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红细胞膜骨架蛋白网络的电子自旋共振研究:血影蛋白聚集状态对膜蛋白、双层脂质及细胞表面碳水化合物物理状态的影响。

ESR studies of the erythrocyte membrane skeletal protein network: influence of the state of aggregation of spectrin on the physical state of membrane proteins, bilayer lipids, and cell surface carbohydrates.

作者信息

Farmer B T, Harmon T M, Butterfield D A

出版信息

Biochim Biophys Acta. 1985 Dec 19;821(3):420-30. doi: 10.1016/0005-2736(85)90046-x.

DOI:10.1016/0005-2736(85)90046-x
PMID:3000446
Abstract

The stability of the human erythrocyte membrane skeletal network is reported to be dependent on the state of aggregation of spectrin and decreased or increased by polyphosphate anions or the polyamine, spermine, respectively. We have employed polyacrylamide gel electrophoresis and electron spin resonance (ESR) utilizing spin labels specific for membrane proteins, bilayer lipids, or cell-surface sialic acid in order to gain insight into these observations and into the reliability of the ESR spectra of the protein-specific spin label used to correctly report the interactions of the skeletal protein network. The major findings are: (1) We confirm previous reports that the preferred state of spectrin aggregation in the skeletal network is tetrameric and that spectrin can be reversibly transformed to dimeric spectrin and back to tetrameric spectrin on the membrane. (2) The ESR spectra of the protein specific maleimide spin label employed accurately reflect the state of aggregation of spectrin. (3) As dimeric spectrin is increased on the membrane or when 2,3-bisphosphoglycerate was added to spin-labeled membranes, increased segmental motion of protein spin label binding sites reflecting decreased protein-protein interactions in the skeletal network is observed (P less than 0.002 and P less than 0.005, respectively). (4) Conversely, as protein-protein interactions between skeletal proteins or between skeletal proteins and the bilayer are increased by spermine (reflected in the total inability to extract spectrin from the membrane in contrast to control membranes), highly decreased segmental motion of the protein specific spin label binding site is observed (P less than 0.005). (5) The dimeric-tetrameric state of spectrin aggregation on the membrane does not have influence on the order or motion of bilayer lipids nor on the rotational rate of spin-labeled, cell-surface sialic acid, a result also observed when protein-protein interactions were decreased by 2,3-bisphosphoglycerate. In contrast, increased protein-protein interactions by addition of spermine produced a small, but significant, increase in order and decrease in motion of bilayer lipids near the membrane surface as well as a nearly 40% decrease in the apparent rotational correlation time of spin labeled, cell surface sialic acid (P less than 0.002). These latter observations are discussed with reference to possible associations of phospholipids and the major, transmembrane sialoglycoprotein with the skeletal protein network.

摘要

据报道,人红细胞膜骨架网络的稳定性取决于血影蛋白的聚集状态,多磷酸阴离子或多胺精胺分别会使其降低或增加。我们采用了聚丙烯酰胺凝胶电泳和电子自旋共振(ESR)技术,利用对膜蛋白、双层脂质或细胞表面唾液酸具有特异性的自旋标记,以便深入了解这些观察结果以及用于正确报告骨架蛋白网络相互作用的蛋白特异性自旋标记的ESR光谱的可靠性。主要发现如下:(1)我们证实了先前的报道,即骨架网络中血影蛋白聚集的优选状态是四聚体,并且血影蛋白在膜上可以可逆地转变为二聚体血影蛋白并再变回四聚体血影蛋白。(2)所使用的蛋白特异性马来酰亚胺自旋标记的ESR光谱准确反映了血影蛋白的聚集状态。(3)当膜上二聚体血影蛋白增加时,或者当向自旋标记的膜中添加2,3 - 二磷酸甘油酸时,观察到蛋白自旋标记结合位点的片段运动增加,这反映了骨架网络中蛋白 - 蛋白相互作用的减少(P分别小于0.002和P小于0.005)。(4)相反,当精胺增加骨架蛋白之间或骨架蛋白与双层之间的蛋白 - 蛋白相互作用时(与对照膜相比,这表现为完全无法从膜中提取血影蛋白),观察到蛋白特异性自旋标记结合位点的片段运动高度降低(P小于0.005)。(5)膜上血影蛋白聚集的二聚体 - 四聚体状态对双层脂质的有序性或运动以及自旋标记的细胞表面唾液酸的旋转速率没有影响,当2,3 - 二磷酸甘油酸降低蛋白 - 蛋白相互作用时也观察到了这一结果。相比之下,添加精胺增加蛋白 - 蛋白相互作用会使膜表面附近的双层脂质的有序性略有但显著增加,运动略有降低,并且自旋标记的细胞表面唾液酸的表观旋转相关时间降低近40%(P小于0.002)。后面这些观察结果将结合磷脂和主要的跨膜唾液糖蛋白与骨架蛋白网络可能的关联进行讨论。

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