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配体与干酪乳杆菌MTX/R二氢叶酸还原酶结合的圆二色性研究。

Circular-dichroism studies of ligand binding to dihydrofolate reductase from Lactobacillus casei MTX/R.

作者信息

Hood K, Bayley P M, Roberts G C

出版信息

Biochem J. 1979 Feb 1;177(2):425-32. doi: 10.1042/bj1770425.

Abstract

Circular-dichroism spectra (200--450 nm) were recorded for Lactobacillus casei MTX/R dihydrofolate reductase and its complexes with substrates, inhibitors and coenzymes. These spectra are compared with those reported by others for dihydrofolate reductase from other sources. The binding of NADP+ or NADPH is associated with the perturbation of one or more aromatic amino acid residues, and there is marked enhancement of the negative c.d. band at 340 nm arising from the dihydronicotinamide chromophore of NADPH. The substrates folate and dihydrofolate give rise to substantial extrinsic c.d. bands on binding, which show a number of specific differences between enzymes from different sources. The binary complexes between the enzyme and the inhibitors methotrexate or trimethoprim also show strong c.d. bands, and these are qualitatively very similar for all dihydrofolate reductases studied so far. The ternary complexes between enzyme, NADPH and trimethoprim or methotrexate are very different from the sum of the spectra of the binary complexes. Trimethoprim leads to the disappearance of the 340 nm c.d. band of bound NADPH, whereas in the methotrexate--NADPH--enzyme ternary complex a "couplet" c.d. spectrum is observed at long wavelengths. Analysis of this latter feature suggests that it arises from a direct interaction between the dihydronicotinamide and pteridine rings in the ternary complex.

摘要

记录了干酪乳杆菌MTX/R二氢叶酸还原酶及其与底物、抑制剂和辅酶复合物的圆二色光谱(200 - 450纳米)。将这些光谱与其他来源的二氢叶酸还原酶的光谱进行了比较。NADP⁺或NADPH的结合与一个或多个芳香族氨基酸残基的扰动有关,并且NADPH的二氢烟酰胺发色团在340纳米处的负圆二色带显著增强。底物叶酸和二氢叶酸在结合时产生大量的外在圆二色带,不同来源的酶之间存在一些特定差异。酶与抑制剂甲氨蝶呤或甲氧苄啶之间的二元复合物也显示出很强的圆二色带,到目前为止,所有研究的二氢叶酸还原酶的这些带在性质上非常相似。酶、NADPH与甲氧苄啶或甲氨蝶呤之间的三元复合物与二元复合物光谱的总和非常不同。甲氧苄啶导致结合的NADPH在340纳米处的圆二色带消失,而在甲氨蝶呤 - NADPH - 酶三元复合物中,在长波长处观察到一个“偶合”圆二色光谱。对后一特征的分析表明,它源于三元复合物中二氢烟酰胺和蝶啶环之间的直接相互作用。

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