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Utilization of Super BAC Pools and Fluidigm Access Array Platform for High-Throughput BAC Clone Identification: Proof of Concept

机译:超级BAC池和Fluidigm访问阵列平台用于高通量BAC克隆鉴定的概念验证

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摘要

Bacterial artificial chromosome (BAC) libraries are critical for identifying full-length genomic sequences, correlating genetic and physical maps, and comparative genomics. Here we describe the utilization of the Fluidigm access array genotyping system in conjunction with KASPar genotyping technology to identify individual BAC clones corresponding to specific single-nucleotide polymorphisms (SNPs) from an Amplicon Express seven-plate super pooled Amaranthus hypochondriacus BAC library. Ninety-six SNP loci, spanning the length of A. hypochondriacus linkage groups 1, 2, and 15, were simultaneously tested for clone identification from four BAC super pools, corresponding to 28 384-well plates, using a single Fluidigm integrated fluidic chip (IFC). Forty-six percent of the SNPs were associated with a single unambiguous identified BAC clone. PCR amplification and next-generation sequencing of individual BAC clones confirmed the IFC clone identification. Utilization of the Fluidigm Dynamic array platform allowed for the simultaneous PCR screening of 10,752 BAC pools for 96 SNP tag sites in less than three hours at a cost of ~$0.05 per reaction.
机译:细菌人工染色体(BAC)库对于鉴定全长基因组序列,关联遗传图谱和物理图谱以及比较基因组学至关重要。在这里,我们描述了Fluidigm访问阵列基因分型系统与KASPar基因分型技术结合使用,以从Amplicon Express七板超级池A菜软骨细胞BAC库中识别与特定单核苷酸多态性(SNP)相对应的单个BAC克隆。使用单个Fluidigm集成流体芯片,同时测试了四个跨BAC超级池(对应于28384孔板)的跨跨A.hypochondriacus连锁组1、2和15的长度的96个SNP位点的克隆鉴定( IFC)。 46%的SNP与单个明确的BAC克隆相关。单个BAC克隆的PCR扩增和下一代测序证实了IFC克隆的鉴定。利用Fluidigm Dynamic阵列平台,可在不到三小时的时间内对10,752个BAC库进行96个SNP标签位点的同时PCR筛选,每个反应的成本约为0.05美元。

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