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首页> 外文期刊>Nucleic Acids Research >Multiplex sequencing of paired-end ditags (MS-PET): a strategy for the ultra-high-throughput analysis of transcriptomes and genomes
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Multiplex sequencing of paired-end ditags (MS-PET): a strategy for the ultra-high-throughput analysis of transcriptomes and genomes

机译:配对末端双标签(MS-PET)的多重测序:转录组和基因组的超高通量分析策略

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The paired-end ditagging (PET) technique has been shown to be efficient and accurate for large-scale transcriptome and genome analysis. However, as with other DNA tag-based sequencing strategies, it is constrained by the current efficiency of Sanger technology. A recently developed multiplex sequencing method (454-sequencingTM) using picolitre-scale reactions has achieved a remarkable advance in efficiency, but suffers from short-read lengths, and a lack of paired-end information. To further enhancethe efficiency of PET analysis and at the same time overcome the drawbacks of the new sequencing method, we coupled multiplex sequencing with paired-end ditagging (MS-PET) using modified PET procedures to simultaneously sequence 200 000 to 300 000 dimerized PET (diPET) templates, with an output of nearly half-alpha-million PET sequences in a single 4 h machine run. We demonstrate the utility and robustness of MS-PET by analyzing the transcriptome of human breast carcinoma cells, and by mapping p53 binding sites in the genome of human colorectal carcinoma cells. This combined sequencing strategy achieved an approximate 100-fold efficiency increase over the current standard for PET analysis, and furthermore enables the short-read-length multiplex sequencing procedure to acquire paired-end information from large DNA fragments.
机译:配对末端双标签(PET)技术已被证明对于大规模转录组和基因组分析是有效和准确的。但是,与其他基于DNA标签的测序策略一样,它受到Sanger技术当前效率的限制。最近开发的使用皮脂级反应的多重测序方法(454-sequencingTM)在效率方面取得了显着进步,但存在读取长度短和缺乏配对末端信息的问题。为了进一步提高PET分析的效率并克服新测序方法的弊端,我们使用改良的PET程序将多重测序与配对末端双标签(MS-PET)结合使用,以同时测序20万至30万个二聚化PET( diPET)模板,在一次4小时的机器运行中就输出了近半百万个PET序列。我们通过分析人类乳腺癌细胞的转录组,并在人类结肠直肠癌细胞基因组中定位p53结合位点,证明了MS-PET的实用性和鲁棒性。与目前用于PET分析的标准相比,这种组合测序策略实现了大约100倍的效率提高,并且使短读长多重测序程序能够从大的DNA片段中获取配对末端信息。

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