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光系统I中铁硫簇的生物合成:来自集胞藻属聚球藻PCC 7002的全酶NfuA在体外能快速且高效地将[4Fe-4S]簇转移至脱辅基PsaC。

Biogenesis of iron-sulfur clusters in photosystem I: holo-NfuA from the cyanobacterium Synechococcus sp. PCC 7002 rapidly and efficiently transfers [4Fe-4S] clusters to apo-PsaC in vitro.

作者信息

Jin Zhao, Heinnickel Mark, Krebs Carsten, Shen Gaozhong, Golbeck John H, Bryant Donald A

机构信息

Department of Biochemistry and Molecular Biology, The Pennsylvania State University, University Park, Pennsylvania 16802, USA.

出版信息

J Biol Chem. 2008 Oct 17;283(42):28426-35. doi: 10.1074/jbc.M803395200. Epub 2008 Aug 11.

DOI:10.1074/jbc.M803395200
PMID:18694929
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2661401/
Abstract

The NfuA protein has been postulated to act as a scaffolding protein in the biogenesis of photosystem (PS) I and other iron-sulfur (Fe/S) proteins in cyanobacteria and chloroplasts. To determine the properties of NfuA, recombinant NfuA from Synechococcus sp. PCC 7002 was overproduced and purified. In vitro reconstituted NfuA contained oxygen- and EDTA-labile Fe/S cluster(s), which had EPR properties consistent with [4Fe-4S] clusters. After reconstitution with 57Fe2+, Mössbauer studies of NfuA showed a broad quadrupole doublet that confirmed the presence of [4Fe-4S]2+ clusters. Native gel electrophoresis under anoxic conditions and chemical cross-linking showed that holo-NfuA forms dimers and tetramers harboring Fe/S cluster(s). Combined with iron and sulfide analyses, the results indicated that one [4Fe-4S] cluster was bound per NfuA dimer. Fe/S cluster transfer from holo-NfuA to apo-PsaC of PS I was studied by reconstitution of PS I complexes using P700-F(X) core complexes, PsaD, apo-PsaC, and holo-NfuA. Electron transfer measurements by time-resolved optical spectroscopy showed that holo-NfuA rapidly and efficiently transferred [4Fe-4S] clusters to PsaC in a reaction that required contact between the two proteins. The NfuA-reconstituted PS I complexes had typical charge recombination kinetics from F(A)/F(B) to P700+ and light-induced low-temperature EPR spectra. These results establish that cyanobacterial NfuA can act as a scaffolding protein for the insertion of [4Fe-4S] clusters into PsaC of PS I in vitro.

摘要

NfuA蛋白被推测在蓝细菌和叶绿体中光系统(PS)I及其他铁硫(Fe/S)蛋白的生物合成过程中充当支架蛋白。为了确定NfuA的特性,来自聚球藻属PCC 7002的重组NfuA被大量表达并纯化。体外重构的NfuA含有对氧气和EDTA敏感的Fe/S簇,其电子顺磁共振(EPR)特性与[4Fe-4S]簇一致。用57Fe2+重构后,对NfuA进行的穆斯堡尔研究显示出一个宽的四极双峰,证实了[4Fe-4S]2+簇的存在。在缺氧条件下进行的非变性凝胶电泳和化学交联表明,全酶形式的NfuA形成含有Fe/S簇的二聚体和四聚体。结合铁和硫化物分析,结果表明每个NfuA二聚体结合一个[4Fe-4S]簇。通过使用P700-F(X)核心复合物、PsaD、脱辅基PsaC和全酶形式的NfuA重构PS I复合物,研究了从全酶形式的NfuA到PS I的脱辅基PsaC的Fe/S簇转移。通过时间分辨光谱进行的电子转移测量表明,全酶形式的NfuA在一个需要两种蛋白质接触的反应中迅速且有效地将[4Fe-4S]簇转移到PsaC。用NfuA重构的PS I复合物具有从F(A)/F(B)到P700+的典型电荷复合动力学以及光诱导低温EPR光谱。这些结果表明,蓝细菌的NfuA在体外可作为一种支架蛋白,用于将[4Fe-4S]簇插入PS I的PsaC中。

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