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优化的多重聚合酶链反应:高效完成全基因组鸟枪法测序项目

Optimized multiplex PCR: efficiently closing a whole-genome shotgun sequencing project.

作者信息

Tettelin H, Radune D, Kasif S, Khouri H, Salzberg S L

机构信息

The Institute for Genomic Research, 9712 Medical Center Drive, Rockville, Maryland 20850, USA.

出版信息

Genomics. 1999 Dec 15;62(3):500-7. doi: 10.1006/geno.1999.6048.

Abstract

A new method has been developed for rapidly closing a large number of gaps in a whole-genome shotgun sequencing project. The method employs multiplex PCR and a novel pooling strategy to minimize the number of laboratory procedures required to sequence the unknown DNA that falls in between contiguous sequences. Multiplex sequencing, a novel procedure in which multiple PCR primers are used in a single sequencing reaction, is used to interpret the multiplex PCR results. Two protocols are presented, one that minimizes pipetting and another that minimizes the number of reactions. The pipette optimized multiplex PCR method has been employed in the final phases of closing the Streptococcus pneumoniae genome sequence, with excellent results.

摘要

已开发出一种新方法,用于在全基因组鸟枪法测序项目中快速填补大量缺口。该方法采用多重PCR和一种新颖的混合策略,以尽量减少对相邻序列之间未知DNA进行测序所需的实验室操作数量。多重测序是一种在单个测序反应中使用多个PCR引物的新颖方法,用于解读多重PCR结果。本文介绍了两种方案,一种可尽量减少移液操作,另一种可尽量减少反应数量。移液优化的多重PCR方法已应用于肺炎链球菌基因组序列封闭的最后阶段,并取得了优异的结果。

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