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Probing the substrate specificity of hepatitis C virus NS3 serine protease by using synthetic peptides.

机译:通过使用合成肽探测丙型肝炎病毒NS3丝氨酸蛋白酶的底物特异性。

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摘要

We probed the substrate specificity of a recombinant noncovalent complex of the full-length hepatitis C virus (HCV) NS3 serine protease and NS4A cofactor, using a series of small synthetic peptides derived from the three trans-cleavage sites of the HCV nonstructural protein sequence. We observed a distinct cleavage site preference exhibited by the enzyme complex. The values of the turnover number (k(cat)) for the most efficient NS4A/4B, 4B/5A, and 5A/5B peptide substrates were 1.6, 11, and 8 min(-1), respectively, and the values for the corresponding Michaelis-Menten constants (Km) were 280, 160, and 16 microM, providing catalytic efficiency values (k(cat)/Km) of 92, 1,130, and 8,300 M(-1) s(-1). An alanine-scanning study for an NS5A/5B substrate (P6P4') revealed that P1 Cys and P3 Val were critical. Finally, substitutions at the scissile P1 Cys residue by homocysteine (Hcy), S-methylcysteine (Mcy), Ala, S-ethylcysteine (Ecy), Thr, Met, D-Cys, Ser, and penicillamine (Pen) produced progressively less efficient substrates, revealing a stringent stereochemical requirement for a Cys residue at this position.
机译:我们使用源自HCV非结构蛋白序列的三个反式切割位点的一系列小型合成肽,探索了全长丙型肝炎病毒(HCV)NS3丝氨酸蛋白酶和NS4A辅因子的重组非共价复合物的底物特异性。我们观察到由酶复合物表现出的独特的切割位点偏好。最有效的NS4A / 4B,4B / 5A和5A / 5B肽底物的周转数(k(cat))值分别为1.6、11和8 min(-1),而相应的Michaelis-Menten常数(Km)为280、160和16 microM,提供的催化效率值(k(cat)/ Km)为92、1,130和8,300 M(-1)s(-1)。一项针对NS5A / 5B底物(P6P4')的丙氨酸扫描研究表明,P1 Cys和P3 Val至关重要。最后,在同型半胱氨酸(Hcy),S-甲基半胱氨酸(Mcy),Ala,S-乙基半胱氨酸(Ecy),Thr,Met,D-Cys,Ser和青霉胺(Pen)处的易裂P1 Cys残基取代处产生的效率逐渐降低底物,表明在此位置对Cys残基的严格立体化学要求。

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