重组人干扰素α2的时间分辨荧光研究。蛋白质的缔合状态，两个色氨酸残基的空间接近度。

Time-resolved fluorescence study of human recombinant interferon alpha 2. Association state of the protein, spatial proximity of the two tryptophan residues.

作者信息

Vincent M, Li De La Sierra I M, Berberan-Santos M N, Diaz A, Diaz M, Padron G, Gallay J

机构信息

Laboratoire pour l'Utilisation du Rayonnement Electromagnétique, Université Paris Sud, Orsay, France.

出版信息

Eur J Biochem. 1992 Dec 15;210(3):953-61. doi: 10.1111/j.1432-1033.1992.tb17500.x.

DOI:10.1111/j.1432-1033.1992.tb17500.x

PMID:1483478

Abstract

Human recombinant interferon alpha 2 belongs a to family of proteins active against a wide range of viruses. It contains two tryptophan residues located at positions 77 and 141 in the peptide sequence. The fluorescence emission spectrum of these tryptophan residues displays a maximum at 335 nm. The fluorescence intensity decay is described by one broad excited-state-lifetime population centered around a value of 1.7 ns (full width at half maximum, 1.5 ns). These observations suggest that in the native protein, both tryptophan residues emit from similar environments, not directly exposed to the surrounding solvent. The anisotropy decay is essentially biexponential. The correlation-time value characterizing the Brownian rotation of the protein varies linearly with the viscosity/temperature ratio. The calculated hydrodynamic volumes are compatible with the existence of a dimer and a tetramer, at pH 5.5 and 9.4, respectively. Addition of urea at pH 5.5 disrupts the dimer and modifies to some extent the excited-state-lifetime distribution which becomes more heterogeneous. Disulfide-bond reduction also dissociates the dimer and leads to a highly heterogeneous fluorescence-intensity decay with four excited-state-lifetime populations. An opening of the local structure in the Trp region of the protein is likely to occur in these conditions. The fast-anisotropy-decay components can be due to either fast rotation or energy transfer between the indoles. Close proximity of the two Trp residues (less than 1 nm) is suggested from steady-state and time-resolved fluorescence-anisotropy measurements in vitrified medium [95% (by mass) glycerol at -38 degrees C]. This suggestion is in agreement with the recently published three-dimensional structure of the homologous protein murine interferon beta [Senda, T., Shimazu, T., Matsuda, S. Kawano, G., Shimizu, H., Nakamura, K. T. & Mitsui, Y. (1992) EMBO J. 11, 3193-3201].

摘要

人重组干扰素α2属于一类对多种病毒具有活性的蛋白质家族。它在肽序列的第77位和141位含有两个色氨酸残基。这些色氨酸残基的荧光发射光谱在335nm处有最大值。荧光强度衰减由一个以1.7ns为中心的宽激发态寿命群体描述（半高宽为1.5ns）。这些观察结果表明，在天然蛋白质中，两个色氨酸残基在相似的环境中发射，并非直接暴露于周围溶剂中。各向异性衰减基本上是双指数的。表征蛋白质布朗旋转的相关时间值随粘度/温度比线性变化。在pH 5.5和9.4时，计算得到的流体力学体积分别与二聚体和四聚体的存在相符。在pH 5.5时添加尿素会破坏二聚体，并在一定程度上改变激发态寿命分布，使其变得更加不均匀。二硫键还原也会使二聚体解离，并导致具有四个激发态寿命群体的高度不均匀的荧光强度衰减。在这些条件下，蛋白质色氨酸区域的局部结构可能会打开。快速各向异性衰减成分可能是由于吲哚之间的快速旋转或能量转移。通过在玻璃化介质（-38℃下95%（质量）甘油）中的稳态和时间分辨荧光各向异性测量表明，两个色氨酸残基距离很近（小于1nm）。这一推测与最近发表的同源蛋白小鼠干扰素β的三维结构一致[Senda, T., Shimazu, T., Matsuda, S., Kawano, G., Shimizu, H., Nakamura, K. T. & Mitsui, Y. (1992) EMBO J. 11, 3193 - 3201]。