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用于确定羧肽酶底物特异性的荧光共振能量转移肽的位置扫描组合文库:用人组织蛋白酶B进行检测

Positional-scanning combinatorial libraries of fluorescence resonance energy transfer peptides to define substrate specificity of carboxydipeptidases: assays with human cathepsin B.

作者信息

Cotrin Simone Silva, Puzer Luciano, de Souza Judice Wagner Alves, Juliano Luiz, Carmona Adriana K, Juliano Maria Aparecida

机构信息

Department of Biophysics, Escola Paulista de Medicina, UNIFESP, Rua Três de Maio, 100, São Paulo 04044-020, Brazil.

出版信息

Anal Biochem. 2004 Dec 15;335(2):244-52. doi: 10.1016/j.ab.2004.09.012.

Abstract

We have developed positional scanning synthetic combinatorial libraries to define the substrate specificity of carboxydipeptidases. The library Abz-GXXZXK(Dnp)-OH, where Abz is ortho-aminobenzoic acid, K(Dnp) is N(epsilon)-2,4-dinitrophenyl-lysine with free carboxyl group, the Z position was successively occupied with 1 of 19 amino acids (cysteine was omitted), and X represents randomly incorporated residues, was assayed initially with human cathepsin B, and arginine was defined as one of the best residues at the P(1) position. To examine the selectivity of S(1)('), S(2), and S(3) subsites, the sublibraries Abz-GXXRZK(Dnp)-OH, Abz-GXZRXK(Dnp)-OH, and Abz-GZXRXK(Dnp)-OH were then synthesized. The peptide Abz-GIVRAK(Dnp)-OH, which contains the most favorable residues in the P(3)-P(1)(') positions identified by screening of the libraries with cathepsin B, was hydrolyzed by this enzyme with k(cat)/K(m)=7288 mM(-1)s(-1). This peptide is the most efficient substrate described for cathepsin B to this point, and it is highly selective for the enzyme among the lysosomal cysteine proteases.

摘要

我们已开发出位置扫描合成组合文库,以确定羧肽酶的底物特异性。文库Abz-GXXZXK(Dnp)-OH中,Abz为邻氨基苯甲酸,K(Dnp)是具有游离羧基的N(ε)-2,4-二硝基苯基赖氨酸,Z位置依次被19种氨基酸中的一种占据(省略了半胱氨酸),X代表随机掺入的残基,最初用人组织蛋白酶B进行检测,精氨酸被确定为P(1)位置上最佳残基之一。为了研究S(1)'、S(2)和S(3)亚位点的选择性,随后合成了亚文库Abz-GXXRZK(Dnp)-OH、Abz-GXZRXK(Dnp)-OH和Abz-GZXRXK(Dnp)-OH。通过组织蛋白酶B筛选文库确定的在P(3)-P(1)'位置含有最有利残基的肽Abz-GIVRAK(Dnp)-OH,被该酶以k(cat)/K(m)=7288 mM(-1)s(-1)水解。该肽是目前所描述的组织蛋白酶B最有效的底物,并且在溶酶体半胱氨酸蛋白酶中对该酶具有高度选择性。

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