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使用定量、高灵敏度荧光杂交技术的细胞遗传学分析。

Cytogenetic analysis using quantitative, high-sensitivity, fluorescence hybridization.

作者信息

Pinkel D, Straume T, Gray J W

出版信息

Proc Natl Acad Sci U S A. 1986 May;83(9):2934-8. doi: 10.1073/pnas.83.9.2934.

Abstract

This report describes the use of fluorescence in situ hybridization for chromosome classification and detection of chromosome aberrations. Biotin-labeled DNA was hybridized to target chromosomes and subsequently rendered fluorescent by successive treatments with fluorescein-labeled avidin and biotinylated anti-avidin antibody. Human chromosomes in human-hamster hybrid cell lines were intensely and uniformly stained in metaphase spreads and interphase nuclei when human genomic DNA was used as a probe. Interspecies translocations were detected easily at metaphase. The human-specific fluorescence intensity from cell nuclei and chromosomes was proportional to the amount of target human DNA. Human Y chromosomes were fluorescently stained in metaphase and interphase nuclei by using a 0.8-kilobase DNA probe specific for the Y chromosome. Cells from males were 40 times brighter than those from females. Both Y chromosomal domains were visible in most interphase nuclei of XYY amniocytes. Human 28S ribosomal RNA genes on metaphase chromosomes were distinctly stained by using a 1.5-kilobase DNA probe.

摘要

本报告描述了荧光原位杂交技术在染色体分类和染色体畸变检测中的应用。生物素标记的DNA与目标染色体杂交,随后通过用荧光素标记的抗生物素蛋白和生物素化抗抗生物素蛋白抗体进行连续处理使其呈现荧光。当使用人类基因组DNA作为探针时,人-仓鼠杂交细胞系中的人类染色体在中期铺展和间期核中被强烈且均匀地染色。在中期很容易检测到种间易位。来自细胞核和染色体的人类特异性荧光强度与目标人类DNA的量成正比。通过使用针对Y染色体的0.8千碱基DNA探针,人类Y染色体在中期和间期核中被荧光染色。雄性细胞比雌性细胞亮40倍。在XYY羊水细胞的大多数间期核中都可见到两个Y染色体区域。通过使用1.5千碱基DNA探针,中期染色体上的人类28S核糖体RNA基因被清晰地染色。

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