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胶质纤维酸性蛋白的组装、拆卸及交换

Assembly, disassembly, and exchange of glial fibrillary acidic protein.

作者信息

Nakamura Y, Takeda M, Angelides K J, Tada K, Hariguchi S, Nishimura T

机构信息

Department of Neuropsychiatry, Osaka University Medical School, Japan.

出版信息

Glia. 1991;4(1):101-10. doi: 10.1002/glia.440040112.

DOI:10.1002/glia.440040112
PMID:1828780
Abstract

The kinetics and dynamics of glial fibrillary acidic protein (GFAP) assembly was explored by a fluorescence energy transfer assay method. Purified GFAP was stoichiometrically labeled at a single cysteine residue with fluorescein-maleimide. Soluble labeled GFAP in a low ionic strength buffer was assembled into 10 nm filaments by rapidly increasing the ionic strength, and the kinetics of GFAP assembly was monitored by the reduction in fluorescence due to self-quenching of fluorescein. The extent of fluorescence quench correlated with both the formation of 10 nm filament morphology and the amount of protein pelleted at 12,000g. The assembly of GFAP is critically dependent upon both protein and magnesium ion concentration, and at the critical concentration for GFAP assembly is approximately 40 micrograms/ml. Disassembly of GFAP filaments was also observed as a relief of fluorescence quenching after dilution of labeled GFAP filaments. When labeled GFAP filaments were mixed with an excess of unlabeled filaments, a rapid increase of fluorescence was observed, which is due to an exchange of subunits between labeled and unlabeled GFAP filaments. These results indicate that GFAP filaments are dynamic structures and that a small pool of kinetically active unassembled GFAP subunits are in a dynamic equilibrium with assembled GFAP filaments. The ability of GFAP to assemble, disassemble, and undergo subunit exchange has important implications for the organization and dynamics of astroglia cell cytoskeleton during development and in response to injury.

摘要

通过荧光能量转移测定法探究了胶质纤维酸性蛋白(GFAP)组装的动力学和动态过程。纯化的GFAP在单个半胱氨酸残基上用荧光素-马来酰亚胺进行化学计量标记。在低离子强度缓冲液中的可溶性标记GFAP通过快速增加离子强度组装成10纳米的细丝,并且通过荧光素自猝灭导致的荧光降低来监测GFAP组装的动力学。荧光猝灭程度与10纳米细丝形态的形成以及在12,000g下沉淀的蛋白量相关。GFAP的组装严重依赖于蛋白质和镁离子浓度,并且GFAP组装的临界浓度约为40微克/毫升。在标记的GFAP细丝稀释后,也观察到GFAP细丝的解组装表现为荧光猝灭的缓解。当标记的GFAP细丝与过量的未标记细丝混合时,观察到荧光迅速增加,这是由于标记和未标记的GFAP细丝之间的亚基交换。这些结果表明GFAP细丝是动态结构,并且一小部分具有动力学活性的未组装GFAP亚基与组装的GFAP细丝处于动态平衡。GFAP组装、解组装和进行亚基交换的能力对于发育过程中以及对损伤作出反应时星形胶质细胞细胞骨架的组织和动态具有重要意义。

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