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罗氏领鞭毛虫视黄叉/磷酸二酯酶融合蛋白RhoPDE的纯化与特性分析及其作为潜在光遗传学工具的研究

Purification and Characterization of RhoPDE, a Retinylidene/Phosphodiesterase Fusion Protein and Potential Optogenetic Tool from the Choanoflagellate Salpingoeca rosetta.

作者信息

Lamarche Lindsey B, Kumar Ramasamy P, Trieu Melissa M, Devine Erin L, Cohen-Abeles Luke E, Theobald Douglas L, Oprian Daniel D

机构信息

Department of Biochemistry, Brandeis University , Waltham, Massachusetts 02454, United States.

出版信息

Biochemistry. 2017 Oct 31;56(43):5812-5822. doi: 10.1021/acs.biochem.7b00519. Epub 2017 Oct 18.

Abstract

RhoPDE is a type I rhodopsin/phosphodiesterase gene fusion product from the choanoflagellate Salpingoeca rosetta. The gene was discovered around the time that a similar type I rhodopsin/guanylyl cyclase fusion protein, RhoGC, was shown to control phototaxis of an aquatic fungus through a cGMP signaling pathway. RhoPDE has potential as an optogenetic tool catalyzing the hydrolysis of cyclic nucleotides. Here we provide an expression and purification system for RhoPDE, as well as a crystal structure of the C-terminal phosphodiesterase catalytic domain. We show that RhoPDE contains an even number of transmembrane segments, with N- and C-termini both located on the cytoplasmic surface of the cell membrane. The purified protein exhibits an absorption maximum at 490 nm in the dark state, which shifts to 380 nm upon exposure to light. The protein acts as a cGMP-selective phosphodiesterase. However, the activity does not appear to be modulated by light. The protein is also active with cAMP as a substrate, but with a roughly 5-7-fold lower k. A truncation consisting solely of the phosphodiesterase domain is also active with a k for cGMP roughly 6-9-fold lower than that of the full-length protein. The isolated PDE domain was crystallized, and the X-ray structure showed the protein to be a dimer similar to human PDE9. We anticipate that the purification system introduced here will enable further structural and biochemical experiments to improve our understanding of the function and mechanism of this unique fusion protein.

摘要

RhoPDE是来自领鞭毛虫玫瑰薮枝虫(Salpingoeca rosetta)的I型视紫红质/磷酸二酯酶基因融合产物。该基因是在一种类似的I型视紫红质/鸟苷酸环化酶融合蛋白RhoGC被证明通过cGMP信号通路控制水生真菌的趋光性前后被发现的。RhoPDE有潜力作为一种催化环核苷酸水解的光遗传学工具。在这里,我们提供了一种用于RhoPDE的表达和纯化系统,以及C端磷酸二酯酶催化结构域的晶体结构。我们表明,RhoPDE含有偶数个跨膜片段,其N端和C端都位于细胞膜的细胞质表面。纯化后的蛋白在黑暗状态下在490 nm处有最大吸收峰,光照后会转移到380 nm。该蛋白作为一种cGMP选择性磷酸二酯酶发挥作用。然而,其活性似乎不受光的调节。该蛋白以cAMP为底物时也有活性,但k值大约低5 - 7倍。仅由磷酸二酯酶结构域组成的截短体对cGMP的k值也有活性,大约比全长蛋白低6 - 9倍。分离出的PDE结构域被结晶,X射线结构显示该蛋白是一个类似于人PDE9的二聚体。我们预计这里引入的纯化系统将能够进行进一步的结构和生化实验,以增进我们对这种独特融合蛋白的功能和机制的理解。

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