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S100B结合表位TRTK-12的特异性及锌离子增强作用

Specificity and Zn2+ enhancement of the S100B binding epitope TRTK-12.

作者信息

Barber K R, McClintock K A, Jamieson G A, Dimlich R V, Shaw G S

机构信息

Department of Biochemistry and McLaughlin Macromolecular Structure Facility, University of Western Ontario, London, Ontario N6A 5C1, Canada.

出版信息

J Biol Chem. 1999 Jan 15;274(3):1502-8. doi: 10.1074/jbc.274.3.1502.

Abstract

The calcium-binding protein S100B (an S100 dimer composed of two S100beta monomers) is proposed to act as a calcium-sensory protein through interactions with a variety of proteins. While the nature of the exact targets for S100B has yet to be defined, random bacteriophage peptide mapping experiments have elucidated a calcium-sensitive "epitope" (TRTK-12) for S100B recognition. In this work, interactions of TRTK-12 with S100B have been shown to be calcium-sensitive. In addition, the interactions are enhanced by zinc binding to S100B, resulting in an approximate 5-fold decrease in the TRTK-12/S100B dissociation constant. Moreover, Zn2+ binding alone has little effect. TRTK-12 showed little evidence for binding to another S100 protein, S100A11 or to a peptide derived from the N terminus of S100B, indicating both a level of specificity for TRTK-12 recognition by S100B and that the N-terminal region of S100B is probably not involved in protein-protein interactions. NMR spectroscopy revealed residues most responsive to TRTK-12 binding that could be mapped to the surface of the three-dimensional structure of calcium-saturated S100B, revealing a common region indicative of a binding site.

摘要

钙结合蛋白S100B(一种由两个S100β单体组成的S100二聚体)被认为通过与多种蛋白质相互作用而作为一种钙传感蛋白。虽然S100B的确切靶标的性质尚未确定,但随机噬菌体肽图谱实验已经阐明了一个用于S100B识别的钙敏感“表位”(TRTK-12)。在这项工作中,TRTK-12与S100B的相互作用已被证明是钙敏感的。此外,锌与S100B结合可增强这种相互作用,导致TRTK-12/S100B解离常数降低约5倍。而且,单独的Zn2+结合几乎没有影响。TRTK-12几乎没有显示出与另一种S100蛋白S100A11或源自S100B N端的肽结合的证据,这表明S100B对TRTK-12识别具有一定程度的特异性,并且S100B的N端区域可能不参与蛋白质-蛋白质相互作用。核磁共振光谱揭示了对TRTK-12结合最敏感的残基,这些残基可以定位到钙饱和S100B三维结构的表面,揭示了一个指示结合位点的共同区域。

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