首页> 美国卫生研究院文献>Proceedings of the National Academy of Sciences of the United States of America >Mapping of single-copy DNA sequences on human chromosomes by in situ hybridization with biotinylated probes: enhancement of detection sensitivity by intensified-fluorescence digital-imaging microscopy.
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Mapping of single-copy DNA sequences on human chromosomes by in situ hybridization with biotinylated probes: enhancement of detection sensitivity by intensified-fluorescence digital-imaging microscopy.

机译:通过与生物素化探针的原位杂交在人染色体上绘制单拷贝DNA序列的图谱:通过增强荧光数字成像显微镜增强检测灵敏度。

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摘要

Two single-copy DNA segments of 6 kilobases (kb) and 2.3 kb were labeled with biotin-labeled dUTP (Bio11-dUTP) and hybridized to human chromosomes. These probes were detected by immunofluorescence and directly mapped on chromosomes by using classical fluorescence microscopy and a microchannel-plate-intensified video camera. By a subsequent R-banding, the 6-kb and 2.3-kb fragments were precisely localized to the 18p11.3 band and to the 22q11.2 band, respectively, in agreement with previous results obtained with radioactive probes. The adaptation of fluorescence intensification and digital image processing (frame integration to enhance signal-to-noise ratio and linear contrast stretching) to microscopy makes it possible to detect very weak fluorescent spots on chromosomes. This system allows a high spatial resolution (less than 0.6 micron), even at very low fluorescence levels. The efficiency and the specificity of the hybridization and detection methodology give a direct and precise localization of the short single-copy sequences on human chromosomes.
机译:用生物素标记的dUTP(Bio11-dUTP)标记6个碱基(kb)和2.3 kb的两个单拷贝DNA片段,并与人类染色体杂交。这些探针通过免疫荧光检测,并通过经典荧光显微镜和微通道板增强摄像机直接定位在染色体上。通过随后的R谱带,将6 kb和2.3 kb片段分别精确定位在18p11.3波段和22q11.2波段,这与放射性探针获得的先前结果相符。将荧光增强和数字图像处理(帧整合以增强信噪比和线性对比度拉伸)与显微镜相适应,可以检测染色体上非常弱的荧光点。该系统即使在非常低的荧光水平下也可以实现高空间分辨率(小于0.6微米)。杂交和检测方法的效率和特异性为人类染色体上的短单拷贝序列提供了直接而精确的定位。

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