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细胞色素P-450的旋转。I. 磷脂囊泡和肝微粒体中细胞色素P-450的蛋白质-蛋白质相互作用研究。

Rotation of cytochrome P-450. I. Investigations of protein-protein interactions of cytochrome P-450 in phospholipid vesicles and liver microsomes.

作者信息

Kawato S, Gut J, Cherry R J, Winterhalter K H, Richter C

出版信息

J Biol Chem. 1982 Jun 25;257(12):7023-9.

PMID:7085615
Abstract

Rotation of cytochrome P-450 was examined in both liver microsomes and reconstituted and phospholipid vesicles. Purified cytochrome P-450 was incorporated into lipid vesicles composed of phosphatidylcholine-phosphatidylethanolamine-Phosphatidylserne. Rotational diffusion was measured by detecting the decay of absorption anisotropy, r(t), after photolysis of the heme. CO complex by a vertically polarized laser flash. No contribution of vesicle tumbling to r(t) was observed over the experimental time range of 0-500 mus for samples in 60% sucrose. Analysis of r(t) was based on a "rotation-about-membrane normal" model. The measurements were used to investigate intermolecular interactions of cytochrome P-450. In vesicles of a high lipid to protein ratio (=30 by weight), the residual time-independent normalized anisotropy, r (infinity)/r (0), reached a limiting low value, implying that all cytochrome P-450 was rotating. The mean rotational relaxation time, phi 1, was about 95 mus. In contrast, about 35% of cytochrome P-450 was immobilized in vesicles of a low lipid to protein ratio (=1), with phi 1 of about 95 mus for the mobile fraction. The immobile fraction is presumably due to self-aggregation of cytochrome P-450. In rat liver microsomes, 0-50% of cytochrome P-450 was mobile with phi 1 of about 120 mus at 20 degrees C, and the rest was immobile. A significant temperature dependence of r(t) was observed in microsomes. All cytochrome P-450 was immobile below 7 degrees C, and about 50% of the enzyme was mobile at 37 degrees C with phi 1 approximately 60 mus. From the limiting value of r(infinity)/r(0) congruent to 0.12, the tilt angle of the heme plane of cytochrome p-450 from the membrane plane was calculated to be about 40 degrees.

摘要

在肝微粒体、重组磷脂囊泡中研究了细胞色素P - 450的旋转情况。将纯化的细胞色素P - 450掺入由磷脂酰胆碱 - 磷脂酰乙醇胺 - 磷脂酰丝氨酸组成的脂质囊泡中。通过检测血红素CO复合物经垂直偏振激光闪光光解后吸收各向异性r(t)的衰减来测量旋转扩散。在60%蔗糖溶液中的样品,在0 - 500微秒的实验时间范围内未观察到囊泡翻滚对r(t)有贡献。对r(t)的分析基于“绕膜法线旋转”模型。这些测量用于研究细胞色素P - 450的分子间相互作用。在高脂质与蛋白质比例(重量比 = 30)的囊泡中,与时间无关的归一化剩余各向异性r(∞)/r(0)达到一个极限低值,这意味着所有细胞色素P - 450都在旋转。平均旋转弛豫时间φ1约为95微秒。相比之下,在低脂质与蛋白质比例(重量比 = 1)的囊泡中,约35%的细胞色素P - 450是固定的,可移动部分的φ1约为95微秒。固定部分可能是由于细胞色素P - 450的自聚集。在大鼠肝微粒体中,在20℃时,0 - 50%的细胞色素P - 450是可移动的,φ1约为120微秒,其余部分是固定的。在微粒体中观察到r(t)对温度有显著依赖性。在7℃以下所有细胞色素P - 450都是固定的,在37℃时约50%的酶是可移动的,φ1约为60微秒。根据r(∞)/r(0)约为0.12的极限值,计算出细胞色素P - 450血红素平面与膜平面的倾斜角约为40度。

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