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从叶绿体中纯化或重组的光系统II的PsbS亚基的生化特性。

Biochemical properties of the PsbS subunit of photosystem II either purified from chloroplast or recombinant.

作者信息

Dominici Paola, Caffarri Stefano, Armenante Franca, Ceoldo Stefania, Crimi Massimo, Bassi Roberto

机构信息

Dipartimento Scientifico e Tecnologico, Università degli Studi di Verona, 37134 Verona, Italy.

出版信息

J Biol Chem. 2002 Jun 21;277(25):22750-8. doi: 10.1074/jbc.M200604200. Epub 2002 Apr 4.

DOI:10.1074/jbc.M200604200
PMID:11934892
Abstract

The biochemical properties of PsbS protein, a nuclear-encoded Photosystem II subunit involved in the high energy quenching of chlorophyll fluorescence, have been studied using preparations purified from chloroplasts or obtained by overexpression in bacteria. Despite the homology with chlorophyll a/b/xanthophyll-binding proteins of the Lhc family, native PsbS protein does not show any detectable ability to bind chlorophylls or carotenoids in conditions in which Lhc proteins maintain full pigment binding. The recombinant protein, when refolded in vitro in the presence of purified pigments, neither binds chlorophylls nor xanthophylls, differently from the homologous proteins LHCII, CP26, and CP29 that refold into stable pigment-binding complexes. Thus, it is concluded that if PsbS is a pigment-binding protein in vivo, the binding mechanism must be different from that present in other Lhc proteins. Primary sequence analysis provides evidence for homology of PsbS helices I and III with the central 2-fold symmetric core of chlorophyll a/b-binding proteins. Moreover, a structural homology owed to the presence of acidic residues in each of the two lumen-exposed loops is found with the dicyclohexylcarbodiimide/Ca(2+)-binding domain of CP29. Consistently, both native and recombinant PsbS proteins showed [(14)C]dicyclohexylcarbodiimide binding, thus supporting a functional basis for its homology with CP29 on the lumen-exposed loops. This domain is suggested to be involved in sensing low luminal pH.

摘要

PsbS蛋白是一种参与叶绿素荧光高能猝灭的核编码光系统II亚基,其生化特性已通过从叶绿体中纯化得到的制剂或在细菌中过表达获得的制剂进行了研究。尽管与Lhc家族的叶绿素a/b/叶黄素结合蛋白具有同源性,但在Lhc蛋白保持完全色素结合的条件下,天然PsbS蛋白未显示出任何可检测到的结合叶绿素或类胡萝卜素的能力。与能重折叠成稳定色素结合复合物的同源蛋白LHCII、CP26和CP29不同,重组蛋白在体外纯化色素存在下重折叠时,既不结合叶绿素也不结合叶黄素。因此,可以得出结论,若PsbS在体内是一种色素结合蛋白,其结合机制必定不同于其他Lhc蛋白。一级序列分析为PsbS的螺旋I和III与叶绿素a/b结合蛋白的中心2倍对称核心的同源性提供了证据。此外,发现由于两个暴露于腔的环中均存在酸性残基,PsbS与CP29的二环己基碳二亚胺/Ca(2+)结合结构域存在结构同源性。一致地,天然和重组PsbS蛋白均显示出[(14)C]二环己基碳二亚胺结合,从而支持了其在暴露于腔的环上与CP29同源的功能基础。该结构域被认为参与感知低腔内pH值。

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