首页> 美国卫生研究院文献>Nucleic Acids Research >Quantitative analysis of electrophoresis data: novel curve fitting methodology and its application to the determination of a protein-DNA binding constant.
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Quantitative analysis of electrophoresis data: novel curve fitting methodology and its application to the determination of a protein-DNA binding constant.

机译:电泳数据的定量分析:新型曲线拟合方法及其在测定蛋白质-DNA结合常数中的应用。

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摘要

A computer program, GelExplorer, which uses a new methodology for obtaining quantitative information about electrophoresis has been developed. It provides a straightforward, easy-to-use graphical interface, and includes a number of features which offer significant advantages over existing methods for quantitative gel analysis. The method uses curve fitting with a nonlinear least-squares optimization to deconvolute overlapping bands. Unlike most curve fitting approaches, the data is treated in two dimensions, fitting all the data across the entire width of the lane. This allows for accurate determination of the intensities of individual, overlapping bands, and in particular allows imperfectly shaped bands to be accurately modeled. Experiments described in this paper demonstrate empirically that the Lorentzian lineshape reproduces the contours of an individual gel band and provides a better model than the Gaussian function for curve fitting of electrophoresis bands. Results from several fitting applications are presented and a discussion of the sources and magnitudes of uncertainties in the results is included. Finally, the method is applied to the quantitative analysis of a hydroxyl radical footprint titration experiment to obtain the free energy of binding of the lambda repressor protein to the OR1 operator DNA sequence.
机译:已经开发了一种计算机程序GelExplorer,该程序使用一种新的方法来获得有关电泳的定量信息。它提供了一个简单易用的图形界面,并包括许多功能,这些功能比现有的定量凝胶分析方法具有明显优势。该方法使用具有非线性最小二乘法优化的曲线拟合来对重叠谱带进行反卷积。与大多数曲线拟合方法不同,数据在二维上进行处理,从而在车道的整个宽度上拟合所有数据。这允许精确地确定各个重叠带的强度,并且特别地允许对不完美成形的带进行精确建模。本文所述的实验从经验上证明,洛伦兹线形可重现单个凝胶带的轮廓,并提供比高斯函数更好的电泳带曲线拟合模型。提出了几种拟合应用程序的结果,并对结果的不确定性来源和大小进行了讨论。最后,将该方法用于羟自由基足迹滴定实验的定量分析,以获得λ阻遏蛋白与OR1操纵子DNA序列结合的自由能。

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