首页> 美国卫生研究院文献>Biochemical Journal >Subsite specificity (S3 S2 S1 S2 and S3) of oligopeptidase B from Trypanosoma cruzi and Trypanosoma brucei using fluorescent quenched peptides: comparative study and identification of specific carboxypeptidase activity.
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Subsite specificity (S3 S2 S1 S2 and S3) of oligopeptidase B from Trypanosoma cruzi and Trypanosoma brucei using fluorescent quenched peptides: comparative study and identification of specific carboxypeptidase activity.

机译:克鲁氏锥虫和布鲁氏锥虫的寡肽酶B的亚位特异性(S3S2S1S2和S3)使用荧光猝灭肽:比较研究和特定羧肽酶活性的鉴定。

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摘要

We characterized the extended substrate binding site of recombinant oligopeptidase B enzymes from Trypanosoma cruzi (Tc-OP) and Trypanosoma brucei (Tb-OP), evaluating the specificity of their S3, S2, S1', S2' and S3' subsites. Five series of internally quenched fluorescent peptides based on the substrate Abz-AGGRGAQ-EDDnp [where Abz is o -aminobenzoic acid and EDDnp is N -(2,4-dinitrophenyl)ethylenediamine] were designed to contain amino acid residues with side chains of a minimum size, and each residue position of this substrate was modified. Synthetic peptides of different lengths derived from the human kininogen sequence were also examined, and peptides of up to 17 amino acids were found to be hydrolysed by Tc-OP and Tb-OP. These two oligopeptidases were essentially arginyl hydrolases, since for all peptides examined the only cleavage site was the Arg-Xaa bond. We also demonstrated that Tc-OP and Tb-OP have a very specific carboxypeptidase activity for basic amino acids, which depends on the presence of at least of a pair of basic amino acids at the C-terminal end of the substrate. The peptide with triple Arg residues (Abz-AGRRRAQ-EDDnp) was an efficient substrate for Tc-OP and Tb-OP: the Arg-Ala peptide bond was cleaved first and then two C-terminal Arg residues were successively removed. The S1' subsite seems to be an important determinant of the specificity of both enzymes, showing a preference for Tyr, Ser, Thr and Gln as hydrogen donors. The presence of these amino acids at P1' resulted in substrates that were hydrolysed with K (m) values in the sub-micromolar range. Taken together, this work supports the view that oligopeptidase B is a specialized protein-processing enzyme with a specific carboxypeptidase activity. Excellent substrates were obtained for Tb-OP and Tc-OP (Abz-AMRRTISQ-EDDnp and Abz-AHKRYSHQ-EDDnp respectively), which were hydrolysed with remarkably high k (cat) and low K (m) values.
机译:我们表征了来自克鲁氏锥虫(Tc-OP)和布鲁氏锥虫(Tb-OP)的重组寡肽酶B酶的扩展底物结合位点,评估了它们的S3,S2,S1',S2'和S3'亚位点的特异性。基于底物Abz-AGGRGAQ-EDDnp [其中Abz是邻氨基苯甲酸,而EDDnp是N-(2,4-二硝基苯基)乙二胺]的五种内部淬灭的荧光肽被设计为包含带有a侧链的氨基酸残基最小尺寸,并修改该底物的每个残基位置。还检查了源自人激肽原序列的不同长度的合成肽,发现多达17个氨基酸的肽被Tc-OP和Tb-OP水解。这两个寡肽酶本质上是精氨酸水解酶,因为对于所有检查的肽,唯一的切割位点是Arg-Xaa键。我们还证明了Tc-OP和Tb-OP对碱性氨基酸具有非常特定的羧肽酶活性,这取决于底物C末端至少存在一对碱性氨基酸。具有三个Arg残基的肽(Abz-AGRRRAQ-EDDnp)是Tc-OP和Tb-OP的有效底物:首先裂解Arg-Ala肽键,然后依次去除两个C末端Arg残基。 S1'亚位点似乎是两种酶特异性的重要决定因素,显示出优先选择Tyr,Ser,Thr和Gln作为氢供体。这些氨基酸在P1'处的存在会导致底物被亚微摩尔范围内的K(m)值水解。综上所述,这项工作支持以下观点:寡肽酶B是一种具有特定羧肽酶活性的专门的蛋白质加工酶。获得了出色的Tb-OP和Tc-OP底物(分别为Abz-AMRRTISQ-EDDnp和Abz-AHKRYSHQ-EDDnp),它们分别以高k(cat)和低K(m)值水解。

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