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鸡骨骼肌肌钙蛋白C的克隆、表达及定点诱变

Cloning, expression, and site-directed mutagenesis of chicken skeletal muscle troponin C.

作者信息

Reinach F C, Karlsson R

机构信息

Departamento de Bioquimica, Universidade de Sao Paulo C.P., Brazil.

出版信息

J Biol Chem. 1988 Feb 15;263(5):2371-6.

PMID:2963002
Abstract

Skeletal muscle troponin C (TNC) is structured into two separate domains linked by a nine-turn alpha-helix (D/E helix). It has been demonstrated that calcium binding to the regulatory sites within the N-terminal domain induces conformational changes in the C-terminal domain of isolated TNC. Since the only contact between the two domains is the long D/E helix, the transfer of information must involve conformational changes within this helix. The center of the helix is occupied by a glycine (Gly-92). A postulated mechanism for allowing interdomain interaction involves a conformational change of the D/E helix around Gly-92 (Herzberg, O., and James, M. N. G. (1985) Nature 312, 653-659). We tested this hypothesis using site-directed mutants of troponin C. Two separate mutants containing an alanine and a proline replacing Gly-92 were constructed and compared with wild type TNC. Calcium binding studies showed no significant differences among the TNC species. The different TNC were assembled into thin filaments and used to assay the calcium regulation of actin-activated ATPase of myosin. All TNC species were able to mediate the calcium regulation of ATPase. Under the conditions used for the assays, no differences were detected among the TNC species. These results show that Gly-92 is not essential for the proper interaction of the calcium regulatory sites with the other components of the thin filament, and therefore exclude a large rotation around Gly-92 as the mechanism of information transfer between the two domains of troponin C.

摘要

骨骼肌肌钙蛋白C(TNC)由两个通过九圈α-螺旋(D/E螺旋)相连的独立结构域组成。已经证明,钙与N端结构域内的调节位点结合会诱导分离的TNC的C端结构域发生构象变化。由于两个结构域之间唯一的接触是长的D/E螺旋,信息传递必定涉及该螺旋内的构象变化。螺旋中心被一个甘氨酸(Gly-92)占据。一种假定的允许结构域间相互作用的机制涉及D/E螺旋围绕Gly-92的构象变化(赫茨伯格,O.,和詹姆斯,M.N.G.(1985年)《自然》312,653 - 659)。我们使用肌钙蛋白C的定点突变体来检验这一假设。构建了两个分别含有丙氨酸和脯氨酸取代Gly-92的独立突变体,并与野生型TNC进行比较。钙结合研究表明,不同TNC种类之间没有显著差异。将不同的TNC组装成细肌丝,并用于测定肌动蛋白激活的肌球蛋白ATP酶的钙调节作用。所有TNC种类都能够介导ATP酶的钙调节。在用于测定的条件下,未检测到不同TNC种类之间存在差异。这些结果表明,Gly-92对于钙调节位点与细肌丝其他成分的正确相互作用并非必不可少,因此排除了围绕Gly-92的大幅旋转作为肌钙蛋白C两个结构域之间信息传递机制的可能性。

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