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铁氧还蛋白:铁氧还蛋白-NADP⁺还原酶电子转移复合物:结构相互作用的进化优化

Fd : FNR Electron Transfer Complexes: Evolutionary Refinement of Structural Interactions.

作者信息

Hanke Guy T, Kurisu Genji, Kusunoki Masami, Hase Toshiharu

机构信息

Division of Enzymology, Institute for Protein Research, Osaka University, Suita, Osaka, 565-0871, Japan,

出版信息

Photosynth Res. 2004;81(3):317-27. doi: 10.1023/B:PRES.0000036885.01534.b8.

Abstract

During the evolution of higher-plant root and leaf-type-specific Fd : FNR complexes from an original cyanobacterial type progenitor, rearrangement of molecular interaction has altered the relative orientation of prosthetic groups and there have been changes in complex induced conformational change. Selection has presumably worked on mutation of residues responsible for interaction between the two proteins, favoring optimized electron flow in a specific direction, and efficient dissociation following specific oxidation of leaf Fd and reduction of root Fd. Major changes appear to be: loss in both leaf and root complexes of a cyanobacterial mechanism that ensures Fd dissociation from the complex following change in Fd redox state, development of a structural rearrangement of Fd on binding to leaf FNR that results in a negative shift in Fd redox potential favorable to photosynthetic electron flow, creation of a vacant space in the root Fd:FNR complex that may allow access to the redox centers of other enzymes to ensure efficient channeling of heterotrophic reductant into bioassimilation. Further structural analysis is essential to establish how root type FNR distinguishes between Fd isoforms, and discover how residues not directly involved in intermolecular interactions may affect complex formation.

摘要

在高等植物根和叶型特异性铁氧还蛋白

铁氧还蛋白-NADP+还原酶(Fd:FNR)复合物从原始蓝细菌型祖先进化而来的过程中,分子相互作用的重排改变了辅基的相对取向,并且复合物诱导的构象变化也发生了改变。选择可能作用于负责两种蛋白质之间相互作用的残基突变,有利于在特定方向上优化电子流,以及在叶铁氧还蛋白特异性氧化和根铁氧还蛋白还原后有效解离。主要变化似乎包括:叶和根复合物中丧失了一种蓝细菌机制,该机制可确保在铁氧还蛋白氧化还原状态改变后铁氧还蛋白从复合物中解离;铁氧还蛋白与叶铁氧还蛋白-NADP+还原酶结合时发生结构重排,导致铁氧还蛋白氧化还原电位负移,有利于光合电子流;在根铁氧还蛋白:铁氧还蛋白-NADP+还原酶复合物中产生一个空位,这可能允许其他酶的氧化还原中心进入,以确保异养还原剂有效导入生物同化过程。进一步的结构分析对于确定根型铁氧还蛋白-NADP+还原酶如何区分铁氧还蛋白同工型,以及发现不直接参与分子间相互作用的残基如何影响复合物形成至关重要。

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