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光合放氧复合体的锰结合蛋白

Manganese-binding proteins of the oxygen-evolving complex.

作者信息

Mei R, Green J P, Sayre R T, Frasch W D

机构信息

Department of Biology, University of Michigan, Ann Arbor 48109-1048.

出版信息

Biochemistry. 1989 Jun 27;28(13):5560-7. doi: 10.1021/bi00439a033.

DOI:10.1021/bi00439a033
PMID:2673350
Abstract

The extrinsic 33-kDa protein (P33) was cross-linked covalently to the binding site on P33-depleted PSII preparations which is responsible for reconstitution of photosynthetic water oxidation after PSII preparations have been washed with 1 M CaCl2. Conditions were found in which more than half of the cross-linked protein complexes formed in the PSII preparations retained the ability to catalyze the oxidation of water. The complex is composed of the P33 cross-linked to the D1 and D2 proteins and a 34-kDa protein, which is present in lower abundance than the other three proteins. After solubilization of the membranes with SDS and purification by preparative SDS-PAGE, the complex retains bound manganese and can catalyze the conversion of H2O2 to O2. Calcium and chloride increased the catalase activity of the purified cross-linked complex while lanthanum or hydroxylamine abolished the activity. By use of the specific activity of the H2O2-dependent reaction to follow the extent of purification of the cross-linked complex, the most highly purified complex was determined to contain 0.34 microgram of manganese/180 micrograms of protein. The mole ratio of Mn/protein was calculated to range from 3.6 to 4.5 depending on the assumed stoichiometry of the protein subunits. The results presented here provide direct evidence that one or more of the three proteins that have cross-linked to the P33 are responsible for binding the manganese of the oxygen-evolving complex.

摘要

外在的33 kDa蛋白(P33)与经1 M氯化钙洗涤后的P33缺失型光系统II(PSII)制剂上的结合位点共价交联,该位点负责PSII制剂光合水氧化的重建。发现了这样的条件,即PSII制剂中形成的超过一半的交联蛋白复合物保留了催化水氧化的能力。该复合物由与D1和D2蛋白交联的P33以及一种34 kDa蛋白组成,该蛋白的丰度低于其他三种蛋白。在用SDS溶解膜并通过制备性SDS-PAGE纯化后,该复合物保留结合的锰并能催化H2O2转化为O2。钙和氯增加了纯化的交联复合物的过氧化氢酶活性,而镧或羟胺则消除了该活性。通过使用依赖H2O2的反应的比活性来跟踪交联复合物的纯化程度,确定最高度纯化的复合物含有0.34微克锰/180微克蛋白质。根据蛋白质亚基的假定化学计量,计算出Mn/蛋白质的摩尔比范围为3.6至4.5。此处给出的结果提供了直接证据,表明与P33交联的三种蛋白质中的一种或多种负责结合放氧复合物的锰。

相似文献

1
Manganese-binding proteins of the oxygen-evolving complex.光合放氧复合体的锰结合蛋白
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2
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引用本文的文献

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Photosynthetic water oxidation: The protein framework.光合作用水氧化:蛋白质框架。
Photosynth Res. 1993 Jan;38(3):249-63. doi: 10.1007/BF00046750.
2
Molecular topology of the Photosystem II chlorophyll a binding protein, CP 43: Topology of a thylakoid membrane protein.光系统 II 叶绿素 a 结合蛋白 CP43 的分子拓扑结构:类囊体膜蛋白的拓扑结构。
Photosynth Res. 1994 Apr;40(1):11-9. doi: 10.1007/BF00019041.
3
Occurrence of the 32-kDa QB-binding protein of photosystem II in vegetative cells, heterocysts and akinetes ofAzolla carotiniana cyanobionts.
满江红鱼腥藻光合系统 II 32kDa QB 结合蛋白在营养细胞、异形胞和静息孢子中的存在。
Planta. 1990 Sep;180(3):361-71. doi: 10.1007/BF01160391.
4
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Planta. 1990 Feb;180(3):361-71. doi: 10.1007/BF00198787.
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Structures and functions of the extrinsic proteins of photosystem II from different species.不同物种光系统II外在蛋白的结构与功能
Photosynth Res. 2008 Oct-Dec;98(1-3):349-63. doi: 10.1007/s11120-008-9343-9. Epub 2008 Aug 21.
6
Characterization of the Expression of the Photosystem II-Oxygen Evolving Complex in C(4) Species of Flaveria.描述 Flaveria 属 C(4)种中光系统 II-放氧复合体的表达特征。
Plant Physiol. 1992 Mar;98(3):1154-62. doi: 10.1104/pp.98.3.1154.
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EMBO J. 1990 Jun;9(6):1743-8. doi: 10.1002/j.1460-2075.1990.tb08298.x.