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Amplification-free library preparation with SAFE Hi-C uses ligation products for deep sequencing to improve traditional Hi-C analysis

机译:使用SAFE Hi-C进行的无扩增文库制备使用连接产物进行深度测序以改善传统的Hi-C分析

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摘要

PCR amplification of Hi-C libraries introduces unusable duplicates and results in a biased representation of chromatin interactions. We present a simplified, fast, and economically efficient Hi-C library preparation procedure, SAFE Hi-C, which generates sufficient non-amplified ligation products for deep sequencing from 30 million Drosophila cells. Comprehensive analysis of the resulting data shows that amplification-free Hi-C preserves higher complexity of chromatin interaction and lowers sequencing depth for the same number of unique paired reads. For human cells which have a large genome, SAFE Hi-C recovers enough ligated fragments for direct high-throughput sequencing without amplification from as few as 250,000 cells. Comparison with published in situ Hi-C data from millions of human cells demonstrates that amplification introduces distance-dependent amplification bias, which results in an increased background noise level against genomic distance. With amplification bias avoided, SAFE Hi-C may produce a chromatin interaction network more faithfully reflecting the real three-dimensional genomic architecture.
机译:Hi-C文库的PCR扩增引入了无法使用的重复项,并导致染色质相互作用的偏倚表示。我们提出了一种简化,快速且经济高效的Hi-C库制备程序SAFE Hi-C,该程序可生成足够的非扩增连接产物,用于从3000万果蝇细胞中进行深度测序。对所得数据的综合分析表明,对于相同数量的独特配对读段,无扩增的Hi-C保留了较高的染色质相互作用复杂性,并降低了测序深度。对于具有大型基因组的人类细胞,SAFE Hi-C可回收足够的连接片段,以直接进行高通量测序,而无需从多达250,000个细胞中扩增。与来自数百万个人类细胞的已发布原位Hi-C数据的比较表明,扩增引入了距离相关的扩增偏差,这导致相对于基因组距离的背景噪声水平增加。避免了放大偏差,SAFE Hi-C可以产生染色质相互作用网络,从而更忠实地反映真实的三维基因组架构。

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