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人类18号染色体三个区域特异性显微切割文库的构建与表征

Construction and characterization of three region-specific microdissection libraries for human chromosome 18.

作者信息

Kao F T, Tong S, Shen Y, Yu J

机构信息

Eleanor Roosevelt Institute for Cancer Research, Denver, Colorado 80206, USA.

出版信息

Somat Cell Mol Genet. 1996 May;22(3):191-9. doi: 10.1007/BF02369909.

DOI:10.1007/BF02369909
PMID:8914604
Abstract

Three region-specific libraries for the entire human chromosome 18 were constructed using microdissection and Mbol linker-adaptor microcloning techniques. The libraries included 18pter-p11.1 (designated 18P library), 18q11.1-q12.3 (18Q1 library), and 18q21.1-qter (18Q2 library). Samples of the microclones from each library were analyzed in detail. The insert sizes ranged between 50-600 bp, with a mean of 180-220 bp for the three libraries. The libraries contained approximately 40-60% microclones with unique sequence inserts. More than 30 unique sequence microclones from each library were analyzed by Southern blot hybridization to demonstrate that they are human specific and were derived from chromosome 18. The human genomic HindIII fragments hybridized to each microclone were determined and microclones cross-hybridized to rodent species were identified. These region-specific libraries and the unique sequence microclones from the libraries are useful reagents for (1) isolating highly polymorphic microsatellite markers for refined linkage analysis, (2) identifying corresponding YAC, BAC or other clones with large inserts for contig assembly and high resolution physical mapping, (3) isolating cDNA clones from the dissected region, and (4) convenient sequencing of the microclones to prepare high density markers and sequence-tagged sites (STSs). Such applications have been demonstrated in a series of similarly constructed microdissection libraries from other regions of the human genome.

摘要

利用显微切割和MboI接头-衔接子微克隆技术构建了覆盖整个人类18号染色体的三个区域特异性文库。这些文库包括18pter-p11.1(命名为18P文库)、18q11.1-q12.3(18Q1文库)和18q21.1-qter(18Q2文库)。对每个文库的微克隆样本进行了详细分析。插入片段大小在50-600bp之间,三个文库的平均大小为180-220bp。文库中约40-60%的微克隆含有独特序列插入片段。通过Southern印迹杂交分析了每个文库中30多个独特序列微克隆,以证明它们是人类特异性的且源自18号染色体。确定了与每个微克隆杂交的人类基因组HindIII片段,并鉴定了与啮齿动物物种交叉杂交的微克隆。这些区域特异性文库以及文库中的独特序列微克隆是有用的试剂,可用于:(1)分离高度多态的微卫星标记用于精细连锁分析;(2)鉴定相应的YAC、BAC或其他大插入片段克隆用于重叠群组装和高分辨率物理图谱绘制;(3)从切割区域分离cDNA克隆;(4)方便地对微克隆进行测序以制备高密度标记和序列标签位点(STS)。在一系列来自人类基因组其他区域的类似构建的显微切割文库中已经证明了此类应用。

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