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Solubilization of native integral membrane proteins in aqueous buffer by noncovalent chelation with monomethoxy poly(ethylene glycol) (mPEG) polymers.通过与单甲氧基聚乙二醇(mPEG)聚合物的非共价螯合作用在水缓冲液中溶解天然整体膜蛋白。
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Refolding of an integral membrane protein. Denaturation, renaturation, and reconstitution of intact bacteriorhodopsin and two proteolytic fragments.整合膜蛋白的重折叠。完整细菌视紫红质及其两个蛋白水解片段的变性、复性和重组。
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聚乙二醇-细菌视紫红质水溶性缀合物的复性及质子泵浦活性

Refolding and proton pumping activity of a polyethylene glycol-bacteriorhodopsin water-soluble conjugate.

作者信息

Sirokmán G, Fasman G D

机构信息

Graduate Department of Biochemistry, Brandeis University, Waltham, Massachusetts 02254-9110.

出版信息

Protein Sci. 1993 Jul;2(7):1161-70. doi: 10.1002/pro.5560020711.

DOI:10.1002/pro.5560020711
PMID:8358299
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2142423/
Abstract

Bacteriorhodopsin (BR), from the purple membrane (PM) of Halobacterium halobium, was chemically modified with methoxypolyethylene glycol (m-PEG; molecular weight = 5,000 Da) succinimidyl carbonate. The polyethylene glycol-bacteriorhodopsin (m-PEG-SC-BR33) conjugate, containing one polyethylene glycol chain, was water soluble. The secondary structure of the conjugate in water appeared partially denatured, but was shown to contain alpha-helical segments by circular dichroism spectroscopy. The isolated bacteriorhodopsin conjugate, with added retinal, was refolded in a mixed detergent-lipid micelle and had an absorption maximum at 555 nm. The refolded conjugate was transferred into vesicles that pumped protons, upon illumination, as efficiently as did native BR. Modification of the PM with m-PEG did not alter the native structure or inhibit proton pumping, and therefore it is suggested that the glycol polymer is present as a moiety covalently linked to residues unnecessary for proton pumping and proper folding. The site of attachment of m-PEG was determined to be at either Lys 129 or Lys 159, with position Lys 129 the most probable site of attachment. The m-PEG-SC-BR33 could be stepwise refolded to the native conformation by the addition of trifluoroethanol to lower the dielectric constant, simulating the insertion of the BR into the phospholipid bilayer.

摘要

嗜盐菌紫膜中的细菌视紫红质(BR)用甲氧基聚乙二醇(m-PEG;分子量 = 5000 Da)琥珀酰亚胺碳酸酯进行化学修饰。含有一条聚乙二醇链的聚乙二醇-细菌视紫红质(m-PEG-SC-BR33)缀合物是水溶性的。该缀合物在水中的二级结构呈现部分变性,但通过圆二色光谱显示含有α-螺旋片段。分离得到的添加了视黄醛的细菌视紫红质缀合物在混合去污剂-脂质胶束中重折叠,其最大吸收峰在555 nm处。重折叠后的缀合物被转移到囊泡中,光照时能像天然BR一样有效地泵送质子。用m-PEG对紫膜进行修饰不会改变其天然结构或抑制质子泵送,因此表明二醇聚合物作为一个部分共价连接到质子泵送和正确折叠所不必要的残基上。确定m-PEG的连接位点在赖氨酸129或赖氨酸159处,其中赖氨酸129最可能是连接位点。通过添加三氟乙醇以降低介电常数,模拟BR插入磷脂双层,m-PEG-SC-BR33可以逐步重折叠为天然构象。