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首页> 外文期刊>Nucleic Acids Research >TELP, a sensitive and versatile library construction method for next-generation sequencing
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TELP, a sensitive and versatile library construction method for next-generation sequencing

机译:TELP,一种灵敏且通用的下一代测序文库构建方法

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摘要

Next-generation sequencing has been widely used for the genome-wide profiling of histone modifications, transcription factor binding and gene expression through chromatin immunoprecipitated DNA sequencing (ChIP-seq) and cDNA sequencing (RNA-seq). Here, we describe a versatile library construction method that can be applied to both ChIP-seq and RNA-seq on the widely used Illumina platforms. Standard methods for ChIP-seq library construction require nanograms of starting DNA, substantially limiting its application to rare cell types or limited clinical samples. By minimizing the DNA purification steps that cause major sample loss, our method achieved a high sensitivity in ChIP-seq library preparation. Using this method, we achieved the following: (i) generated high-quality epigenomic and transcription factor-binding maps using ChIP-seq for murine adipocytes; (ii) successfully prepared a ChIP-seq library from as little as 25 pg of starting DNA; (iii) achieved paired-end sequencing of the ChIP-seq libraries; (iv) systematically profiled gene expression dynamics during murine adipogenesis using RNA-seq and (v) preserved the strand specificity of the transcripts in RNA-seq. Given its sensitivity and versatility in both double-stranded and single-stranded DNA library construction, this method has wide applications in genomic, epigenomic, transcriptomic and interactomic studies.
机译:下一代测序已广泛用于通过染色质免疫沉淀DNA测序(ChIP-seq)和cDNA测序(RNA-seq)对组蛋白修饰,转录因子结合和基因表达进行全基因组分析。在这里,我们描述了一种通用的文库构建方法,该方法可以应用于广泛使用的Illumina平台上的ChIP-seq和RNA-seq。 ChIP-seq库构建的标准方法需要纳克级的起始DNA,从而将其应用仅限于稀有细胞类型或有限的临床样品。通过最小化导致主要样品丢失的DNA纯化步骤,我们的方法在ChIP-seq文库制备中实现了高灵敏度。使用这种方法,我们实现了以下目标:(i)使用ChIP-seq生成鼠类脂肪细胞的高质量表观基因组和转录因子结合图; (ii)从低至25 pg的起始DNA成功制备了ChIP-seq文库; (iii)实现了ChIP-seq文库的配对末端测序; (iv)使用RNA-seq在鼠脂肪形成过程中系统地分析了基因表达的动力学,以及(v)保留了RNA-seq中转录本的链特异性。鉴于其在双链和单链DNA文库构建中的敏感性和多功能性,该方法在基因组,表观基因组,转录组和相互作用组学研究中具有广泛的应用。

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