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大肠杆菌的乳糖通透酶:精氨酸-302作为假定质子传递体的一个组成部分。

lac permease of Escherichia coli: arginine-302 as a component of the postulated proton relay.

作者信息

Menick D R, Carrasco N, Antes L, Patel L, Kaback H R

机构信息

Roche Institute of Molecular Biology, Roche Research Center, Nutley, New Jersey 07110.

出版信息

Biochemistry. 1987 Oct 20;26(21):6638-44. doi: 10.1021/bi00395a012.

Abstract

The lac permease of Escherichia coli was modified by site-directed mutagenesis such that Arg-302 in putative helix IX was replaced with Leu. In addition, Ser-300 (helix IX) was replaced with Ala, and Lys-319 in putative helix X was replaced with Leu. Permease with Leu at position 302 manifests properties that are similar to those of permease with Arg in place of His-322 [Püttner, I. B., Sarkar, H. K., Poonian, M. S., & Kaback, H. R. (1986) Biochemistry 25, 4483]. Thus, permease with Leu-302 is markedly defective in active lactose transport, efflux, exchange, and counterflow but catalyzes downhill influx of lactose at high substrate concentrations without H+ translocation. In contrast, permease molecules with Ala at position 300 or Leu at position 319 catalyze lactose/H+ symport in a manner indistinguishable from that of wild-type permease. By molecular modeling, Arg-302 may be positioned in helix IX so that it faces the postulated His-322/Glu-325 ion pair in helix X. In this manner, the guanidino group in Arg-302 may interact with the imidazole of His-322 and thereby play a role in the H+ relay suggested to be involved in lactose/H+ symport [Carrasco, N., Antes, L. M., Poonian, M. S., & Kaback, H. R. (1986) Biochemistry 25, 4486].

摘要

通过定点诱变对大肠杆菌的乳糖通透酶进行修饰,使推定的螺旋IX中的精氨酸-302被亮氨酸取代。此外,螺旋IX中的丝氨酸-300被丙氨酸取代,推定的螺旋X中的赖氨酸-319被亮氨酸取代。302位为亮氨酸的通透酶表现出与322位组氨酸被精氨酸取代的通透酶相似的特性[普特纳,I.B.,萨卡尔,H.K.,普尼安,M.S.,&卡巴克,H.R.(1986年)《生物化学》25卷,4483页]。因此,302位为亮氨酸的通透酶在主动乳糖转运、外排、交换和逆向流动方面存在明显缺陷,但在高底物浓度下催化乳糖的顺浓度梯度内流且不伴有氢离子转运。相比之下,300位为丙氨酸或319位为亮氨酸的通透酶分子催化乳糖/氢离子同向转运的方式与野生型通透酶无法区分。通过分子建模,精氨酸-302可能位于螺旋IX中,使其面对螺旋X中假定的组氨酸-322/谷氨酸-325离子对。通过这种方式,精氨酸-302中的胍基可能与组氨酸-322的咪唑相互作用,从而在被认为参与乳糖/氢离子同向转运的氢离子传递中发挥作用[卡拉斯科,N.,安特斯,L.M.,普尼安,M.S.,&卡巴克,H.R.(1986年)《生物化学》25卷,4486页]。

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