Polovinkin V, Gushchin I, Sintsov M, Round E, Balandin T, Chervakov P, Shevchenko V, Utrobin P, Popov A, Borshchevskiy V, Mishin A, Kuklin A, Willbold D, Chupin V, Popot J-L, Gordeliy V
Univ. Grenoble Alpes, IBS, 38044, Grenoble, France.
J Membr Biol. 2014 Oct;247(9-10):997-1004. doi: 10.1007/s00232-014-9700-x. Epub 2014 Sep 6.
Amphipols (APols) have become important tools for the stabilization, folding, and in vitro structural and functional studies of membrane proteins (MPs). Direct crystallization of MPs solubilized in APols would be of high importance for structural biology. However, despite considerable efforts, it is still not clear whether MP/APol complexes can form well-ordered crystals suitable for X-ray crystallography. In the present work, we show that an APol-trapped MP can be crystallized in meso. Bacteriorhodopsin (BR) trapped by APol A8-35 was mixed with a lipidic mesophase, and crystallization was induced by adding a precipitant. The crystals diffract beyond 2 Å. The structure of BR was solved to 2 Å and found to be indistinguishable from previous structures obtained after transfer from detergent solutions. We suggest the proposed protocol of in meso crystallization to be generally applicable to APol-trapped MPs.
两性离子双亲分子(APols)已成为用于膜蛋白(MPs)的稳定化、折叠以及体外结构和功能研究的重要工具。直接结晶溶解在APols中的MPs对结构生物学具有高度重要性。然而,尽管付出了相当大的努力,但MP/APol复合物是否能形成适用于X射线晶体学的有序晶体仍不清楚。在本工作中,我们表明被APol捕获的MP可以在介晶中结晶。被APol A8 - 35捕获的细菌视紫红质(BR)与脂质中间相混合,并通过添加沉淀剂诱导结晶。这些晶体的衍射分辨率超过2 Å。BR的结构解析到2 Å,发现与先前从去污剂溶液转移后获得的结构没有区别。我们认为所提出的介晶结晶方案通常适用于被APol捕获的MPs。
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