Pinheiro T J, Venning J D, Jackson J B
Department of Biological Sciences, University of Warwick, Coventry CV4 7AL, United Kingdom.
J Biol Chem. 2001 Nov 30;276(48):44757-61. doi: 10.1074/jbc.M109227200. Epub 2001 Sep 27.
Transhydrogenase couples the redox reaction between NAD(H) and NADP(H) to proton translocation across a membrane. Coupling is achieved through changes in protein conformation. Upon mixing, the isolated nucleotide-binding components of transhydrogenase (dI, which binds NAD(H), and dIII, which binds NADP(H)) form a catalytic dI(2).dIII(1) complex, the structure of which was recently solved by x-ray crystallography. The fluorescence from an engineered Trp in dIII changes when bound NADP(+) is reduced. Using a continuous flow device, we have measured the Trp fluorescence change when dI(2).dIII(1) complexes catalyze reduction of NADP(+) by NADH on a sub-millisecond scale. At elevated NADH concentrations, the first-order rate constant of the reaction approaches 21,200 s(-1), which is larger than that measured for redox reactions of nicotinamide nucleotides in other, soluble enzymes. Rather high concentrations of NADH are required to saturate the reaction. The deuterium isotope effect is small. Comparison with the rate of the reverse reaction (oxidation of NADPH by NAD(+)) reveals that the equilibrium constant for the redox reaction on the complex is >36. This high value might be important in ensuring high turnover rates in the intact enzyme.
转氢酶将NAD(H)和NADP(H)之间的氧化还原反应与质子跨膜转运偶联起来。偶联是通过蛋白质构象的变化实现的。混合后,转氢酶的分离核苷酸结合组分(结合NAD(H)的dI和结合NADP(H)的dIII)形成催化性dI(2).dIII(1)复合物,其结构最近通过X射线晶体学解析出来。当结合的NADP(+)被还原时,dIII中工程化色氨酸的荧光会发生变化。使用连续流动装置,我们在亚毫秒尺度上测量了dI(2).dIII(1)复合物催化NADH还原NADP(+)时色氨酸荧光的变化。在较高的NADH浓度下,反应的一级速率常数接近21200 s(-1),这比在其他可溶性酶中烟酰胺核苷酸的氧化还原反应所测得的速率常数要大。需要相当高浓度的NADH才能使反应饱和。氘同位素效应较小。与逆反应(NAD(+)氧化NADPH)的速率比较表明,复合物上氧化还原反应的平衡常数>36。这个高值可能对确保完整酶中的高周转率很重要。
