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Direct observation of enzymes replicating DNA using a single-molecule DNA stretching assay

机译:使用单分子DNA拉伸测定法直接观察复制DNA的酶

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摘要

We describe a method for observing real time replication of individual DNA molecules mediated by proteins of the bacteriophage replication system. Linearized lambda DNA is modified to have a biotin on the end of one strand, and a digoxigenin moiety on the other end of the same strand. The biotinylated end is attached to a functionalized glass coverslip and the digoxigeninated end to a small bead. The assembly of these DNA-bead tethers on the surface of a flow cell allows a laminar flow to be applied to exert a drag force on the bead. As a result, the DNA is stretched close to and parallel to the surface of the coverslip at a force that is determined by the flow rate (Figure 1). The length of the DNA is measured by monitoring the position of the bead. Length differences between single- and double-stranded DNA are utilized to obtain real-time information on the activity of the replication proteins at the fork. Measuring the position of the bead allows precise determination of the rates and processivities of DNA unwinding and polymerization (Figure 2).
机译:我们描述了一种方法,用于观察由噬菌体复制系统的蛋白质介导的单个DNA分子的实时复制。对线性化的λDNA进行修饰,使其在一条链的末端具有生物素,在同一条链的另一末端具有洋地黄毒苷部分。生物素化的末端附着在功能化的玻璃盖玻片上,而地高辛化的末端附着在小珠上。这些DNA珠子系链在流通池表面上的组装允许施加层流以在珠子上施加阻力。结果,DNA在盖玻片的表面附近并以与流速平行的力拉伸(图1)。通过监测珠子的位置来测量DNA的长度。利用单链和双链DNA之间的长度差异来获得有关叉处复制蛋白活性的实时信息。测量珠子的位置可以精确确定DNA展开和聚合的速率和可操作性(图2)。

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