首页> 外文期刊>Analytical Biochemistry: An International Journal of Analytical and Preparative Methods >Structural analysis of RecA protein-DNA complexes by fluorescence-detected linear dichroism: Absence of structural change of filament for pairing of complementary DNA strands
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Structural analysis of RecA protein-DNA complexes by fluorescence-detected linear dichroism: Absence of structural change of filament for pairing of complementary DNA strands

机译:通过荧光检测的线性二色性对RecA蛋白-DNA复合物的结构分析:缺少用于互补DNA链配对的细丝结构变化

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We have developed a simple measuring system for fluorescence-detected linear dichroism and applied it to the structural analysis of the RecA-DNA complex filaments, which are intermediates of the homologous recombination reaction. Taking advantage of the selectivity of fluorescence signals, we distinguished the linear dichroism signals of ethidium bromide and tryptophan residues in the RecA-DNA-ethidium bromide complex, whereas the conventional (absorption-detected) linear dichroism measurement provides only the sum of the signals because signals overlap each other and that of DNA. We further observed that the tryptophan residue at position 290 of RecA in the RecA-DNA-adenosine-5'-O-(3-thiotriphosphate) complex was oriented parallel to the long axis of the filament, in good agreement with the previous site-specific linear dichroism analysis, and that this orientation was not significantly modified by the pairing of the complementary DNA strand. These results suggest that the pairing reaction occurs without a large structural change of the RecA filament. (c) 2006 Elsevier Inc. All rights reserved.
机译:我们已经开发出一种用于荧光检测线性二色性的简单测量系统,并将其应用于RecA-DNA复合细丝的结构分析,该复合细丝是同源重组反应的中间产物。利用荧光信号的选择性,我们区分了RecA-DNA-溴化乙锭复合物中溴化乙锭和色氨酸残基的线性二色性信号,而传统的(吸收检测)线性二色性测量仅提供信号之和,因为信号彼此重叠,与DNA重叠。我们进一步观察到,RecA-DNA-腺苷-5'-O-(3-硫代三磷酸)络合物中RecA位置290的色氨酸残基与丝的长轴平行,与之前的位点-线性二色性分析,并且该方向没有被互补DNA链配对显着修饰。这些结果表明,在没有RecA细丝的大结构变化的情况下发生配对反应。 (c)2006 Elsevier Inc.保留所有权利。

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