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Chimeric microbial rhodopsins for optical activation of Gs-proteins

机译:用于光学活化的GS-蛋白的嵌合微生物杂皮物

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We previously showed that the chimeric proteins of microbial rhodopsins, such as light-driven proton pump bacteriorhodopsin (BR) andGloeobacterrhodopsin (GR) that contain cytoplasmic loops of bovine rhodopsin, are able to activate Gt protein upon light absorption. These facts suggest similar protein structural changes in both the light-driven proton pump and animal rhodopsin. Here we report two trials to engineer chimeric rhodopsins, one for the inserted loop, and another for the microbial rhodopsin template. For the former, we successfully activated Gs protein by light through the incorporation of the cytoplasmic loop of β2-adrenergic receptor (β2AR). For the latter, we did not observe any G-protein activation for the light-driven sodium pump fromIndibacter alkaliphilus(IndiR2) or a light-driven chloride pump halorhodopsin fromNatronomonas pharaonis(NpHR), whereas the light-driven proton pump GR showed light-dependent G-protein activation. This fact suggests that a helix opening motion is common to G protein coupled receptor (GPCR) and GR, but not toIndiR2 andNpHR. Light-induced difference FTIR spectroscopy revealed similar structural changes between WT and the third loop chimera for each light-driven pump. A helical structural perturbation, which was largest for GR, was further enhanced in the chimera. We conclude that similar structural dynamics that occur on the cytoplasmic side of GPCR are needed to design chimeric microbial rhodopsins.
机译:我们以前表明,含有牛罗霉素的细胞质回路的微生物紫红蛋白酶的嵌合蛋白,例如含有细胞质环的细胞质循环,能够在光吸收时激活GT蛋白。这些事实表明了灯驱动质子泵和动物杂皮物的类似蛋白质结构变化。在这里,我们将两项试验报告给工程师嵌合罗摩蛋白,一个用于插入的环,另一个用于微生物窝模板。对于前者,我们通过掺入β2-肾上腺素能受体(β2AR)的细胞质回路来通过光成功激活了GS蛋白。对于后者,我们没有观察到从屈曲碱度(Indir2)的光驱动钠泵的任何G蛋白激活或从NORRONONONAS(NPHR)的光驱动的氯化物泵Halorhodopsin,而光驱动质子泵GR显示出光线 - 依赖性g蛋白激活。这一事实表明,螺旋打开运动是G蛋白偶联受体(GPCR)和GR的常见,但不是ToIndir2 Andnphr。光引起的差异FTIR光谱显示器在每个光从动泵的WT和第三环嵌合之间显示出类似的结构变化。在嵌合体中进一步增强了GR最大的螺旋结构扰动。我们得出结论,需要在GPCR的细胞质侧发生的类似结构动态来设计嵌合微生物罗豆蛋白酶。

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