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嗜热栖热放线菌光系统II结构中亚基D1变异拷贝的建模。

Modeling of variant copies of subunit D1 in the structure of photosystem II from Thermosynechococcus elongatus.

作者信息

Loll Bernhard, Broser Matthias, Kós Peter B, Kern Jan, Biesiadka Jacek, Vass Imre, Saenger Wolfram, Zouni Athina

机构信息

Institute of Chemistry and Biochemistry/Crystallography, Free University Berlin, Takustrasse 6, D-14195 Berlin, Germany.

出版信息

Biol Chem. 2008 May;389(5):609-17. doi: 10.1515/bc.2008.058.

Abstract

In the cyanobacterium Thermosynechococcus elongatus BP-1, living in hot springs, the light environment directly regulates expression of genes that encode key components of the photosynthetic multi-subunit protein-pigment complex photosystem II (PSII). Light is not only essential as an energy source to power photosynthesis, but leads to formation of aggressive radicals which induce severe damage of protein subunits and organic cofactors. Photosynthetic organisms develop several protection mechanisms against this photo-damage, such as the differential expression of genes coding for the reaction center subunit D1 in PSlI. Testing the expression of the three different genes (psbAI, psbAII, psbAIII) coding for D1 in T. elongatus under culture conditions used for preparing the material used in crystallization of PSII showed that under these conditions only subunit PsbA1 is present. However, exposure to high-light intensity induced partial replacement of PsbA1 with PsbA3. Modeling of the variant amino acids of the three different D1 copies in the 3.0 A resolution crystal structure of PSII revealed that most of them are in the direct vicinity to redox-active cofactors of the electron transfer chain. Possible structural and mechanistic consequences for electron transfer are discussed.

摘要

在生活于温泉中的蓝藻嗜热栖热菌BP-1中,光照环境直接调控编码光合多亚基蛋白色素复合物光系统II(PSII)关键组分的基因的表达。光不仅作为驱动光合作用的能量来源至关重要,还会导致具有攻击性的自由基形成,这些自由基会对蛋白质亚基和有机辅因子造成严重损伤。光合生物发展出了多种针对这种光损伤的保护机制,比如PSII中编码反应中心亚基D1的基因的差异表达。在用于制备PSII结晶所用材料的培养条件下,对嗜热栖热菌中编码D1的三个不同基因(psbAI、psbAII、psbAIII)的表达进行检测,结果表明在这些条件下仅存在亚基PsbA1。然而,暴露于高光强度会诱导PsbA1被PsbA3部分取代。在PSII 3.0埃分辨率晶体结构中对三个不同D1拷贝的变异氨基酸进行建模显示,它们大多数都紧邻电子传递链的氧化还原活性辅因子。文中讨论了对电子传递可能产生的结构和机制影响。

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