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A new strategy useful for rapid identification of microsatellites from DNA libraries with large size inserts.

机译:一种新的策略可用于从具有大尺寸插入片段的DNA库中快速识别微卫星。

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摘要

Microsatellites are new powerful polymorphic markers used for gene mapping. Their characterization requires that all the sequence surrounding the repeat be known in order to be able to design primers for PCR amplification. However, when using DNA libraries with large cloned inserts, this sequence characterization is not immediately practicable. In this paper, we describe a new strategy, based both on the use of a microsatellite specific probing and on the creation of nested deleted clones with the Exonuclease III, in order to position microsatellites in a range allowing direct sequencing. This method was applied to the screening of a mouse chromosome 19 DNA specific library. In this way, thirteen clones were identified by specific probing and seven were submitted to the nested deletion strategy. Five of them presented microsatellite sequences in specific deleted subclones which were selected and sequenced. Primers were designed for each of them and polymorphism between the genomes of several inbred strain of mouse have been determined. These microsatellites were mapped, three of them to chromosome 19 and two to chromosome 11.
机译:微卫星是用于基因定位的新型强大的多态标记。它们的表征要求知道重复序列周围的所有序列,以便能够设计用于PCR扩增的引物。但是,当使用具有大克隆插入片段的DNA文库时,这种序列表征并非立即可行。在本文中,我们描述了一种新策略,该策略基于微卫星特异性探针的使用以及利用核酸外切酶III创建嵌套缺失克隆的目的,目的是将微卫星定位在允许直接测序的范围内。该方法用于筛选小鼠19号染色体DNA特异文库。这样,通过特异性探测鉴定出13个克隆,并将7个克隆提交给嵌套缺失策略。他们中的五个在特定缺失的亚克隆中呈现了微卫星序列,这些亚克隆被选择并测序。为每个引物设计引物,并确定了几种自交系小鼠的基因组之间的多态性。这些微卫星被定位,其中三个到19号染色体,两个到11号染色体。

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