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肌钙蛋白调节功能和动力学通过氘/氢交换质谱法揭示。

Troponin regulatory function and dynamics revealed by H/D exchange-mass spectrometry.

机构信息

Department of Medicine, University of Illinois at Chicago, Chicago, Illinois 60612, USA.

出版信息

J Biol Chem. 2010 Jan 22;285(4):2686-94. doi: 10.1074/jbc.M109.062349. Epub 2009 Nov 17.

Abstract

Muscle contraction is tightly regulated by Ca(2+) binding to the thin filament protein troponin. The mechanism of this regulation was investigated by detailed mapping of the dynamic properties of cardiac troponin using amide hydrogen exchange-mass spectrometry. Results were obtained in the presence of either saturation or non-saturation of the regulatory Ca(2+) binding site in the NH(2) domain of subunit TnC. Troponin was found to be highly dynamic, with 60% of amides exchanging H for D within seconds of exposure to D(2)O. In contrast, portions of the TnT-TnI coiled-coil exhibited high protection from exchange, despite 6 h in D(2)O. The data indicate that the most stable portion of the trimeric troponin complex is the coiled-coil. Regulatory site Ca(2+) binding altered dynamic properties (i.e. H/D exchange protection) locally, near the binding site and in the TnI switch helix that attaches to the Ca(2+)-saturated TnC NH(2) domain. More notably, Ca(2+) also altered the dynamic properties of other parts of troponin: the TnI inhibitory peptide region that binds to actin, the TnT-TnI coiled-coil, and the TnC COOH domain that contains the regulatory Ca(2+) sites in many invertebrate as opposed to vertebrate troponins. Mapping of these affected regions onto the troponin highly extended structure suggests that cardiac troponin switches between alternative sets of intramolecular interactions, similar to previous intermediate resolution x-ray data of skeletal muscle troponin.

摘要

肌肉收缩受 Ca(2+)与细肌丝蛋白肌钙蛋白结合的紧密调控。通过酰胺氢交换-质谱法详细绘制心脏肌钙蛋白的动态特性,研究了这种调控的机制。结果是在肌钙蛋白 C 亚基 NH2 结构域的调节 Ca(2+)结合位点饱和或非饱和的情况下获得的。肌钙蛋白被发现具有高度的动态性,有 60%的酰胺在暴露于 D2O 后的几秒钟内交换 H 为 D。相比之下,尽管在 D2O 中存在 6 小时,TnT-TnI 卷曲螺旋的部分仍表现出对交换的高度保护。数据表明,三聚体肌钙蛋白复合物最稳定的部分是卷曲螺旋。调节位点 Ca(2+)结合局部改变了动力学特性(即 H/D 交换保护),靠近结合位点和连接到 Ca(2+)饱和的 TnC NH2 结构域的 TnI 开关螺旋。更值得注意的是,Ca(2+)还改变了肌钙蛋白的其他部分的动力学特性:与肌动蛋白结合的 TnI 抑制肽区域、TnT-TnI 卷曲螺旋以及 TnC COOH 结构域,其中包含许多无脊椎动物而非脊椎动物肌钙蛋白的调节 Ca(2+)位点。这些受影响的区域映射到肌钙蛋白的高度扩展结构上表明,心脏肌钙蛋白在类似先前骨骼肌肌钙蛋白的中间分辨率 X 射线数据的不同的分子内相互作用之间切换。

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