Literature DB >> 1826002

Modified calcium-dependent regulatory function of troponin C central helix mutants.

Z Dobrowolski1, G Q Xu, S E Hitchcock-DeGregori.   

Abstract

Mutations have been made in the exposed region of the avian troponin C central helix, the D/E linker, which change its length and the orientation of the Ca2(+)-binding domains relative to each other. The region 87Glu-Asp-Ala-Lys-Gly-Lys-Ser-Glu-Glu-Glu97 has been altered in five deletion (d) mutants: dEDA, dKG, dKGK, dSEEE, and dKEDAKGK. The recombinant troponin Cs were expressed in Escherichia coli, purified, and assayed for function. All mutants retained basic troponin C function. They all bound Ca2+ to the low and high affinity sites, and they all were able to confer Ca2+ sensitivity on the regulated actomyosin ATPase. However, the regulatory function of all mutants except dSEEE was defective in one part of the Ca2+ switch or the other. In certain conditions dKGK and dKEDAKGK failed to inhibit fully whereas dEDA and dKG failed to activate the regulated actomyosin ATPase fully. The following general conclusions have been made. (a) The length of the D/E linker per se (assuming the linker is helical) and the orientation of the two Ca2(+)-binding domains relative to each other are not crucial for regulation. (b) The conserved charge cluster 95Glu-Glu-Glu97, in a region of troponin C known to bind to troponin I and postulated to be required for regulation, appears to be unimportant for function. (c) Deletion of 88Glu-Asp-Ala90 resulted in a troponin C that could not activate the actomyosin (or S1) ATPase over the level of actomyosin alone, thus defining a role for troponin C in this aspect of thin filament regulation. The results have been interpreted in terms of the crystallographic structure of troponin C and related to results with analogous calmodulin mutants.

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Year:  1991        PMID: 1826002

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


  10 in total

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3.  Determination of the folding of proteins as a function of denaturants, osmolytes or ligands using circular dichroism.

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4.  Role of interchain alpha-helical hydrophobic interactions in Ca2+ affinity, formation, and stability of a two-site domain in troponin C.

Authors:  O D Monera; G S Shaw; B Y Zhu; B D Sykes; C M Kay; R S Hodges
Journal:  Protein Sci       Date:  1992-07       Impact factor: 6.725

5.  Molecular and functional consequences of mutations in the central helix of cardiac troponin C.

Authors:  Nicholas Swindle; Acchia N J Albury; Belal Baroud; Maryam Burney; Svetlana B Tikunova
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6.  Interdomain orientation of cardiac troponin C characterized by paramagnetic relaxation enhancement NMR reveals a compact state.

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7.  The role of glycine (residue 89) in the central helix of EF-hand protein troponin-C exposed following amino-terminal alpha-helix deletion.

Authors:  X L Ding; A B Akella; H Su; J Gulati
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8.  Molecular and functional characterization of novel hypertrophic cardiomyopathy susceptibility mutations in TNNC1-encoded troponin C.

Authors:  Andrew P Landstrom; Michelle S Parvatiyar; Jose R Pinto; Michelle L Marquardt; J Martijn Bos; David J Tester; Steve R Ommen; James D Potter; Michael J Ackerman
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9.  Mutations in the N- and D-helices of the N-domain of troponin C affect the C-domain and regulatory function.

Authors:  L Smith; N J Greenfield; S E Hitchcock-DeGregori
Journal:  Biophys J       Date:  1999-01       Impact factor: 4.033

10.  Molecular dynamics simulations of the cardiac troponin complex performed with FRET distances as restraints.

Authors:  Jayant James Jayasundar; Jun Xing; John M Robinson; Herbert C Cheung; Wen-Ji Dong
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  10 in total

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