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高多重条码测序:一种用于并行分析混合样本的高效方法。

Highly-multiplexed barcode sequencing: an efficient method for parallel analysis of pooled samples.

机构信息

Department of Molecular Genetics, University of Toronto, 1 King's College Circle, Toronto, Ontario M5S 1A8, Canada.

出版信息

Nucleic Acids Res. 2010 Jul;38(13):e142. doi: 10.1093/nar/gkq368. Epub 2010 May 11.

Abstract

Next-generation sequencing has proven an extremely effective technology for molecular counting applications where the number of sequence reads provides a digital readout for RNA-seq, ChIP-seq, Tn-seq and other applications. The extremely large number of sequence reads that can be obtained per run permits the analysis of increasingly complex samples. For lower complexity samples, however, a point of diminishing returns is reached when the number of counts per sequence results in oversampling with no increase in data quality. A solution to making next-generation sequencing as efficient and affordable as possible involves assaying multiple samples in a single run. Here, we report the successful 96-plexing of complex pools of DNA barcoded yeast mutants and show that such 'Bar-seq' assessment of these samples is comparable with data provided by barcode microarrays, the current benchmark for this application. The cost reduction and increased throughput permitted by highly multiplexed sequencing will greatly expand the scope of chemogenomics assays and, equally importantly, the approach is suitable for other sequence counting applications that could benefit from massive parallelization.

摘要

下一代测序技术已被证明是一种非常有效的分子计数应用技术,其中序列读取的数量为 RNA-seq、ChIP-seq、Tn-seq 和其他应用提供了数字读数。每次运行可以获得的大量序列读取允许对越来越复杂的样本进行分析。然而,对于较低复杂度的样本,当每个序列的计数数量导致过度采样而没有提高数据质量时,就会达到收益递减的临界点。使下一代测序尽可能高效和经济实惠的解决方案涉及在单个运行中分析多个样本。在这里,我们报告了成功地对 DNA 条形码酵母突变体的复杂池进行了 96 重测序,并表明这种“Bar-seq”对这些样本的评估与条形码微阵列提供的数据相当,条形码微阵列是该应用的当前基准。高度多重化测序所允许的成本降低和通量增加将极大地扩展化学生物学测定的范围,同样重要的是,该方法适用于其他可能受益于大规模并行化的序列计数应用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e0a6/2910071/abaea859b916/gkq368f1.jpg

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