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牛脑腺苷脱氨酶活性位点的功能残基。

Functional residues at the active site of bovine brain adenosine deaminase.

作者信息

Lupidi G, Marmocchi F, Venardi G, Cristalli G

机构信息

Dept. of Biology M.C.A., University of Camerino, Italy.

出版信息

Biochem Mol Biol Int. 1997 Dec;43(6):1339-52. doi: 10.1080/15216549700205161.

Abstract

Brain adenosine deaminase was investigated in order to identify amino acid residues essential for its catalytic activity. The pH dependence of log Vmax shows that the enzyme activity depends on two ionizing groups with pK values of 5.4, that must be unprotonated, and 8.4, that must be protonated, for the catalysis. These same groups are observed in the Vmax/Km profiles. The plausible role of histidine residues at the active site of brain adenosine deaminase was proved by chemical modification with (DEP). The histidine specific reagent inactivated the enzyme following a pseudo first-order kinetics with a second-order rate constant of 8.9 10(-3) (+/- 1.8 10(-3)) M-1 min-1. The inhibition of the enzyme with PCMBS was studied monitoring the enzyme activity after incubation with the inhibitor. Brain adenosine deaminase exhibited a characteristic intrinsic tryptophan fluorescence with an emission peak centered at 335 nm. Stern-Volmer quenching parameters in the presence of acrylamide and iodide indicated that tryptophan residues are buried in the native molecule. Tryptophan residues also showed a high heterogeneity that was increased after binding of ground- and transition-state analogs to the enzyme.

摘要

为了确定对其催化活性至关重要的氨基酸残基,对脑腺苷脱氨酶进行了研究。log Vmax对pH的依赖性表明,酶活性取决于两个电离基团,催化时pK值分别为5.4(必须未质子化)和8.4(必须质子化)。在Vmax/Km曲线中也观察到了这些相同的基团。通过用(DEP)进行化学修饰,证明了脑腺苷脱氨酶活性位点处组氨酸残基的可能作用。组氨酸特异性试剂使酶失活,遵循假一级动力学,二级速率常数为8.9×10⁻³(±1.8×10⁻³)M⁻¹ min⁻¹。在用PCMBS抑制该酶时,通过监测与抑制剂孵育后的酶活性进行了研究。脑腺苷脱氨酶表现出特征性的内在色氨酸荧光,发射峰位于335 nm处。在丙烯酰胺和碘化物存在下的Stern-Volmer猝灭参数表明,色氨酸残基埋藏在天然分子中。色氨酸残基也表现出高度的异质性,在底物和过渡态类似物与酶结合后这种异质性增加。

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