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The average unwinding angle of DNA duplex produced by the binding of chromomycin A3.

机译:结合霉素霉素产生的DNA双链体的平均展开角。

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The effect of chromomycin A3 binding on the geometry of DNA duplex (plasmid pBR322) has been examined using topoisomerase I relaxation followed by gel electrophoresis. To determine the equilibrium constant of this drug-DNA binding-dissociation reaction in the same concentration range (ca. 10(-5) M) in the same buffer as those for the topoisomerase reaction (at 37 degrees C), fluorescence measurements were made of the same plasmid-drug system, followed by a Scatchard plot and an analysis using McGhee-von Hippel's exclusion site model. The binding constant has been found to be 3.8 x 10(5) M-1 in the particular buffer (buffer-T) at 37 degrees C, and the number of base pairs involved in the site of one chromomycin molecule on the duplex has been found to be 5. It has been concluded that one chromomycin molecule, bound to the duplex, unwinds it by 11.8 +/- 1.1 degrees. In addition, the enthalpy of binding was determined to be 31.81 kJ/mole using a titration calorimeter with a more concentrated (6.2 mM) solution.
机译:已使用拓扑异构酶I松弛法进行了凝胶电泳,研究了嗜霉素A3结合对DNA双链体(质粒pBR322)的几何形状的影响。为了确定在相同浓度范围内(约10(-5)M)和拓扑异构酶反应(在37摄氏度)的相同缓冲液中此药物-DNA结合解离反应的平衡常数,进行了荧光测量相同的质粒-药物系统,然后进行Scatchard图,并使用McGhee-von Hippel的排除位点模型进行分析。已发现在37°C下特定缓冲液(buffer-T)中的结合常数为3.8 x 10(5)M-1,双链体上一个嗜霉素分子的位点所涉及的碱基对数目为发现是5。已经得出结论,与双链体结合的一个嗜霉素分子将其展开11.8 +/- 1.1度。此外,使用滴定热量计和更浓的溶液(6.2 mM)确定结合焓为31.81 kJ / mol。

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