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通过稳态荧光和吸光度测量研究fura-2的肌质结合。

Myoplasmic binding of fura-2 investigated by steady-state fluorescence and absorbance measurements.

作者信息

Konishi M, Olson A, Hollingworth S, Baylor S M

机构信息

Department of Physiology, University of Pennsylvania, Philadelphia 19104-6085.

出版信息

Biophys J. 1988 Dec;54(6):1089-104. doi: 10.1016/S0006-3495(88)83045-5.

Abstract

Binding of the fluorescent Ca2+ indicator dye fura-2 by intracellular constituents has been investigated by steady-state optical measurements. Fura-2's (a) fluorescence intensity, (b) fluorescence emission anisotropy, (c) fluorescence emission spectrum, and (d) absorbance spectra were measured in glass capillary tubes containing solutions of purified myoplasmic proteins; properties b and c were also measured in frog skeletal muscle fibers microinjected with fura-2. The results indicate that more than half, and possibly as much as 85%, of fura-2 molecules in myoplasm are in a protein-bound form, and that the binding changes many properties of the dye. For example, in vitro characterization of the Ca2+-dye reaction indicates that when fura-2 is bound to aldolase (a large and abundant myoplasmic protein), the dissociation constant of the dye for Ca2+ is three- to fourfold larger than that measured in the absence of protein. The problems raised by intracellular binding of fura-2 to cytoplasmic proteins may well apply to cells other than skeletal muscle fibers.

摘要

通过稳态光学测量研究了细胞内成分对荧光钙指示剂染料fura-2的结合情况。在含有纯化肌质蛋白溶液的玻璃毛细管中测量了fura-2的(a)荧光强度、(b)荧光发射各向异性、(c)荧光发射光谱和(d)吸收光谱;还在显微注射了fura-2的青蛙骨骼肌纤维中测量了特性b和c。结果表明,肌质中超过一半、可能多达85%的fura-2分子呈蛋白质结合形式,且这种结合改变了染料的许多特性。例如,对钙-染料反应的体外表征表明,当fura-2与醛缩酶(一种大量且丰富的肌质蛋白)结合时,染料对钙的解离常数比在无蛋白质情况下测得的解离常数大三到四倍。fura-2与细胞质蛋白在细胞内结合所引发的问题很可能也适用于骨骼肌纤维以外的其他细胞。

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