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Defining SH2 domain and PTP specificity by screening combinatorial peptide libraries

机译:通过筛选组合肽库定义SH2结构域和PTP特异性

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摘要

Src homology 2 (SH2) domains mediate protein-protein interactions by recognizing short phosphotyrosyl (pY) peptide motifs in their partner proteins. Protein tyrosine phosphatases (PTPs) catalyze the dephosphorylation of pY proteins, counteracting the protein tyrosine kinases. Both types of proteins exhibit primary sequence specificity, which plays at least a partial role in dictating their physiological interacting partners or substrates. A combinatorial peptide library method has been developed to systematically assess the sequence specificity of SH2 domains and PTPs. A “one-bead-one-compound” pY peptide library is synthesized on 90-μm TenteGel beads and screened against an SH2 domain or PTP of interest for binding or catalysis. The beads that carry the tightest binding sequences against the SH2 domain or the most efficient substrates of the PTP are selected by an enzyme-linked assay and individually sequenced by a partial Edman degradation/mass spectrometry technique. The combinatorial method has been applied to determine the sequence specificity of 8 SH2 domains from Src and Csk kinases, adaptor protein Grb2, and phosphatases SHP-1, SHP-2, and SHIP1 and a prototypical PTP, PTP1B.
机译:Src同源2(SH2)域通过识别其伴侣蛋白中的短磷酸酪氨酰(pY)肽基序来介导蛋白-蛋白相互作用。蛋白质酪氨酸磷酸酶(PTP)催化pY蛋白质的去磷酸化,抵消了蛋白质酪氨酸激酶。两种类型的蛋白质均显示一级序列特异性,其在决定其生理相互作用伴侣或底物方面起至少部分作用。已经开发了组合肽库方法来系统地评估SH2域和PTP的序列特异性。在90-μmTenteGel珠上合成“单珠一化合物” pY肽文库,并针对感兴趣的SH2域或PTP进行结合或催化筛选。通过酶联测定选择带有针对SH2结构域或PTP最有效底物的最紧密结合序列的珠子,并通过部分Edman降解/质谱技术分别测序。组合方法已应用于确定Src和Csk激酶,衔接蛋白Grb2和磷酸酶SHP-1,SHP-2和SHIP1以及原型PTP PTP1B的8个SH2域的序列特异性。

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