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肌酸激酶同工酶在肌原纤维中的定位。I. 鸡骨骼肌

Localization of creatine kinase isoenzymes in myofibrils. I. Chicken skeletal muscle.

作者信息

Wallimann T, Turner D C, Eppenberger H M

出版信息

J Cell Biol. 1977 Nov;75(2 Pt 1):297-317. doi: 10.1083/jcb.75.2.297.

Abstract

Purified, repeatedly washed, skeletal muscle myofibrils contain approx. 0.2 U of creatine kinase (CK) activity (equivalent to 2.5 micrograms CK) per milligram dry weight; this firmly bound CK activity is estimated to represent 3-5% of the total cellular CK. It had been shown previously that the myofibrillar CK, which can be quantitatively extracted at low ionic strength and purified to homogeneity, is very similar, if not identical, to the bulk MM-CK. It is shown that the two protein preparations also have the same peptide pattern after cyanogen bromide fractionation and very similar specific activities, confirming their identity. The earlier demonstration that the bound CK is specifically located at the M-lines of isolated myofibrils has been confirmed by immunofluorescence. Antibodies directed against purified MM- and BB-CK were used in the indirect fluorescent antibody technique to study the specificity of myofibril binding sites for different forms of CK. With myofibrils from adult muscle, which has only MM-CK, as well as from early developmental stages in which BB-CK is the predominant isoenzyme, M-type CK was localized exclusively at the M-line, while greater or lesser amounts of B-type CK were found at the Z-line. The data provide strong evidence that the MM-CK at the M-lines in skeletal myofibrils is not adventitiously bound but is rather an integral element in the M-line structure. The amount of CK bound is reasonably consistent with the earlier proposal that the CK molecules might be the transverse M-bridges and appears to be sufficient to regenerate all of the ATP hydrolyzed during muscle contraction.

摘要

纯化且经反复洗涤的骨骼肌肌原纤维每毫克干重约含0.2单位的肌酸激酶(CK)活性(相当于2.5微克CK);这种紧密结合的CK活性估计占细胞总CK的3 - 5%。先前已经表明,在低离子强度下可定量提取并纯化至同质的肌原纤维CK,即便不完全相同,也与大部分MM - CK非常相似。结果表明,这两种蛋白质制剂在溴化氰分级分离后也具有相同的肽图谱和非常相似的比活性,证实了它们的同一性。通过免疫荧光证实了早期的发现,即结合的CK特异性定位于分离的肌原纤维的M线。在间接荧光抗体技术中,使用针对纯化的MM - CK和BB - CK的抗体来研究不同形式CK的肌原纤维结合位点的特异性。对于仅含有MM - CK的成年肌肉的肌原纤维以及以BB - CK为主的早期发育阶段的肌原纤维,M型CK仅定位于M线,而在Z线发现了或多或少的B型CK。这些数据提供了有力证据,表明骨骼肌肌原纤维M线处的MM - CK并非偶然结合,而是M线结构的一个组成部分。结合的CK量与早期提出的CK分子可能是横向M桥的观点相当一致,并且似乎足以再生肌肉收缩过程中水解的所有ATP。

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