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Determination of the molecular weight of DNA-bound protein(s) responsible for gel electrophoretic mobility shift of linear DNA fragments examplified with purified viral myb protein.

机译:确定负责纯化的病毒myb蛋白的线性DNA片段的凝胶电泳迁移率变化的DNA结合蛋白的分子量。

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摘要

A protein-DNA complex has less gel electrophoretic mobility than the free DNA fragment. One parameter for the degree of retardation of a linear DNA fragment in a protein-DNA complex is the molecular weight of the bound protein(s). The quotient of the migration distances of free DNA (m) and protein-DNA complex (m') is a function of the molecular weight (MW) of the bound protein(s). Based on the evaluation of the lac repressor induced mobility shift of a 203 bp DNA fragment containing the lac operator in a 5% non-denaturating polyacrylamide gel a direct proportionality could be shown between (m/m'-1) and MW with the proportionality factor K = 215 kDa. The factor K depends on the acrylamide concentration in the gel, getting lower values with increasing acrylamide concentrations. A calculation is given to determine the molecular weight of DNA-binding factors responsible for the decreased electrophoretic mobility of a linear DNA fragment. As an example this calculation was used in order to analyse DNA-binding of the isolated viral myb protein. It could be demonstrated that the viral myb protein binds to DNA as a monomer and as a dimer.
机译:蛋白质-DNA复合物的凝胶电泳迁移率低于游离DNA片段。蛋白质-DNA复合物中线性DNA片段的延迟程度的一个参数是结合的蛋白质的分子量。游离DNA(m)和蛋白质-DNA复合物(m')的迁移距离的商是结合蛋白质的分子量(MW)的函数。根据对lac阻遏物诱导的203 bp含lac操纵子的DNA片段在5%非变性聚丙烯酰胺凝胶中的迁移率迁移的评估,可以显示(m / m'-1)与MW之间成正比因子K = 215 kDa。因子K取决于凝胶中丙烯酰胺的浓度,随着丙烯酰胺浓度的增加,其值将降低。进行计算以确定引起线性DNA片段电泳迁移率降低的DNA结合因子的分子量。例如,该计算用于分析分离的病毒myb蛋白的DNA结合。可以证明病毒myb蛋白以单体和二聚体的形式结合到DNA上。

著录项

  • 作者

    Bading, H;

  • 作者单位
  • 年度 1988
  • 总页数
  • 原文格式 PDF
  • 正文语种 en
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