首页> 美国卫生研究院文献>Proceedings of the National Academy of Sciences of the United States of America >Structure and function in rhodopsin: Kinetic studies of retinal binding to purified opsin mutants in defined phospholipid–detergent mixtures serve as probes of the retinal binding pocket
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Structure and function in rhodopsin: Kinetic studies of retinal binding to purified opsin mutants in defined phospholipid–detergent mixtures serve as probes of the retinal binding pocket

机译:视紫红质的结构和功能:在确定的磷脂-洗涤剂混合物中视网膜与纯化视蛋白突变体结合的动力学研究可作为视网膜结合袋的探针

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摘要

In the current standard procedure for preparation of mammalian rhodopsin mutants, transfected COS-1 cells expressing the mutant opsin genes are treated with 5 μM 11-cis-retinal before detergent solubilization for purification. We found that binding of 11-cis-retinal to opsin mutants with single amino acid changes at Trp-265 (W265F,Y,A) and a retinitis pigmentosa mutant (A164V) was far from complete and required much higher concentrations of 11-cis-retinal. By isolation of the expressed opsins in a stable form, kinetic studies of retinal binding to the opsins in vitro have been carried out by using defined phospholipid–detergent mixtures. The results show wide variation in the rates of 11-cis-retinal binding. Thus, the in vitro reconstitution procedure serves as a probe of the retinal-binding pocket in the opsins. Further, a method is described for purification and characterization of the rhodopsin mutants after retinal binding to the opsins in vitro.
机译:在制备哺乳动物视紫红质突变体的当前标准程序中,在用去污剂溶解纯化之前,用5μM11-顺式-视网膜处理表达突变视蛋白基因的转染的COS-1细胞。我们发现11-顺-视网膜与视蛋白突变体的结合在Trp-265(W265F,Y,A)和色素性视网膜炎突变体(A164V)具有单个氨基酸变化远未完成,需要更高浓度的11-顺式-视网膜。通过以稳定的形式分离表达的视蛋白,通过使用确定的磷脂-洗涤剂混合物,进行了视网膜与视蛋白结合的动力学研究。结果显示11-顺-视网膜结合的速率差异很大。因此,体外重建程序充当视蛋白中视网膜结合袋的探针。此外,描述了在视网膜与视蛋白结合后体外纯化和鉴定视紫红质突变体的方法。

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