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Calretinin and calbindin D28k have different domain organizations.钙结合蛋白和钙结合蛋白D28k具有不同的结构域组织。
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The EF-hand Ca(2+)-binding protein p22 associates with microtubules in an N-myristoylation-dependent manner.EF 手型钙离子结合蛋白 p22 以 N-肉豆蔻酰化依赖的方式与微管结合。
Mol Biol Cell. 1999 Oct;10(10):3473-88. doi: 10.1091/mbc.10.10.3473.

本文引用的文献

1
S-100 (alpha and beta) binding peptide (TRTK-12) blocks S-100/GFAP interaction: identification of a putative S-100 target epitope within the head domain of GFAP.S-100(α和β)结合肽(TRTK-12)阻断S-100/GFAP相互作用:在GFAP头部结构域内鉴定一个假定的S-100靶表位。
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2
The solution structure of the bovine S100B protein dimer in the calcium-free state.无钙状态下牛S100B蛋白二聚体的溶液结构。
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3
Solution structure of rat apo-S100B(beta beta) as determined by NMR spectroscopy.通过核磁共振光谱法测定的大鼠载脂蛋白-S100B(ββ)的溶液结构。
Biochemistry. 1996 Sep 10;35(36):11577-88. doi: 10.1021/bi9612226.
4
The CD4 determinant for downregulation by HIV-1 Nef directly binds to Nef. Mapping of the Nef binding surface by NMR.HIV-1 Nef介导下调作用的CD4决定簇直接与Nef结合。通过核磁共振对Nef结合表面进行图谱分析。
Biochemistry. 1996 Aug 13;35(32):10256-61. doi: 10.1021/bi9611164.
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The S100 family of EF-hand calcium-binding proteins: functions and pathology.EF 手型钙结合蛋白的 S100 家族:功能与病理学
Trends Biochem Sci. 1996 Apr;21(4):134-40. doi: 10.1016/s0968-0004(96)80167-8.
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NMR analysis of interacting soluble forms of the cell-cell recognition molecules CD2 and CD48.细胞间识别分子CD2和CD48相互作用可溶性形式的核磁共振分析。
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Ca2+/S100 regulation of giant protein kinases.巨蛋白激酶的钙离子/ S100调节
Nature. 1996 Apr 18;380(6575):636-9. doi: 10.1038/380636a0.
8
Identification of a chemotactic domain of the pro-inflammatory S100 protein CP-10.促炎S100蛋白CP-10趋化结构域的鉴定。
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9
Identification of an S100 target protein: glycogen phosphorylase.一种S100靶蛋白的鉴定:糖原磷酸化酶。
Cell Calcium. 1993 Apr;14(4):323-32. doi: 10.1016/0143-4160(93)90053-9.
10
Binding site of annexin XI on the calcyclin molecule.膜联蛋白XI在钙调蛋白分子上的结合位点。
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确定肌动蛋白封端蛋白CapZ在S100B蛋白上的结合位点。

Identification of the binding site on S100B protein for the actin capping protein CapZ.

作者信息

Kilby P M, Van Eldik L J, Roberts G C

机构信息

Department of Biochemistry and Biological NMR Centre, University of Leicester, United Kingdom.

出版信息

Protein Sci. 1997 Dec;6(12):2494-503. doi: 10.1002/pro.5560061202.

DOI:10.1002/pro.5560061202
PMID:9416599
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2143613/
Abstract

The calcium-binding protein S100B binds to several potential target proteins, but there is no detailed information showing the location of the binding site for any target protein on S100B. We have made backbone assignments of the calcium-bound form of S100B and used chemical-shift changes in spectra of 15N-labeled protein to locate the site that binds a peptide corresponding to residues 265-276 from CapZ alpha, the actin capping protein. The largest chemical-shift changes are observed for resonances arising from residues around the C terminus of the C-terminal helix of S100B and residues Val-8 to Asp-12 of the N-terminal helix. These residues are close to but not identical to residues that have been identified by mutational analysis to be important in other S100 protein-protein interactions. They make up a patch across the S100B dimer interface and include some residues that are quite buried in the structure of calcium-free S100B. We believe we may have identified a binding site that could be common to many S100 protein-protein interactions.

摘要

钙结合蛋白S100B可与多种潜在的靶蛋白结合,但尚无详细信息表明任何靶蛋白在S100B上的结合位点位置。我们已对钙结合形式的S100B进行了主链归属,并利用15N标记蛋白光谱中的化学位移变化来定位与肌动蛋白封端蛋白CapZα的265 - 276位残基对应的肽段的结合位点。在S100B C末端螺旋C末端附近的残基以及N末端螺旋的Val - 8至Asp - 12残基产生的共振中观察到最大的化学位移变化。这些残基与通过突变分析确定在其他S100蛋白 - 蛋白相互作用中重要的残基相近但不相同。它们构成了跨越S100B二聚体界面的一个区域,并且包括一些在无钙S100B结构中相当隐蔽的残基。我们认为我们可能已经确定了一个可能为许多S100蛋白 - 蛋白相互作用所共有的结合位点。