Literature DB >> 29642034

TnI Structural Interface with the N-Terminal Lobe of TnC as a Determinant of Cardiac Contractility.

Anthony D Vetter1, Evelyne M Houang1, Jordan J Sell1, Brian R Thompson1, Yuk Y Sham1, Joseph M Metzger2.   

Abstract

The heterotrimeric cardiac troponin complex is a key regulator of contraction and plays an essential role in conferring Ca2+ sensitivity to the sarcomere. During ischemic injury, rapidly accumulating protons acidify the myoplasm, resulting in markedly reduced Ca2+ sensitivity of the sarcomere. Unlike the adult heart, sarcomeric Ca2+ sensitivity in fetal cardiac tissue is comparatively pH insensitive. Replacement of the adult cardiac troponin I (cTnI) isoform with the fetal troponin I (ssTnI) isoform renders adult cardiac contractile machinery relatively insensitive to acidification. Alignment and functional studies have determined histidine 132 of ssTnI to be the predominant source of this pH insensitivity. Substitution of histidine at the cognate position 164 in cTnI confers the same pH insensitivity to adult cardiac myocytes. An alanine at position 164 of cTnI is conserved in all mammals, with the exception of the platypus, which expresses a proline. Prolines are biophysically unique because of their innate conformational rigidity and helix-disrupting function. To provide deeper structure-function insight into the role of the TnC-TnI interface in determining contractility, we employed a live-cell approach alongside molecular dynamics simulations to ascertain the chemo-mechanical implications of the disrupted helix 4 of cTnI where position 164 exists. This important motif belongs to the critical switch region of cTnI. Substitution of a proline at position 164 of cTnI in adult rat cardiac myocytes causes increased contractility independent of alterations in the Ca2+ transient. Free-energy perturbation calculations of cTnC-Ca2+ binding indicate no difference in cTnC-Ca2+ affinity. Rather, we propose the enhanced contractility is derived from new salt bridge interactions between cTnI helix 4 and cTnC helix A, which are critical in determining pH sensitivity and contractility. Molecular dynamics simulations demonstrate that cTnI A164P structurally phenocopies ssTnI under baseline but not acidotic conditions. These findings highlight the evolutionarily directed role of the TnI-cTnC interface in determining cardiac contractility.
Copyright © 2018. Published by Elsevier Inc.

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Year:  2018        PMID: 29642034      PMCID: PMC5954295          DOI: 10.1016/j.bpj.2018.02.015

Source DB:  PubMed          Journal:  Biophys J        ISSN: 0006-3495            Impact factor:   4.033


  57 in total

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Authors:  S S Lehrer; E P Morris
Journal:  J Biol Chem       Date:  1982-07-25       Impact factor: 5.157

6.  pH-responsive titratable inotropic performance of histidine-modified cardiac troponin I.

Authors:  Nathan J Palpant; Evelyne M Houang; Yuk Y Sham; Joseph M Metzger
Journal:  Biophys J       Date:  2012-04-03       Impact factor: 4.033

7.  Increasing mammalian cardiomyocyte contractility with residues identified in trout troponin C.

Authors:  Todd E Gillis; Bo Liang; Franca Chung; Glen F Tibbits
Journal:  Physiol Genomics       Date:  2005-03-22       Impact factor: 3.107

Review 8.  Review of the monotreme fossil record and comparison of palaeontological and molecular data.

Authors:  A M Musser
Journal:  Comp Biochem Physiol A Mol Integr Physiol       Date:  2003-12       Impact factor: 2.320

9.  Effect of temperature on the structure of trout troponin C.

Authors:  Tharin M A Blumenschein; Todd E Gillis; Glen F Tibbits; Brian D Sykes
Journal:  Biochemistry       Date:  2004-05-04       Impact factor: 3.162

10.  Interaction between the regulatory domain of cardiac troponin C and the acidosis-resistant cardiac troponin I A162H.

Authors:  Sandra E Pineda-Sanabria; Ian M Robertson; Monica X Li; Brian D Sykes
Journal:  Cardiovasc Res       Date:  2012-11-25       Impact factor: 10.787

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Review 2.  Computational Studies of Cardiac and Skeletal Troponin.

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Journal:  Front Mol Biosci       Date:  2019-08-09

3.  Loss of dysferlin or myoferlin results in differential defects in excitation-contraction coupling in mouse skeletal muscle.

Authors:  David Y Barefield; Jordan J Sell; Ibrahim Tahtah; Samuel D Kearns; Elizabeth M McNally; Alexis R Demonbreun
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