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>Evaluation of hydrogen-bonding and enantiomeric P2-S2 hydrophobic contacts in dynamic aspects of molecular recognition by papain
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Evaluation of hydrogen-bonding and enantiomeric P2-S2 hydrophobic contacts in dynamic aspects of molecular recognition by papain
p1. 2-(N′-Acetyl-D-phenylalanyl)hydroxyethyl 2′-pyridyl disulphide (compound IV) (m.p. 59 degrees C; [alpha]D20 -6.6 degrees (c 1.2 in methanol)) was synthesized. 2. The results of a study of the pH-dependence of the second-order rate constant (k) for its reaction with the catalytic-site thiol group (Cys-25) of papain (EC 3.4.22.2) together with analogous kinetic data for the reactions of related time-dependent inhibitors, notably the L-enantiomer of compound (IV) (compound III) and the L- and D-enantiomers of 2-(N′-acetylphenylalanylamino)ethyl 2′-pyridyl disulphide (compounds I and II respectively), were used to assess the contributions of the (P1)-NH ... O = C & (Asp-158) and (P2) & C = O ... H-N-(Gly-66) hydrogen bonds and enantiomeric P2-S2 hydrophobic contacts in two manifestations of dynamic molecular recognition in papain-ligand association: (a) signalling to the catalytic-site region to provide for a (His-159)-IM(+)-H-assisted transition state and (b) the dependence of P2-S2 stereoselectivity on hydrogen-bonding interactions outside the S2 subsite. The analysis involved determination of the reactivities of individual ionization states of the reactions (pH-independent rate constants, k) and associated macroscopic pKa values and difference kinetic specificity energies (delta delta GKS = -RT1n(k1/k2), where k1 is the pH-independent second-order rate constant for reaction with one inhibitor and k2 is the analogous rate constant in the same ionization state for reaction with another inhibitor so that, when the structural change provides that k2 & k1, delta delta GKS is positive. 3. The kinetic data further illuminate the nature of the interdependence of binding interactions in papain first noted by Kowlessur, Topham, Thomas, O9Driscoll, Templeton & Brocklehurst [(1989) Biochem. J. 258, 755-764] in the S2 subsite, S1-S2 intersubsite and catalytic-site regions. Of particular note is the apparent dependence of the binding of the N-Ac-D-Phe moiety on the binding of the leaving group to (His-159)-Im+H and the fact that the resulting rate enhancement is more effective when (P1)-N-H is absent than when it is present. This result revealed by kinetic analysis goes beyond the conclusion suggested by model building that it is possible to make all of the binding contacts in complexes involving the D-enantiomers [(II) and (IV)] as in those involving the L-enantiomers [(I) and (III)].(ABSTRACT TRUNCATED AT 400 WORDS)/p
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机译:> 1。合成了2-(N'-乙酰基-D-苯丙氨酰基)羟乙基2'-吡啶基二硫化物(化合物IV)(熔点59℃;αD20-6.6℃(在甲醇中为c 1.2))。 2.研究第二速率常数(k)与木瓜蛋白酶催化位点巯基(Cys-25)反应的pH依赖性(EC 3.4.22.2)的结果以及类似的动力学数据对于相关的时间依赖性抑制剂的反应,尤其是化合物(IV)的L对映体(化合物III)和2-(N'-乙酰苯基丙氨酰氨基)乙基2'-吡啶基二硫化物的L和D对映体(化合物I分别用于评估(P1)-NH的贡献。 (Asp-158)和(P2) C = O ... HN-(Gly-66)氢键和对映体P2-S2疏水性接触,在木瓜蛋白酶-配体缔合中动态分子识别的两种表现形式:(a)信号传递至催化位点区域,以提供( His-159)-IM(+)-H辅助的过渡态和(b)P2-S2立体选择性对S2子位点外部氢键相互作用的依赖性。该分析涉及确定反应的各个电离状态的反应性(与pH无关的速率常数,k)以及相关的宏观pKa值和不同的动力学比能(δdelta GKS = -RT1n(k1 / k2),其中k1为与一种抑制剂的反应与pH无关的二级速率常数和k 2与在与另一种抑制剂反应的相同电离态下的相似速率常数类似,因此,当结构变化使得k 2> k 1时,δ-δGKS为正。 3.动力学数据进一步阐明了木瓜蛋白酶中的结合相互作用的相互依赖性的性质,首先由Kowlessur,Topham,Thomas,O9Driscoll,Templeton& Brocklehurst [(1989)Biochem。J. 258,755-764]注意到。 ,特别是值得注意的是,N-Ac-D-Phe部分的结合明显依赖于离去基团与(His-159)-Im + H和事实上,结果(P1)-N-H不存在时,速率增强比存在时更有效。动力学分析揭示的结果超出了模型构建所建议的结论,即与涉及L-对映体[[II]和(IV)]的复合物中的所有结合接触都是可能的。 (I)和(III)]。(摘要截断了400个单词)
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