从稳态荧光测量评估蛋白质中的结合位点数量。

On the evaluation of the number of binding sites in proteins from steady state fluorescence measurements.

机构信息

Facultad de Química y Biología, Universidad de Santiago de Chile, Casilla 40- Correo 33, Santiago, Chile.

出版信息

J Fluoresc. 2011 Sep;21(5):1831-3. doi: 10.1007/s10895-011-0887-2. Epub 2011 Apr 12.

Abstract

The number of binding sites for a given solute in a protein is a most relevant parameter. This number can be derived from fluorescence quenching data which provides the fraction of sites occupied at a given free solute concentration. Data are generally treated according to Scatchard´s or Ward´s equations. Lately, a double logarithmic plot of the data has been extensively used with this purpose. The present communication discus the validity of this procedure. It is concluded that this type of plot provides an evaluation of the stoichiometry (molecularity) of the binding process but not the number of equivalent binding sites per protein.

摘要

给定溶质在蛋白质中结合位点的数量是一个非常重要的参数。这个数量可以从荧光猝灭数据中得出，该数据提供了在给定游离溶质浓度下占据的位点分数。数据通常根据 Scatchard 或 Ward 方程进行处理。最近，为了达到这个目的，广泛使用了数据的双对数图。本通讯讨论了这个程序的有效性。结论是，这种类型的图提供了对结合过程的化学计量（分子数）的评估，但不是每个蛋白质的等效结合位点的数量。

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从稳态荧光测量评估蛋白质中的结合位点数量。

On the evaluation of the number of binding sites in proteins from steady state fluorescence measurements.

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