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无细胞合成的连接蛋白 43 直接整合到脂质体中形成半通道。

Direct integration of cell-free-synthesized connexin-43 into liposomes and hemichannel formation.

机构信息

Institute of Biomaterials and Bioengineering, Tokyo Medical and Dental University, Tokyo, Japan.

出版信息

FEBS J. 2010 Aug;277(16):3343-52. doi: 10.1111/j.1742-4658.2010.07736.x. Epub 2010 Jul 1.

Abstract

Proteoliposomes were directly prepared by synthesizing membrane proteins with the use of minimal protein synthesis factors isolated from Escherichia coli (the PURE system) in the presence of liposomes. Connexin-43 (Cx43), which is a water-insoluble integral membrane protein that forms a hexameric complex in membranes, was cotranslationally integrated with an essentially uniform orientation in liposomes. The addition of liposomes following protein expression (post-translational presence of liposomes) did not lead to the integration of Cx43 into the liposome membranes. The amount of integrated Cx43 increased as the liposome concentration increased. The presence of liposomes did not influence the total amount of synthesized Cx43. The Cx43 integrated into the liposome membranes formed open membrane pores. These results indicate that the liposomes act in a chaperone-like manner by preventing Cx43 from aggregating in solution, because of integration into the bilayer, and also by functionalization of the integrated Cx43 in the membrane. This is the first report that cell-free-synthesized water-insoluble membrane protein is directly integrated with a uniform orientation as a functional oligomer into liposome membranes. This simple proteoliposome preparation procedure should be a valuable approach for structural and functional studies of membrane proteins.

摘要

通过使用从大肠杆菌中分离的最小蛋白合成因子(PURE 系统)在脂质体存在的情况下直接合成膜蛋白,制备了类脂体。间隙连接蛋白 43(Cx43)是一种不溶于水的整合膜蛋白,在膜中形成六聚体复合物,在脂质体中以基本均匀的取向共翻译整合。在蛋白表达后(脂质体的翻译后存在)添加脂质体不会导致 Cx43 整合到脂质体膜中。随着脂质体浓度的增加,整合的 Cx43 数量增加。脂质体的存在并不影响合成的 Cx43 的总量。整合到脂质体膜中的 Cx43 形成开放的膜孔。这些结果表明,脂质体通过将 Cx43 整合到双层中防止其在溶液中聚集,以及通过对膜中整合的 Cx43 进行功能化,以类似伴侣的方式发挥作用。这是首次报道无细胞合成的不溶于水的膜蛋白直接以均匀的取向作为功能性寡聚体整合到脂质体膜中。这种简单的类脂体制备方法应该是膜蛋白结构和功能研究的一种有价值的方法。

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