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尿苷二磷酸葡萄糖脱氢酶与抑制剂尿苷二磷酸木糖的相互作用。

Interactions of urdine diphosphate glucose dehydrogenase with the inhibitor urdine diphosphate xylose.

作者信息

Gainey P A, Phelps C F

出版信息

Biochem J. 1975 Feb;145(2):129-34. doi: 10.1042/bj1450129.

Abstract
  1. UDP-xylose and UDP-glucose both bind to UDP-glucose dehydrogenase in the absence of NAD+, causing an enhancement of protein fluorescence. 2. The binding of UDP-xylose is pH-dependent, tighter binding being observed at pH8.2 than at pH8.7. 3. At low protein concentrations sigmiodal profiles of fluorescence enhancement are obtained on titration of the enzyme with UDP-xylose. As the protein concentration is increased the titration profiles become progressively more hypebolic in shape. 4. The markedly different titration profiles obtained on titrating enzyme and the enzyme-NAD+ complex with UDP-xylose suggests a conformational difference between these two species 5. NAD+ lowere the apparent affinity of the enzyme for UDP-xylose. 6. There is no change in the apparent moleculare weight of UDP-glucose dehydrogenase on binging UDP-xylose. 7. Protein modification by either diethyl pyrocarbonate or 5, 5'-dithiobis-(2-nitrobenzoate) does not "desensitize" the enzyme with respect to the inhibition by UDP-xylose. 8. UDP-xylose lowers the affinity of the enzyme for NADG. 9. It is suggested that UDP-xylose is acting as a substrate analogue of UDP-glucose and causes protein-conformational changes on binding to the enzyme.
摘要
  1. 在没有烟酰胺腺嘌呤二核苷酸(NAD⁺)的情况下,尿苷二磷酸木糖(UDP - 木糖)和尿苷二磷酸葡萄糖(UDP - 葡萄糖)均与UDP - 葡萄糖脱氢酶结合,导致蛋白质荧光增强。2. UDP - 木糖的结合依赖于pH值,在pH8.2时观察到的结合比在pH8.7时更紧密。3. 在低蛋白浓度下,用UDP - 木糖滴定该酶时可获得荧光增强的S形曲线。随着蛋白质浓度的增加,滴定曲线的形状逐渐变得更加双曲线。4. 用UDP - 木糖滴定酶和酶 - NAD⁺复合物时获得的明显不同的滴定曲线表明这两种物质之间存在构象差异。5. NAD⁺降低了该酶对UDP - 木糖的表观亲和力。6. 结合UDP - 木糖后,UDP - 葡萄糖脱氢酶的表观分子量没有变化。7. 用焦碳酸二乙酯或5,5'-二硫代双(2 - 硝基苯甲酸)对蛋白质进行修饰,不会使该酶对UDP - 木糖的抑制作用“脱敏”。8. UDP - 木糖降低了该酶对NADG的亲和力。9. 有人认为,UDP - 木糖作为UDP - 葡萄糖的底物类似物,在与酶结合时会引起蛋白质构象变化。

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