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拥挤蛋白质溶液中的蛋白质自缔合:时间分辨荧光偏振研究

Protein self-association in crowded protein solutions: a time-resolved fluorescence polarization study.

作者信息

Zorrilla Silvia, Rivas Germán, Acuña A Ulises, Lillo M Pilar

机构信息

Instituto de Química Física Rocasolano, CSIC, Serrano 119, 28006 Madrid, Spain.

出版信息

Protein Sci. 2004 Nov;13(11):2960-9. doi: 10.1110/ps.04809404. Epub 2004 Sep 30.

Abstract

The self-association equilibrium of a tracer protein, apomyoglobin (apoMb), in highly concentrated crowded solutions of ribonuclease A (RNase A) and human serum albumin (HSA), has been studied as a model system of protein interactions that occur in crowded macromolecular environments. The rotational diffusion of the tracer protein labeled with two different fluorescent dyes, 8-anilinonaphthalene-1-sulfonate and fluorescein isothiocyanate, was successfully recorded as a function of the two crowder concentrations in the 50-200 mg/mL range, using picosecond-resolved fluorescence anisotropy methods. It was found that apoMb molecules self-associate at high RNase A concentration to yield a flexible dimer. The apparent dimerization constant, which increases with RNase A concentration, could also be estimated from the fractional contribution of monomeric and dimeric species to the total fluorescence anisotropy of the samples. In contrast, an equivalent mass concentration of HSA does not result in tracer dimerization. This different effect of RNase A and HSA is much larger than that predicted from simple models based only on the free volume available to apoMb, indicating that additional, nonspecific interactions between tracer and crowder should come into play. The time-resolved fluorescence polarization methods described here are expected to be of general applicability to the detection and quantification of crowding effects in a variety of macromolecules of biological relevance.

摘要

作为在拥挤的大分子环境中发生的蛋白质相互作用的模型系统,已对示踪蛋白脱辅基肌红蛋白(apoMb)在高浓度的核糖核酸酶A(RNase A)和人血清白蛋白(HSA)拥挤溶液中的自缔合平衡进行了研究。使用皮秒分辨荧光各向异性方法,成功记录了用两种不同荧光染料8-苯胺基萘-1-磺酸盐和异硫氰酸荧光素标记的示踪蛋白的旋转扩散,该扩散是50-200 mg/mL范围内两种拥挤剂浓度的函数。研究发现,apoMb分子在高浓度RNase A下会自缔合形成柔性二聚体。表观二聚化常数随RNase A浓度增加,也可从单体和二聚体物种对样品总荧光各向异性的分数贡献中估算出来。相比之下,同等质量浓度的HSA不会导致示踪剂二聚化。RNase A和HSA的这种不同效应比仅基于apoMb可利用的自由体积的简单模型预测的效应大得多,这表明示踪剂与拥挤剂之间应存在额外的非特异性相互作用。本文所述的时间分辨荧光偏振方法有望普遍适用于检测和定量各种具有生物学相关性的大分子中的拥挤效应。

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