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心肌肌钙蛋白I羧基末端可移动结构域和连接序列在调节心脏收缩中的作用。

Role of cardiac troponin I carboxy terminal mobile domain and linker sequence in regulating cardiac contraction.

作者信息

Meyer Nancy L, Chase P Bryant

机构信息

Department of Biochemistry and Molecular Biology, Oregon Health and Science University, Portland, OR, USA.

Department of Biological Science and Program in Molecular Biophysics, Florida State University, Tallahassee, FL, USA.

出版信息

Arch Biochem Biophys. 2016 Jul 1;601:80-7. doi: 10.1016/j.abb.2016.03.010. Epub 2016 Mar 10.

Abstract

Inhibition of striated muscle contraction at resting Ca(2+) depends on the C-terminal half of troponin I (TnI) in thin filaments. Much focus has been on a short inhibitory peptide (Ip) sequence within TnI, but structural studies and identification of disease-associated mutations broadened emphasis to include a larger mobile domain (Md) sequence at the C-terminus of TnI. For Md to function effectively in muscle relaxation, tight mechanical coupling to troponin's core-and thus tropomyosin-is presumably needed. We generated recombinant, human cardiac troponins containing one of two TnI constructs: either an 8-amino acid linker between Md and the rest of troponin (cTnILink8), or an Md deletion (cTnI1-163). Motility assays revealed that Ca(2+)-sensitivity of reconstituted thin filament sliding was markedly increased with cTnILink8 (∼0.9 pCa unit leftward shift of speed-pCa relation compared to WT), and increased further when Md was missing entirely (∼1.4 pCa unit shift). Cardiac Tn's ability to turn off filament sliding at diastolic Ca(2+) was mostly (61%), but not completely eliminated with cTnI1-163. TnI's Md is required for full inhibition of unloaded filament sliding, although other portions of troponin-presumably including Ip-are also necessary. We also confirm that TnI's Md is not responsible for superactivation of actomyosin cycling by troponin.

摘要

在静息钙浓度下,横纹肌收缩的抑制取决于细肌丝中肌钙蛋白I(TnI)的C端半段。此前研究大多聚焦于TnI内的一个短抑制肽(Ip)序列,但结构研究以及疾病相关突变的鉴定使人们将重点扩展至包括TnI C端一个更大的可移动结构域(Md)序列。为使Md在肌肉舒张中有效发挥作用,可能需要与肌钙蛋白核心以及原肌球蛋白紧密机械偶联。我们构建了重组人心脏肌钙蛋白,其包含两种TnI构建体之一:要么是Md与肌钙蛋白其余部分之间有一个8个氨基酸的接头(cTnILink8),要么是Md缺失(cTnI1 - 163)。运动分析显示,与野生型相比,cTnILink8使重组细肌丝滑动的钙敏感性显著增加(速度 - pCa关系向左移动约0.9个pCa单位),而当Md完全缺失时进一步增加(约1.4个pCa单位的移动)。心脏肌钙蛋白在舒张期钙浓度下关闭肌丝滑动的能力大部分(61%)但并非完全被cTnI1 - 163消除。虽然肌钙蛋白的其他部分(可能包括Ip)也是必需的,但TnI的Md对于完全抑制无负荷肌丝滑动是必需的。我们还证实,TnI的Md并不负责肌钙蛋白对肌动球蛋白循环的超激活作用。

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