4.5 Article

Single amino acid substitutions define isoform-specific effects of troponin I on myofilament Ca2+ and pH sensitivity

Journal

JOURNAL OF MOLECULAR AND CELLULAR CARDIOLOGY
Volume 43, Issue 2, Pages 107-118

Publisher

ELSEVIER SCI LTD
DOI: 10.1016/j.yjmcc.2007.05.017

Keywords

troponin I; heart; myocyte; Ca2+ sensitivity; contractility

Funding

  1. NHLBI NIH HHS [R01 HL067254, HL59301, R01 HL067254-01A1, HL67254, R01 HL059301, R01 HL059301-06] Funding Source: Medline
  2. NIDDK NIH HHS [P60 DK020572, 5P60 DK20572] Funding Source: Medline

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Troponin I isoforms play a key role in determining myofilament Ca2+ sensitivity in cardiac muscle. The goal here was to identify domain clusters and residues that confer troponin I isoform-specific myofilament Ca2+ and pH sensitivities of contraction. Key domains/residues that contribute to troponin I isoform-specific Ca2+ and pH sensitivity were studied using gene transfer of a slow skeletal troponin I (ssTnI) template, with targeted cardiac troponin I (cTnI) residue substitutions. Substitutions in ssTnI with cognate cTnI residues R125 (Q) under bar, H132 (A) under bar, and V134 (E) under bar, studied both independently and together (ssTnIQAE), resulted in efficient stoichiometric replacement of endogenous myofilament cTnI in adult cardiac myocytes. In permeabilized myocytes, the pCa(50) of tension ([Ca2+] required for half maximal force), and the acidosis-induced rightward shift of pCa50 were converted to the cTnI phenotype in myocytes expressing ssTnIQAE or ssTnIH132A, and there was no functionally additive effect of ssTnIQAE versus ssTnIH132A. Interestingly, only the acidosis-induced shift in Ca2+ sensitivity was comparable to cTnI in myocytes expressing ssTnIV134E, while ssTnIR125Q fully retained the ssTnI phenotype. An additional ssTnIN141H substitution, which lies within the same structural region of TnI as V 134, produced a shift in myofilament Ca2+ sensitivity comparable to cTnI at physiological pH, while the acidic pH response was similar to the effect of wild-type ssTnl. Analysis of sarcomere shortening in intact adult cardiac myocytes was consistent with the force measurements. Targeted substitutions in the carboxyl portion of TnI produced residue-specific influences on myofilament Ca2+ and pH sensitivity of force and give new molecular insights into the TnI isoform dependence of myofilament function. Published by Elsevier Inc.

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