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Fluorescence probes for studying the mechanisms of transcription activation

机译:用于研究转录激活机制的荧光探针

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Regulation of transcription involves a complex interplay between protein-ligand, protein-DNA and protein-protein interactions. Fluorescence probes seem to be very well suited to study such complex systems since the selectivity and sensitivity of fluorescence makes possible to select only a part of the system for observation leaving the rest of it transparent to the technique. We have used fluorescence spectroscopy to study the activation of E.coli RNA polymerase by CAMP receptor protein (CRP). The CAMP interactions with CRP, domain flexibility in CRP molecule, the structure of CRP-DNA complex and interaction of CRP with RNA-polymerase have been studied. Here we report the preparation and properties of 5-OH-Trp derivative of the sigma subunit of E.coli RNA polymerase. This subunit is responsible for specific promoter recognition. The obtained results show that the biological activities of the derivative are identical as observed for the native protein. Comparison of fluorescence properties of the 5-OH-Tip sigma derivative free and bound to the core RNA polymerase suggests a conformational change in the sigma protein induced by this interaction. These data show that replacement of Trp residues with 5-OH-Trp can be a very useful approach to prepare specific fluorescence derivatives of multimeric proteins.
机译:转录调节涉及蛋白质 - 配体,蛋白质-DNA和蛋白质 - 蛋白质相互作用之间的复杂相互作用。荧光探针似乎非常适合研究这种复杂的系统,因为荧光的选择性和灵敏度可以仅选择一个系统的一部分,以便观察到其余的技术对该技术透明。我们使用荧光光谱法通过CAMP受体蛋白(CRP)来研究E.coli RNA聚合酶的活化。研究了CRP,CRP分子中的域灵活性,CRP-DNA复合物的结构和CRP与RNA聚合酶的相互作用的相互作用。在这里,我们报告了大肠杆菌RNA聚合酶Sigma亚基的5-OH-TRP衍生物的制备和性质。该亚基负责特定的推动者识别。得到的结果表明,对于天然蛋白,衍生物的生物活性是相同的。 5-OH-Tip Sigma衍生物无且与核心RNA聚合酶结合的荧光性质的比较表明该相互作用诱导的Sigma蛋白的构象变化。这些数据表明,用5-OH-TRP更换TRP残基可以是制备多聚体蛋白的特异性荧光衍生物的非常有用的方法。

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