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Single-Molecule Spectroscopic Determination of Lac Repressor-DNA Loop Conformation

机译:单分子光谱法测定Lac阻遏物-DNA环的构象

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摘要

The Escherichia coli lactose repressor protein (LacI) provides a classic model for understanding protein-induced DNA looping. LacI has a C-terminal four-helix bundle tetramerization domain that may act as a flexible hinge. In previous work, several DNA constructs, each containing two lac operators bracketing a sequence-induced bend, were designed to stabilize different possible looping geometries. The resulting hyperstable LacI-DNA loops exist as both a compact “closed” form with a V-shaped repressor and also a more “open” form with an extended hinge. The “9C14” construct was of particular interest because footprinting, electrophoretic mobility shift, and ring closure experiments suggested that it forms both geometries. Previous fluorescence resonance energy transfer (FRET) measurements gave an efficiency of energy transfer (ET) of 70%, confirming the existence of a closed form. These measurements could not determine whether open form or intermediate geometries are populated or the timescale of interconversion. We have now applied single-molecule FRET to Cy3, Cy5 double-labeled LacI-DNA loops diffusing freely in solution. By using multiple excitation wavelengths and by carefully examining the behavior of the zero-ET peak during titration with LacI, we show that the LacI-9C14 loop exists exclusively in a single closed form exhibiting essentially 100% ET.
机译:大肠杆菌乳糖阻遏蛋白(LacI)为了解蛋白诱导的DNA环化提供了经典模型。 LacI具有一个C端四螺旋束四聚结构域,可以充当柔性铰链。在以前的工作中,设计了几种DNA结构,每个结构都包含两个由lac操纵子括起来的序列诱导的弯曲,以稳定不同的可能的环状结构。产生的超稳定LacI-DNA环以带有V形阻遏物的紧凑“闭合”形式和带有延伸铰链的更“开放”形式存在。 “ 9C14”构建体特别受关注,因为足迹,电泳迁移率变化和闭环实验表明它同时形成了两种几何形状。先前的荧光共振能量转移(FRET)测量给出了70%的能量转移效率(ET),证实了封闭形式的存在。这些测量无法确定是否填充了开放形式或中间几何形状或相互转换的时间尺度。现在,我们将单分子FRET应用于在溶液中自由扩散的Cy3,Cy5双标记的LacI-DNA环。通过使用多个激发波长并通过仔细检查用LacI滴定期间零ET峰的行为,我们表明LacI-9C14环仅以单个闭合形式存在,基本上表现出100%的ET。

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