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利用锚定TAA重复引物从细菌人工染色体克隆中快速开发基因标记微卫星标记

Rapid development of gene-tagged microsatellite markers from bacterial artificial chromosome clones using anchored TAA repeat primers.

作者信息

Waldbieser Geoffrey C, Quiniou Sylvie M A, Karsi Attila

机构信息

United States Department of Agriculture, Agricultural Research Service, Stoneville, MS, USA.

出版信息

Biotechniques. 2003 Nov;35(5):976-9. doi: 10.2144/03355st05.

Abstract

We developed a technique to improve the efficiency of producing TAA repeat microsatellite markers linked to interspecific conserved genes. Template DNA was prepared from cultures derived from single bacterial artificial chromosome (BAC) colonies using a simple alkaline lysis miniprep. The presence of conserved genes in each BAC clone was verified by sequencing with gene-specific primers. The BAC templates were directly sequenced using short tandem repeat-anchored primers (STRAPs), consisting of TAA repeats with one or two unique 3' terminal bases. At least one STRAP provided sufficient 3' flanking sequence from each clone for the design of a BAC-specific primer. The BAC-specific primer was used to sequence back through the tandem repeat and obtain 5' flanking sequence, and a second BAC-specific primer was designed for microsatellite genotype analysis. This technique quickly provided microsatellite markers with an average of 15 tandem repeats for the BAC clones tested. The identification of polymorphic microsatellite loci in these clones permits the identification of alleles linked to candidate genes, placement of conserved genes on genetic linkage maps, and integration of linkage and physical maps.

摘要

我们开发了一种技术,以提高与种间保守基因连锁的TAA重复微卫星标记的生产效率。使用简单的碱性裂解小量制备法从单个细菌人工染色体(BAC)菌落衍生的培养物中制备模板DNA。通过用基因特异性引物测序来验证每个BAC克隆中保守基因的存在。使用由带有一个或两个独特3'末端碱基的TAA重复序列组成的短串联重复锚定引物(STRAP)对BAC模板进行直接测序。每个克隆至少有一个STRAP提供足够的3'侧翼序列,用于设计BAC特异性引物。BAC特异性引物用于反向测序串联重复序列并获得5'侧翼序列,并且设计了第二个BAC特异性引物用于微卫星基因型分析。该技术为测试的BAC克隆快速提供了平均具有15个串联重复序列的微卫星标记。鉴定这些克隆中的多态性微卫星位点可以鉴定与候选基因连锁的等位基因,将保守基因定位在遗传连锁图谱上,以及整合连锁图谱和物理图谱。

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