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使用多重寡核苷酸杂交组装的小鼠11号染色体锚定框架BAC图谱。

An anchored framework BAC map of mouse chromosome 11 assembled using multiplex oligonucleotide hybridization.

作者信息

Cai W W, Reneker J, Chow C W, Vaishnav M, Bradley A

机构信息

Department of Molecular and Human Genetics, Howard Hughes Medical Institute, Baylor College of Medicine, One Baylor Plaza, Houston, Texas, 77030, USA.

出版信息

Genomics. 1998 Dec 15;54(3):387-97. doi: 10.1006/geno.1998.5620.

Abstract

Despite abundant library resources for many organisms, physical mapping of these organisms has been seriously limited due to lack of efficient library screening techniques. We have developed a highly efficient strategy for large-scale screening of genomic libraries based on multiplex oligonucleotide hybridization on high-density genomic filters. We have applied this strategy to generate a bacterial artificial chromosome (BAC) anchored map of mouse chromosome 11. Using the MIT mouse SSLP data, 320 pairs of oligonucleotide probes were designed with an "overgo" computer program that selects new primer sequences that avoid the microsatellite repeat. BACs identified by these probes are automatically anchored to the chromosome. Ninety-two percent of the probes identified positive clones from a 5.9-fold coverage mouse BAC library with an average of 7 positive clones per marker. An average of 4.2 clones was confirmed for 204 markers by PCR. Our data show that a large number of clones can be efficiently isolated from a large genomic library using this strategy with minimal effort. This strategy will have wide application for large-scale mapping and sequencing of human and other large genomes.

摘要

尽管有许多生物的丰富文库资源,但由于缺乏有效的文库筛选技术,这些生物的物理图谱绘制受到严重限制。我们基于高密度基因组滤膜上的多重寡核苷酸杂交,开发了一种用于大规模筛选基因组文库的高效策略。我们已将此策略应用于构建小鼠11号染色体的细菌人工染色体(BAC)锚定图谱。利用麻省理工学院小鼠简单序列长度多态性(SSLP)数据,用“overgo”计算机程序设计了320对寡核苷酸探针,该程序选择新的引物序列以避开微卫星重复序列。由这些探针鉴定出的BAC自动锚定到染色体上。92%的探针从一个覆盖5.9倍的小鼠BAC文库中鉴定出阳性克隆,每个标记平均有7个阳性克隆。通过聚合酶链反应(PCR)对204个标记平均确认了4.2个克隆。我们的数据表明,使用该策略可以轻松地从大型基因组文库中高效分离出大量克隆。该策略将广泛应用于人类和其他大型基因组的大规模图谱绘制和测序。

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