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使用自相互作用色谱法准确测量第二维里系数:实验考虑因素。

The accurate measurement of second virial coefficients using self-interaction chromatography: experimental considerations.

机构信息

Surfaces and Particle Engineering Laboratory, Department of Chemical Engineering, Imperial College London, UK.

出版信息

Eur J Pharm Biopharm. 2013 Nov;85(3 Pt B):1103-11. doi: 10.1016/j.ejpb.2013.04.004. Epub 2013 Apr 25.

Abstract

Measurement of B22, the second virial coefficient, is an important technique for describing the solution behaviour of proteins, especially as it relates to precipitation, aggregation and crystallisation phenomena. This paper describes the best practise for calculating B22 values from self-interaction chromatograms (SIC) for aqueous protein solutions. Detailed analysis of SIC peak shapes for lysozyme shows that non-Gaussian peaks are commonly encountered for SIC, with typical peak asymmetries of 10%. This asymmetry reflects a non-linear chromatographic retention process, in this case heterogeneity of the protein-protein interactions. Therefore, it is important to use the centre of mass calculations for determining accurate retention volumes and thus B22 values. Empirical peak maximum chromatogram analysis, often reported in the literature, can result in errors of up to 50% in B22 values. A methodology is reported here for determining both the mean and the variance in B22 from SIC experiments, includes a correction for normal longitudinal peak broadening. The variance in B22 due to chemical effects is quantified statistically and is a measure of the heterogeneity of protein-protein interactions in solution. In the case of lysozyme, a wide range of B22 values are measured which can vary significantly from the average B22 values.

摘要

测量第二维里系数 B22 是描述蛋白质溶液行为的重要技术,特别是在与沉淀、聚集和结晶现象有关时。本文描述了从水相蛋白质溶液的自相互作用色谱(SIC)计算 B22 值的最佳实践。对溶菌酶的 SIC 峰形的详细分析表明,SIC 中通常会遇到非高斯峰,典型的峰不对称性为 10%。这种不对称性反映了非线性色谱保留过程,在这种情况下是蛋白质-蛋白质相互作用的不均匀性。因此,使用质心计算来确定准确的保留体积从而确定 B22 值非常重要。文献中经常报道的经验峰最大值色谱分析可能导致 B22 值的误差高达 50%。本文报告了一种从 SIC 实验中确定 B22 的均值和方差的方法,包括对正常纵向峰展宽的修正。由于化学效应引起的 B22 方差在统计学上进行了量化,是溶液中蛋白质-蛋白质相互作用不均匀性的度量。在溶菌酶的情况下,测量到了广泛的 B22 值,这些值与平均 B22 值差异很大。

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