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体细胞杂种中人染色体物质的同步鉴定与显带

Simultaneous identification and banding of human chromosome material in somatic cell hybrids.

作者信息

Tucker J D, Christensen M L, Carrano A V

机构信息

Lawrence Livermore National Laboratory, Biomedical Sciences Division, University of California, Livermore 94550.

出版信息

Cytogenet Cell Genet. 1988;48(2):103-6. doi: 10.1159/000132600.

Abstract

We have developed a method that identifies human chromosomes in human x hamster somatic cell hybrids and simultaneously bands these same metaphases. Other methods generally require separate slides for banding and detection of human chromosome material, making the precise characterization of human material difficult. Our procedure involves denaturing metaphase chromosomes, followed by in situ hybridization of biotinylated whole human DNA. Fluoresceinated avidin is then bound to the biotinylated DNA, staining the human chromosomes yellow-green when excited with UV light. Chromosome banding is achieved by staining the slides with DAPI and actinomycin D. The fluorescein and DAPI excite maximally at 488 and 355 nm and emit at 520 and 450 nm, respectively. This permits identification of the human material at one excitation wavelength and visualization of the banding patterns at another wavelength. With this procedure, we have successfully identified both intact and broken human chromosomes, as well as human material involved in human x hamster translocations. The results indicate that this procedure is more accurate and considerably more rapid than previous methods and can be routinely employed for the cytogenetic analysis of human x rodent hybrids.

摘要

我们开发了一种方法,可在人 - 仓鼠体细胞杂种中鉴定人类染色体,并同时对这些中期染色体进行显带。其他方法通常需要分别制作用于显带和检测人类染色体物质的玻片,这使得对人类物质进行精确表征变得困难。我们的程序包括使中期染色体变性,然后进行生物素化的整个人类DNA的原位杂交。然后将荧光素化抗生物素蛋白与生物素化的DNA结合,在用紫外线激发时将人类染色体染成黄绿色。通过用DAPI和放线菌素D对玻片进行染色来实现染色体显带。荧光素和DAPI分别在488和355nm处具有最大激发波长,并在520和450nm处发射。这允许在一个激发波长下鉴定人类物质,并在另一个波长下观察显带模式。通过这个程序,我们成功地鉴定了完整和断裂的人类染色体,以及涉及人 - 仓鼠易位的人类物质。结果表明,该程序比以前的方法更准确、速度更快,可常规用于人 - 啮齿动物杂种的细胞遗传学分析。

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