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本文引用的文献

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Ultrastructural observations of isolated intact and fragmented junctions of skeletal muscle by use of tannic acid mordanting.利用单宁酸媒染法对骨骼肌分离的完整和断裂连接进行超微结构观察。
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Isolation of sarcoplasmic reticulum by zonal centrifugation and purification of Ca 2+ -pump and Ca 2+ -binding proteins.通过区带离心法分离肌浆网以及纯化钙离子泵和钙离子结合蛋白。
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从骨骼肌中纯化形态完整的三联体结构。

Purification of morphologically intact triad structures from skeletal muscle.

作者信息

Mitchell R D, Palade P, Fleischer S

出版信息

J Cell Biol. 1983 Apr;96(4):1008-16. doi: 10.1083/jcb.96.4.1008.

DOI:10.1083/jcb.96.4.1008
PMID:6300142
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2112327/
Abstract

A procedure has been devised for isolation of triads (t-tubule/sarcoplasmic reticulum (SR) junctional complexes) from rabbit skeletal muscle. The procedure consists of preparation of a heavy microsomal fraction followed by two sequential 90-min sucrose gradient centrifugations to enrich the triads. A pyrophosphate/phosphate/magnesium buffer system was introduced to decrease aggregation in order to achieve effective separation. The preparation time is 12 h. Some differences between purified triads isolated by two variants of this method are noted. The purity of the triad fractions has been estimated by particle counting to be in the vicinity of 50%. There is good retention of morphology and Ca++-loading activity and enrichment in Na+,K+-ATPase and adenylate cyclase. The triads are practically devoid of contractile elements, mitochondria, and free plasmalemma, and low in content of light SR. The method for obtaining enriched triads is reproducible, and sufficient yields are obtained for structural, biochemical, and functional characterization.

摘要

已设计出一种从兔骨骼肌中分离三联体(横小管/肌浆网(SR)连接复合体)的方法。该方法包括制备重微粒体部分,然后进行两次连续90分钟的蔗糖梯度离心以富集三联体。引入焦磷酸/磷酸/镁缓冲系统以减少聚集,从而实现有效分离。制备时间为12小时。注意到通过该方法的两种变体分离得到的纯化三联体之间存在一些差异。通过颗粒计数估计三联体组分的纯度在50%左右。三联体在形态和钙负载活性方面保持良好,并且在Na +,K + -ATP酶和腺苷酸环化酶方面得到富集。三联体实际上不含收缩元件、线粒体和游离质膜,并且轻肌浆网含量低。获得富集三联体的方法具有可重复性,并且能够获得足够的产量用于结构、生化和功能表征。