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对含有单个钙结合位点的肌钙蛋白-C肽片段的质子磁共振研究。

Proton magnetic resonance studies on peptide fragments of troponin-C containing single calcium-binding sites.

作者信息

Leavis P C, Evans J S, Levine B A

出版信息

J Inorg Biochem. 1982 Jul;16(4):257-77. doi: 10.1016/s0162-0134(00)80264-0.

DOI:10.1016/s0162-0134(00)80264-0
PMID:7119770
Abstract

Proton magnetic resonance spectroscopy has been employed to study the solution conformation of three cleavage fragments of troponin-C, each containing a single Ca(II)-binding site and corresponding to different regions in the primary sequence; viz. CB8 (residues 46-77), CB9 (residues 85-134) and TH2 (residues 121-159). Although all three peptides lack a well-defined tertiary fold in the absence of metal ions, several spectral features indicate the presence of local conformational constraints in each apo-peptide. Ca(II) binding led to spectral changes consistent with increased restriction of backbone motility and the adoption of a more compact conformation. Studies using paramagnetic ions as conformational probes support current views concerning the nature of the ligands at the metal binding sites. The nature and kinetics of the structural influence of metal binding suggest that the conformational constraints existing in the CB8 apo-peptide provide an adequate Ca(II)-binding configuration. In contrast, the CB9 and TH2 peptides exhibit spectral changes consistent with an increased local structure in the region of helix E (residues 94-102) in the case of CB9 and helix H (residues 148-159) in the case of TH2. In CB9, conformation changes also appear to be transmitted to a portion of the sequence (residues 87-93) preceding helix E, a putative site of interaction between troponin-C and troponin-I. These data are discussed with reference to the contribution of long-range (interdomain) interactions within troponin-C and the modulation of troponin subunit protein-protein interactions by Ca(II) binding.

摘要

质子磁共振波谱已被用于研究肌钙蛋白C的三个裂解片段的溶液构象,每个片段都含有一个单一的Ca(II)结合位点,并且对应于一级序列中的不同区域;即CB8(残基46 - 77)、CB9(残基85 - 134)和TH2(残基121 - 159)。尽管在没有金属离子的情况下,所有这三个肽都缺乏明确的三级折叠,但几个光谱特征表明每个脱辅基肽中存在局部构象限制。Ca(II)结合导致光谱变化,这与主链运动性的限制增加以及采用更紧凑的构象一致。使用顺磁离子作为构象探针的研究支持了关于金属结合位点处配体性质的当前观点。金属结合的结构影响的性质和动力学表明,CB8脱辅基肽中存在的构象限制提供了一种合适的Ca(II)结合构型。相比之下,CB9和TH2肽表现出的光谱变化与CB9中螺旋E区域(残基94 - 102)以及TH2中螺旋H区域(残基148 - 159)的局部结构增加一致。在CB9中,构象变化似乎也传递到了螺旋E之前的一部分序列(残基87 - 93),这是肌钙蛋白C和肌钙蛋白I之间假定的相互作用位点。本文结合肌钙蛋白C内长程(结构域间)相互作用的贡献以及Ca(II)结合对肌钙蛋白亚基蛋白质 - 蛋白质相互作用的调节对这些数据进行了讨论。

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引用本文的文献

1
Molecular mechanism of troponin-C function.肌钙蛋白C功能的分子机制。
J Muscle Res Cell Motil. 1992 Aug;13(4):383-93. doi: 10.1007/BF01738034.