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FRP 晶体结构及其活性位点的鉴定,以调节蓝藻中 OCP 介导的光保护作用。

Crystal structure of the FRP and identification of the active site for modulation of OCP-mediated photoprotection in cyanobacteria.

机构信息

US Department of Energy, Joint Genome Institute, Walnut Creek, CA 94598, USA.

出版信息

Proc Natl Acad Sci U S A. 2013 Jun 11;110(24):10022-7. doi: 10.1073/pnas.1303673110. Epub 2013 May 28.

Abstract

Photosynthetic reaction centers are sensitive to high light conditions, which can cause damage because of the formation of reactive oxygen species. To prevent high-light induced damage, cyanobacteria have developed photoprotective mechanisms. One involves a photoactive carotenoid protein that decreases the transfer of excess energy to the reaction centers. This protein, the orange carotenoid protein (OCP), is present in most cyanobacterial strains; it is activated by high light conditions and able to dissipate excess energy at the site of the light-harvesting antennae, the phycobilisomes. Restoration of normal antenna capacity involves the fluorescence recovery protein (FRP). The FRP acts to dissociate the OCP from the phycobilisomes by accelerating the conversion of the active red OCP to the inactive orange form. We have determined the 3D crystal structure of the FRP at 2.5 Å resolution. Remarkably, the FRP is found in two very different conformational and oligomeric states in the same crystal. Based on amino acid conservation analysis, activity assays of FRP mutants, FRP:OCP docking simulations, and coimmunoprecipitation experiments, we conclude that the dimer is the active form. The second form, a tetramer, may be an inactive form of FRP. In addition, we have identified a surface patch of highly conserved residues and shown that those residues are essential to FRP activity.

摘要

光合作用反应中心对高光条件敏感,因为活性氧物种的形成,可能会造成损伤。为了防止高光诱导的损伤,蓝细菌已经开发了光保护机制。一种机制涉及一种光活性类胡萝卜素蛋白,它可以减少过剩能量向反应中心的转移。这种蛋白,即橙色类胡萝卜素蛋白(OCP),存在于大多数蓝细菌菌株中;它在高光条件下被激活,能够在光捕获天线即藻胆体的部位耗散过剩能量。恢复正常天线容量涉及荧光恢复蛋白(FRP)。FRP 通过加速活性红色 OCP 向非活性橙色形式的转化,从藻胆体上分离 OCP。我们已经以 2.5 Å 的分辨率确定了 FRP 的 3D 晶体结构。值得注意的是,在同一个晶体中,FRP 存在两种非常不同的构象和寡聚状态。基于氨基酸保守性分析、FRP 突变体的活性测定、FRP:OCP 对接模拟和共免疫沉淀实验,我们得出结论,二聚体是活性形式。第二种形式,四聚体,可能是 FRP 的无活性形式。此外,我们已经确定了一个高度保守残基的表面斑块,并表明这些残基对 FRP 活性至关重要。

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