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带3蛋白群体在红细胞细胞质膜表面的锚定:蛋白质旋转扩散测量。

Anchorage of a band 3 population at the erythrocyte cytoplasmic membrane surface: protein rotational diffusion measurements.

作者信息

Nigg E A, Cherry R J

出版信息

Proc Natl Acad Sci U S A. 1980 Aug;77(8):4702-6. doi: 10.1073/pnas.77.8.4702.

Abstract

Direct physical evidence for the linkage of a band 3 population to the cytoskeleton in the erythrocyte ghost membrane is presented. The rotational diffusion of band 3 proteins was mesured by observing flash-induced transient dichroism of a covalently bound eosin probe. After proteolytic release of a 40,000-dalton cytoplasmic segment of band 3 by trypsin, a considerable enhancement in the decay of the absorption anisotropy was observed. Analysis of the data indicates that proteolytic cleavage of band 3 produces a mobile band 3 population which has restricted mobility in the unperturbed membrane due to protein-protein interactions involving the cytoplasmic band 3 moiety. Band 2.1 (ankyrin) or 4.1 or both are likely to be involved in this interaction because a similar effect on band 3 mobility is observed after low-salt/high-salt extraction of these components. Quantitatively, it is estimated that up to 40% of band 3 may be linked to the cytoskeleton. Because the ankyrin-band 3 dimer stoichiometry in the membrane is approximately 1:5, only about 20% of band 3 dimers can be directly linked to ankyrin. The remainder could be explained by the existence of higher oligomers of band 3 linked to single ankyrin polypeptides or by linkages involving other components such as band 4.1 or 4.2.

摘要

本文提供了红细胞血影膜中带3蛋白群体与细胞骨架相连的直接物理证据。通过观察共价结合的曙红探针的闪光诱导瞬态二色性来测量带3蛋白的旋转扩散。用胰蛋白酶对带3的40000道尔顿细胞质片段进行蛋白水解释放后,观察到吸收各向异性衰减有相当大的增强。数据分析表明,带3的蛋白水解切割产生了一个可移动的带3群体,由于涉及细胞质带3部分的蛋白质-蛋白质相互作用,该群体在未受干扰的膜中移动受限。带2.1(锚蛋白)或4.1或两者可能参与了这种相互作用,因为在对这些成分进行低盐/高盐提取后,观察到对带3迁移率有类似影响。据定量估计,高达40%的带3可能与细胞骨架相连。由于膜中锚蛋白-带3二聚体的化学计量比约为1:5,只有约20%的带3二聚体可以直接与锚蛋白相连。其余部分可以用与单个锚蛋白多肽相连的带3更高寡聚体的存在或涉及其他成分(如带4.1或4.2)的连接来解释。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/59f7/349914/57365ee38a09/pnas00495-0325-a.jpg

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