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Cost-effective high-throughput single-haplotype iterative mapping and sequencing for complex genomic structures

机译:复杂基因组结构具有成本效益的高通量单倍型迭代映射和测序

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The reference sequences of structurally complex regions can be obtained only through highly accurate clone-based approaches. We and others have successfully used single-haplotype iterative mapping and sequencing (SHIMS) 1.0 to assemble structurally complex regions across the sex chromosomes of several vertebrate species and to allow for targeted improvements to the reference sequences of human autosomes. However, SHIMS 1.0 is expensive and time consuming, requiring resources that only a genome center can provide. Here we introduce SHIMS 2.0, an improved SHIMS protocol that allows even a small laboratory to generate high-quality reference sequence from complex genomic regions. Using a streamlined and parallelized library-preparation protocol, and taking advantage of inexpensive high-throughput short-read-sequencing technologies, a small laboratory with both molecular biology and bioinformatics experience can sequence and assemble 192 large-insert bacterial artificial chromosome (BAC) or fosmid clones in 1 week. In SHIMS 2.0, in contrast to other pooling strategies, each clone is sequenced with a unique barcode, thus enabling clones containing nearly identical sequences to be multiplexed in a single sequencing run and assembled separately. Relative to SHIMS 1.0, SHIMS 2.0 decreases the required cost and time by two orders of magnitude while preserving high sequencing accuracy.
机译:结构复杂区域的参考序列只能通过高精度的基于克隆的方法获得。我们和其他人已经成功地使用单倍型迭代映射和测序(垫片)1.0来组装几种脊椎动物物种的性染色体的结构复杂区域,并允许针对人常染色剂的参考序列进行靶向改善。然而,Shims 1.0昂贵且耗时,需要只有基因组中心提供的资源。在这里,我们介绍垫片2.0,一种改进的垫片协议,甚至允许一个小实验室从复杂的基因组区域产生高质量的参考序列。使用流线型和并行化库制备方案,并利用廉价的高通量短读取测序技术,具有分子生物学和生物信息学体验的小实验室可以序列和组装192个大插入细菌人工染色体(BAC)或Fosmid克隆在1周内。在Shims 2.0中,与其他池策略相反,每个克隆用唯一的条形码测序,从而使克隆能够在单个测序运行中与待多路复用的几乎相同的序列进行分离地组装。相对于垫片1.0,垫片2.0减少了两个数量级的所需成本和时间,同时保持高序列精度。

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