Literature DB >> 19369252

Förster resonance energy transfer structural kinetic studies of cardiac thin filament deactivation.

Jun Xing1, Jayant J Jayasundar, Yexin Ouyang, Wen-Ji Dong.   

Abstract

Cardiac thin filament deactivation is initiated by Ca2+ dissociation from troponin C (cTnC), followed by multiple structural changes of thin filament proteins. These structural transitions are the molecular basis underlying the thin filament regulation of cardiac relaxation, but the detailed mechanism remains elusive. In this study Förster resonance energy transfer (FRET) was used to investigate the dynamics and kinetics of the Ca2+-induced conformational changes of the cardiac thin filaments, specifically the closing of the cTnC N-domain, the cTnC-cTnI (troponin I) interaction, and the cTnI-actin interaction. The cTnC N-domain conformational change was examined by monitoring FRET between a donor (AEDANS) attached to one cysteine residue and an acceptor (DDPM) attached the other cysteine of the mutant cTnC(L13C/N51C). The cTnC-cTnI interaction was investigated by monitoring the distance changes from residue 89 of cTnC to residues 151 and 167 of cTnI, respectively. The cTnI-actin interaction was investigated by monitoring the distance changes from residues 151 and 167 of cTnI to residue 374 of actin. FRET Ca2+ titrations and stopped-flow kinetic measurements show that different thin filament structural transitions have different Ca2+ sensitivities and Ca2+ dissociation-induced kinetics. The observed structural transitions involving the regulatory region and the mobile domain of cTnI occurred at fast kinetic rates, whereas the kinetics of the structural transitions involving the cTnI inhibitory region was slow. Our results suggest that the thin filament deactivation upon Ca2+ dissociation is a two-step process. One step involves rapid binding of the mobile domain of cTnI to actin, which is kinetically coupled with the conformational change of the N-domain of cTnC and the dissociation of the regulatory region of cTnI from cTnC. The other step involves switching the inhibitory region of cTnI from interacting with cTnC to interacting with actin. The latter processes may play a key role in regulating cross-bridge kinetics.

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Year:  2009        PMID: 19369252      PMCID: PMC2713534          DOI: 10.1074/jbc.M808075200

Source DB:  PubMed          Journal:  J Biol Chem        ISSN: 0021-9258            Impact factor:   5.157


  39 in total

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Authors:  T Kobayashi; M Kobayashi; Z Gryczynski; J R Lakowicz; J H Collins
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4.  Structural studies of interactions between cardiac troponin I and actin in regulated thin filament using Förster resonance energy transfer.

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Authors:  S Ebashi; M Endo; I Otsuki
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6.  Conformation of the regulatory domain of cardiac muscle troponin C in its complex with cardiac troponin I.

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Authors:  W J Dong; J Xing; J M Robinson; H C Cheung
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Journal:  Am J Physiol Regul Integr Comp Physiol       Date:  2006-11-02       Impact factor: 3.619
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  23 in total

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5.  Structural dynamics of C-domain of cardiac troponin I protein in reconstituted thin filament.

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Journal:  J Biol Chem       Date:  2011-12-28       Impact factor: 5.157

6.  Dynamic Equilibrium of Cardiac Troponin C's Hydrophobic Cleft and Its Modulation by Ca2+ Sensitizers and a Ca2+ Sensitivity Blunting Phosphomimic, cTnT(T204E).

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7.  Structural and kinetic effects of PAK3 phosphorylation mimic of cTnI(S151E) on the cTnC-cTnI interaction in the cardiac thin filament.

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8.  Structural and kinetic effects of hypertrophic cardiomyopathy related mutations R146G/Q and R163W on the regulatory switching activity of rat cardiac troponin I.

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