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Protein Sci. 2007 Jul;16(7):1257-65. doi: 10.1110/ps.062726807. Epub 2007 Jun 13.
2
The tryptophan switch: changing ligand-binding specificity from type I to type II in SH3 domains.色氨酸开关:在SH3结构域中改变配体结合特异性,从I型转变为II型。
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3
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Why the first self-binding peptide of human -Src kinase does not contain class II motif but can bind to its cognate Src homology 3 domain in class II mode?为什么人源 -Src 激酶的第一个自结合肽不含有 II 类模体,但可以以 II 类模式与它的同源 Src 同源 3 结构域结合?
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8
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Chemoselective nitration of phenols with tert-butyl nitrite in solution and on solid support.叔丁基亚硝酸盐在溶液中和固相上对酚的化学选择性硝化。
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本文引用的文献

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Distribution of separations between groups in an engineered calmodulin.工程化钙调蛋白中各组之间的分离分布。
J Fluoresc. 1991 Mar;1(1):15-22. doi: 10.1007/BF00865254.
2
3-Nitrotyrosine as a spectroscopic probe for investigating protein protein interactions.3-硝基酪氨酸作为研究蛋白质-蛋白质相互作用的光谱探针。
Protein Sci. 2006 May;15(5):976-86. doi: 10.1110/ps.051957006.
3
New approaches to high-throughput structure characterization of SH3 complexes: the example of Myosin-3 and Myosin-5 SH3 domains from S. cerevisiae.SH3复合物高通量结构表征的新方法:以酿酒酵母的肌球蛋白-3和肌球蛋白-5 SH3结构域为例
Protein Sci. 2006 Apr;15(4):795-807. doi: 10.1110/ps.051785506.
4
Specificity and versatility of SH3 and other proline-recognition domains: structural basis and implications for cellular signal transduction.SH3及其他脯氨酸识别结构域的特异性与多功能性:细胞信号转导的结构基础及意义
Biochem J. 2005 Sep 15;390(Pt 3):641-53. doi: 10.1042/BJ20050411.
5
Novel Src homology 3 domain-binding motifs identified from proteomic screen of a Pro-rich region.从富含脯氨酸区域的蛋白质组学筛选中鉴定出的新型Src同源3结构域结合基序。
Mol Cell Proteomics. 2005 Aug;4(8):1155-66. doi: 10.1074/mcp.M500108-MCP200. Epub 2005 May 31.
6
The structure of "unstructured" regions in peptides and proteins: role of the polyproline II helix in protein folding and recognition.肽和蛋白质中“非结构化”区域的结构:多聚脯氨酸II螺旋在蛋白质折叠和识别中的作用
Biopolymers. 2005;80(2-3):179-85. doi: 10.1002/bip.20227.
7
Incorporation of the fluorescent amino acid 7-azatryptophan into the core domain 1-47 of hirudin as a probe of hirudin folding and thrombin recognition.将荧光氨基酸7-氮杂色氨酸掺入水蛭素的核心结构域1-47中,作为水蛭素折叠和凝血酶识别的探针。
Protein Sci. 2004 Jun;13(6):1489-502. doi: 10.1110/ps.03542104.
8
The tryptophan switch: changing ligand-binding specificity from type I to type II in SH3 domains.色氨酸开关:在SH3结构域中改变配体结合特异性,从I型转变为II型。
J Mol Biol. 2004 Jan 9;335(2):619-29. doi: 10.1016/j.jmb.2003.10.060.
9
The relationship between conservation, thermodynamic stability, and function in the SH3 domain hydrophobic core.SH3结构域疏水核心中保守性、热力学稳定性与功能之间的关系。
J Mol Biol. 2003 Oct 24;333(3):641-55. doi: 10.1016/j.jmb.2003.08.035.
10
Negative regulation of yeast WASp by two SH3 domain-containing proteins.含两个SH3结构域的蛋白质对酵母WASp的负调控
Curr Biol. 2003 Jun 17;13(12):1000-8. doi: 10.1016/s0960-9822(03)00383-x.

邻硝基酪氨酸和对碘苯丙氨酸作为用于SH3复合物结构表征的光谱探针。

o-Nitrotyrosine and p-iodophenylalanine as spectroscopic probes for structural characterization of SH3 complexes.

作者信息

De Filippis Vincenzo, Draghi Annamaria, Frasson Roberta, Grandi Claudio, Musi Valeria, Fontana Angelo, Pastore Annalisa

机构信息

Department of Pharmaceutical Sciences, University of Padua, Italy.

出版信息

Protein Sci. 2007 Jul;16(7):1257-65. doi: 10.1110/ps.062726807. Epub 2007 Jun 13.

DOI:10.1110/ps.062726807
PMID:17567746
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2206685/
Abstract

High-throughput screening of protein-protein and protein-peptide interactions is of high interest both for biotechnological and pharmacological applications. Here, we propose the use of the noncoded amino acids o-nitrotyrosine and p-iodophenylalanine as spectroscopic probes in combination with circular dichroism and fluorescence quenching techniques (i.e., collisional quenching and resonance energy transfer) as a means to determine the peptide orientation in complexes with SH3 domains. Proline-rich peptides bind SH3 modules in two alternative orientations, according to their sequence motifs, classified as class I and class II. The method was tested on an SH3 domain from a yeast myosin that is known to recognize specifically class I peptides. We exploited the fluorescence quenching effects induced by o-nitrotyrosine and p-iodophenylalanine on the fluorescence signal of a highly conserved Trp residue, which is the signature of SH3 domains and sits directly in the binding pocket. In particular, we studied how the introduction of the two probes at different positions of the peptide sequence (i.e., N-terminally or C-terminally) influences the spectroscopic properties of the complex. This approach provides clear-cut evidence of the orientation of the binding peptide in the SH3 pocket. The chemical strategy outlined here can be easily extended to other protein modules, known to bind linear sequence motifs in a highly directional manner.

摘要

蛋白质 - 蛋白质和蛋白质 - 肽相互作用的高通量筛选在生物技术和药理学应用中都备受关注。在此,我们提议使用非编码氨基酸邻硝基酪氨酸和对碘苯丙氨酸作为光谱探针,结合圆二色性和荧光猝灭技术(即碰撞猝灭和共振能量转移),以此来确定与SH3结构域形成复合物时肽的取向。富含脯氨酸的肽根据其序列基序以两种不同取向结合SH3模块,分为I类和II类。该方法在已知能特异性识别I类肽的酵母肌球蛋白的SH3结构域上进行了测试。我们利用邻硝基酪氨酸和对碘苯丙氨酸对高度保守的色氨酸残基荧光信号的荧光猝灭效应,该色氨酸残基是SH3结构域的特征,直接位于结合口袋中。特别是,我们研究了在肽序列的不同位置(即N端或C端)引入这两种探针如何影响复合物的光谱性质。这种方法为结合肽在SH3口袋中的取向提供了明确的证据。这里概述的化学策略可以很容易地扩展到其他已知以高度定向方式结合线性序列基序的蛋白质模块。