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在 Synechococcus sp. PCC 7002 的光系统 I 电子传递链中,作为功能组件的 PsaC 变体中存在一个 [3Fe-4S] 簇。

Presence of a [3Fe-4S] cluster in a PsaC variant as a functional component of the photosystem I electron transfer chain in Synechococcus sp. PCC 7002.

机构信息

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

Department of Pharmacology and Toxicology, University of Louisville, Louisville, KY, 40202, USA.

出版信息

Photosynth Res. 2018 Apr;136(1):31-48. doi: 10.1007/s11120-017-0437-0. Epub 2017 Sep 15.

Abstract

A site-directed C14G mutation was introduced into the stromal PsaC subunit of Synechococcus sp. strain PCC 7002 in vivo in order to introduce an exchangeable coordination site into the terminal F [4Fe-4S] cluster of Photosystem I (PSI). Using an engineered PSI-less strain (psaAB deletion), psaC was deleted and replaced with recombinant versions controlled by a strong promoter, and the psaAB deletion was complemented. Modified PSI accumulated at lower levels in this strain and supported slower photoautotrophic growth than wild type. As-isolated PSI complexes containing PsaC showed resonances with g values of 2.038 and 2.007 characteristic of a [3Fe-4S] cluster. When the PSI complexes were illuminated at 15 K, these resonances partially disappeared and two new sets of resonances appeared. The majority set had g values of 2.05, 1.95, and 1.85, characteristic of F, and the minority set had g values of 2.11, 1.90, and 1.88 from F' in the modified site. The S = 1/2 spin state of the latter implied the presence of a thiolate as the terminal ligand. The [3Fe-4S] clusters could be partially reconstituted with iron, producing a larger population of [4Fe-4S] clusters. Rates of flavodoxin reduction were identical in PSI complexes isolated from wild type and the PsaC variant strain; this implied equivalent capacity for forward electron transfer in PSI complexes that contained [3Fe-4S] and [4Fe-4S] clusters. The development of this cyanobacterial strain is a first step toward translation of in vitro PSI-based biosolar molecular wire systems in vivo and provides new insights into the formation of Fe/S clusters.

摘要

为了在光合作用系统 I (PSI) 的末端 F [4Fe-4S] 簇中引入一个可交换的配位位点,我们在活体中将一个定点 C14G 突变引入了蓝细菌 Synechococcus sp. 株 PCC 7002 的基质 PsaC 亚基中。利用工程化的 PSI 缺失菌株 (psaAB 缺失),我们删除了 psaC 并用受强启动子控制的重组版本取代,并且补全了 psaAB 缺失。在这种菌株中,修饰后的 PSI 积累水平较低,并且比野生型支持更缓慢的光自养生长。含有 PsaC 的分离 PSI 复合物显示出 g 值为 2.038 和 2.007 的共振,这是 [3Fe-4S] 簇的特征。当 PSI 复合物在 15 K 下被照射时,这些共振部分消失,出现了两组新的共振。主要组的 g 值为 2.05、1.95 和 1.85,这是修饰部位 F 的特征,而少数组的 g 值为 2.11、1.90 和 1.88,这是 F' 的特征。后者的 S = 1/2 自旋状态表明存在硫醇作为末端配体。用铁可以部分重新构建 [3Fe-4S] 簇,产生更多的 [4Fe-4S] 簇。从野生型和 PsaC 变体菌株中分离的 PSI 复合物中,黄素蛋白还原的速率相同;这意味着在含有 [3Fe-4S] 和 [4Fe-4S] 簇的 PSI 复合物中,向前电子转移的能力相同。这种蓝细菌菌株的发展是将体外基于 PSI 的生物太阳能分子线系统在体内进行翻译的第一步,为 Fe/S 簇的形成提供了新的见解。

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