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通过荧光共振能量同转移测量人红细胞带3的寡聚状态。

Oligomeric state of human erythrocyte band 3 measured by fluorescence resonance energy homotransfer.

作者信息

Blackman S M, Piston D W, Beth A H

机构信息

Department of Molecular Physiology and Biophysics, Vanderbilt University, Nashville, Tennessee 37232-0615 USA.

出版信息

Biophys J. 1998 Aug;75(2):1117-30. doi: 10.1016/S0006-3495(98)77601-5.

Abstract

The oligomeric state of the erythrocyte anion exchange protein, band 3, has been assayed by resonance energy homotransfer. Homotransfer between oligomeric subunits, labeled with eosin-5-maleimide at Lys430 in the transmembrane domain, has been demonstrated by steady-state and time-resolved fluorescence spectroscopy, and is readily observed by its depolarization of the eosin fluorescence. Polarized fluorescence measurements of HPLC-purified band 3 oligomers indicate that eosin homotransfer increases progressively with increasing species size. This shows that homotransfer also occurs between labeled band 3 dimers as well as within the dimers, making fluorescence anisotropy measurements sensitive to band 3 self-association. Treatment of ghost membranes with either Zn2+ or melittin, agents that cluster band 3, significantly decreases the anisotropy as a result of the increased homotransfer within the band 3 clusters. By comparison with the anisotropy of species of known oligomeric state, the anisotropy of erythrocyte ghost membranes at 37 degrees C is consistent with dimeric and/or tetrameric band 3, and does not require postulation of a fraction of large clusters. Proteolytic removal of the cytoplasmic domain of band 3, which significantly increases the rotational mobility of the transmembrane domain, does not affect its oligomeric state, as reported by eosin homotransfer. These results support a model in which interaction with the membrane skeleton restricts the mobility of band 3 without significantly altering its self-association state.

摘要

红细胞阴离子交换蛋白(带3蛋白)的寡聚状态已通过共振能量同转移进行了测定。通过稳态和时间分辨荧光光谱法已证实,在跨膜结构域中赖氨酸430位点用5-马来酰亚胺基曙红标记的寡聚亚基之间存在同转移,并且通过曙红荧光的去极化很容易观察到。对经高效液相色谱纯化的带3蛋白寡聚体进行的偏振荧光测量表明,曙红同转移随着物种大小的增加而逐渐增加。这表明同转移也发生在标记的带3蛋白二聚体之间以及二聚体内,使得荧光各向异性测量对带3蛋白的自缔合敏感。用锌离子或蜂毒素(可使带3蛋白聚集的试剂)处理血影膜,由于带3蛋白聚集体内同转移增加,会显著降低各向异性。与已知寡聚状态物种的各向异性相比,37摄氏度下红细胞血影膜的各向异性与二聚体和/或四聚体带3蛋白一致,无需假定存在一部分大聚集体。如曙红同转移所报道的那样,蛋白水解去除带3蛋白的细胞质结构域(这会显著增加跨膜结构域的旋转流动性)不会影响其寡聚状态。这些结果支持了一个模型,即与膜骨架的相互作用限制了带3蛋白的流动性,而不会显著改变其自缔合状态。

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