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红细胞膜糖转运蛋白的增溶、复性及亲和层析尝试

Solubilization, reconstitution, and attempted affinity chromatography of the sugar transporter of the erythrocyte membrane.

作者信息

Weber J, Warden D A, Semenza G, Diedrich D F

出版信息

J Cell Biochem. 1985;27(2):83-96. doi: 10.1002/jcb.240270203.

Abstract

Reconstitution of the sugar transport system of human erythrocytes into artificial liposomes was achieved by freezing, thawing, and sonicating preformed phospholipid vesicles in the presence of intact ghosts, protein-depleted ghosts, or detergent-treated ghosts. D-glucose equilibrium exchange activities and affinity constants in the range of the reported erythrocyte values were reached in the best experiments. Whereas the extraction of peripheral membrane proteins did not depress the transport function crucially after reconstituting these protein-depleted ghosts, the selective solubilization of integral membrane proteins by a variety of nonionic detergents resulted in an uncontrollable, continuously increasing inactivation of the carrier. However, Emulphogene BC-720 extracts could be prepared in which the glucose transporter retained activity for days at 4 degrees C. These extracts were applied to affinity chromatography matrices of phloretin-Agarose, prepared by coupling phloretinyl-3'-benzylamine (PBA) to CH-Sepharose 4B and to Affigel 202. Although the solubilized sugar transporter appeared to be selectively adsorbed to both PBA matrices, it could not be eluted by specific counter ligands or gentle eluants in a biologically active form. However, chaotropic agents could be used to elute intrinsic proteins, including bands 3 and 4.5, from the Affigel affinity medium.

摘要

通过在完整红细胞影、脱蛋白红细胞影或经去污剂处理的红细胞影存在的情况下,对预先形成的磷脂囊泡进行冷冻、解冻和超声处理,实现了将人红细胞的糖转运系统重构到人工脂质体中。在最佳实验中,达到了报道的红细胞值范围内的D - 葡萄糖平衡交换活性和亲和常数。尽管重构这些脱蛋白红细胞影后,外周膜蛋白的提取并没有严重抑制转运功能,但多种非离子去污剂对整合膜蛋白的选择性溶解导致载体出现无法控制的、持续增加的失活。然而,可以制备出Emulphogene BC - 720提取物,其中葡萄糖转运蛋白在4℃下可保持数天的活性。这些提取物被应用于根皮素 - 琼脂糖亲和色谱基质,该基质是通过将根皮素基 - 3'-苄胺(PBA)偶联到CH - Sepharose 4B和Affigel 202上制备的。尽管溶解的糖转运蛋白似乎被选择性吸附到两种PBA基质上,但它不能被特定的反配体或温和的洗脱剂以生物活性形式洗脱。然而,离液剂可用于从Affigel亲和介质中洗脱包括带3和带4.5在内的内在蛋白。

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