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Simultaneous Sequencing of Multiple Polymerase Chain Reaction Products and Combined Polymerase Chain Reaction with Cycle Sequencing in Single Reactions

机译:多个聚合酶链反应产物的同时测序以及聚合酶链反应与单次反应的循环测序

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摘要

DNA sequencing is considered the gold standard for nucleic acid identification and mutation detection. However, sequencing is labor intensive because it requires previous amplification and only a single sequence is analyzed at a time. We developed two novel strategies that substantially improve DNA sequencing. The first allows multiple polymerase chain reaction (PCR) products to be sequenced in a single sequencing reaction and analyzed simultaneously in a single lane or capillary. Simultaneous sequencing by this method, designated “SimulSeq,” can provide either simultaneous single-direction sequencing of multiple genes or simultaneous forward and reverse sequencing from a single gene. In the second approach, designated “AmpliSeq,” we demonstrate a technique combining PCR amplification and sequencing in a single reaction that is analyzed in a single lane or capillary. We demonstrate combined PCR with short bidirectional sequencing, and combined PCR with unidirectional sequencing. We anticipate that these methods will have utility in research and clinical settings where panels of mutations or large numbers of samples are be analyzed and/or when turnaround time is critical.
机译:DNA测序被认为是核酸鉴定和突变检测的金标准。然而,测序是费力的,因为它需要先前的扩增并且一次仅分析单个序列。我们开发了两种可以显着改善DNA测序的新颖策略。第一种方法允许在单个测序反应中对多个聚合酶链反应(PCR)产物进行测序,并在单个泳道或毛细管中同时进行分析。通过这种方法(称为“ SimulSeq”)进行的同时测序可以提供多个基因的同时单向测序或单个基因的同时正向和反向测序。在称为“ AmpliSeq”的第二种方法中,我们演示了在单个反应中结合PCR扩增和测序的技术,该反应在单个泳道或毛细管中进行分析。我们演示了结合PCR与短双向测序,以及结合PCR与单向测序。我们预计这些方法将在研究和临床环境中有用,在这些环境中分析突变或大量样品和/或周转时间至关重要时。

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