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通过荧光原位杂交将染色体重排断点定位到秀丽隐杆线虫的物理图谱上。

Mapping chromosome rearrangement breakpoints to the physical map of Caenorhabditis elegans by fluorescent in situ hybridization.

作者信息

Albertson D G

机构信息

Laboratory of Molecular Biology, Medical Research Council, Cambridge, England.

出版信息

Genetics. 1993 May;134(1):211-9. doi: 10.1093/genetics/134.1.211.

Abstract

A scheme for rapidly mapping chromosome rearrangements relative to the physical map of Caenorhabditis elegans is described that is based on hybridization patterns of cloned DNA on meiotic nuclei, as visualized by fluorescent in situ hybridization. From the nearly complete physical map, DNA clones, in yeast artificial chromosomes (YACs), spanning the rearrangement breakpoint were selected. The purified YAC DNAs were first amplified by degenerate oligonucleotide-primed polymerase chain reaction, then reamplified to incorporate fluorescein dUTP or rhodamine dUTP. The site of hybridization was visualized directly (without the use of antibodies) on meiotic bivalents. This allows chromosome rearrangements to be mapped readily if the duplicated, deficient or translocated regions do not pair with a normal homologous region, because the site or sites of hybridization of the probe on meiotic prophase nuclei will be spatially distinct. The pattern, or number, of hybridization signals from probes from within, or adjacent to, the rearranged region of the genome can be predicted from the genetic constitution of the strain. Characterization of the physical extent of the genetically mapped rearrangements places genetic landmarks on the physical map, and so provides linkage between the two types of map.

摘要

本文描述了一种用于快速绘制相对于秀丽隐杆线虫物理图谱的染色体重排图谱的方案,该方案基于通过荧光原位杂交可视化的克隆DNA在减数分裂细胞核上的杂交模式。从几乎完整的物理图谱中,选择了酵母人工染色体(YAC)中跨越重排断点的DNA克隆。纯化的YAC DNA首先通过简并寡核苷酸引物聚合酶链反应进行扩增,然后再次扩增以掺入荧光素dUTP或罗丹明dUTP。杂交位点在减数分裂二价体上直接可视化(无需使用抗体)。如果重复、缺失或易位区域不与正常同源区域配对,这使得染色体重排能够很容易地被定位,因为探针在减数分裂前期细胞核上的杂交位点在空间上是不同的。来自基因组重排区域内或相邻区域的探针的杂交信号模式或数量可以根据菌株的遗传组成来预测。对遗传定位的重排的物理范围进行表征,可在物理图谱上放置遗传标记,从而在两种类型的图谱之间建立联系。

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