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Rapid sizing of individual fluorescently stained DNA fragments by flow cytometry.

机译:通过流式细胞仪快速确定单个荧光染色的DNA片段的大小。

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摘要

Large, fluorescently stained restriction fragments of lambda phage DNA are sized by passing individual fragments through a focused continuous wave laser beam in an ultrasensitive flow cytometer at a rate of 60 fragments per second. The size of the fluorescence burst emitted by each stained DNA fragment, as it passes through the laser beam, is measured in one millisecond. One hundred sixty four seconds of fluorescence burst data allow linear sizing of DNA with an accuracy of better than two percent over a range of 10 to 50 kbp. This corresponds to analyzing less than 1 pg of DNA. Sizing of DNA fragments by this approach is much faster, requires much less DNA, and can potentially analyze large fragments with better resolution and accuracy than with gel-based electrophoresis.
机译:通过使单个片段以每秒60个片段的速度通过超灵敏流式细胞仪中聚焦的连续波激光束的大小来确定λ噬菌体DNA的荧光染色大片段的大小。每个染色的DNA片段通过激光束时发出的荧光猝发的大小在1毫秒内测量。一百六十四秒的荧光猝发数据可在10至50 kbp的范围内对DNA进行线性调整,其准确度优于百分之二。这对应于分析少于1 pg的DNA。与基于凝胶的电泳相比,通过这种方法确定DNA片段的大小要快得多,所需的DNA少得多,并且有可能以更高的分辨率和准确性分析大片段。

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