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来自红螺菌和结核分枝杆菌的转氢酶杂交体催化快速的氢化物转移,但不催化完整的质子转运反应。

A hybrid of the transhydrogenases from Rhodospirillum rubrum and Mycobacterium tuberculosis catalyses rapid hydride transfer but not the complete, proton-translocating reaction.

作者信息

Wilson Rosalind, Obiozo U Mirian, Quirk Philip G, Besra Gurdyal Singh, Jackson J Baz

机构信息

School of Biosciences, University of Birmingham, Edgbaston, Birmingham, B15 2TT, UK.

出版信息

Biochim Biophys Acta. 2006 Mar;1757(3):215-23. doi: 10.1016/j.bbabio.2006.03.004. Epub 2006 Mar 31.

Abstract

All transhydrogenases appear to have three components: dI, which binds NAD(H), and dIII, which binds NADP(H), protrude from the membrane, and dII spans the membrane. However, the polypeptide composition of the enzymes varies amongst species. The transhydrogenases of Mycobacterium tuberculosis and of Rhodospirillum rubrum have three polypeptides. Sequence analysis indicates that an ancestral three-polypeptide enzyme evolved into transhydrogenases with either two polypeptides (such as the Escherichia coli enzyme) or one polypeptide (such as the mitochondrial enzyme). The fusion steps in each case probably led to the development of an additional transmembrane helix. A hybrid transhydrogenase was constructed from the dI component of the M. tuberculosis enzyme and the dII and dIII components of the R. rubrum enzyme. The hybrid catalyses cyclic transhydrogenation but not the proton-translocating, reverse reaction. This shows that nucleotide-binding/release at the NAD(H) site, and hydride transfer, are fully functional but that events associated with NADP(H) binding/release are compromised. It is concluded that sequence mismatch in the hybrid prevents a conformational change between dI and dIII which is essential for the step accompanying proton translocation.

摘要

所有的转氢酶似乎都有三个组分

结合NAD(H)的dI和结合NADP(H)的dIII从膜中伸出,而dII跨膜。然而,这些酶的多肽组成在不同物种之间有所不同。结核分枝杆菌和红螺菌的转氢酶有三种多肽。序列分析表明,一种原始的三多肽酶进化成了具有两种多肽(如大肠杆菌的酶)或一种多肽(如线粒体的酶)的转氢酶。每种情况下的融合步骤可能导致了一个额外跨膜螺旋的形成。构建了一种由结核分枝杆菌酶的dI组分和红螺菌酶的dII及dIII组分组成的杂合转氢酶。该杂合体催化循环转氢作用,但不催化质子转运的逆向反应。这表明NAD(H)位点的核苷酸结合/释放以及氢化物转移功能完全正常,但与NADP(H)结合/释放相关的事件受到了损害。得出的结论是,杂合体中的序列错配阻止了dI和dIII之间的构象变化,而这种变化对于质子转运所伴随的步骤至关重要。

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