平衡状态的低亲和力Ca2 +指示剂,对于单个动作电位后的[Ca2 +]衰减速率常数以及该速率常数随刺激持续时间增加的降低情况,得到了与FDB和比目鱼肌纤维的fura - 2 [Ca2 +]瞬变相似的值。因此,观察到的Ca2 +衰减速率差异不是由fura - 2记录的动力学校正引入的,而是归因于快肌和慢肌哺乳动物纤维在Ca2 +结合和转运特性方面的差异。
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/d2d8/1159459/c90da15d979a/jphysiol00277-0091-a.jpg

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