Recent technical advancements have facilitated the mapping of epigenomes at single-cell resolution; however, the throughput and quality of these methods have limited their widespread adoption. Here we describe a high-quality (10(5) nuclear fragments per cell) droplet-microfluidics-based method for single-cell profiling of chromatin accessibility. We use this approach, named 'droplet single-cell assay for transposase-accessible chromatin using sequencing' (dscATAC-seq), to assay 46,653 cells for the unbiased discovery of cell types and regulatory elements in adult mouse brain. We further increase the throughput of this platform by combining it with combinatorial indexing (dsciATAC-seq), enabling single-cell studies at a massive scale. We demonstrate the utility of this approach by measuring chromatin accessibility across 136,463 resting and stimulated human bone marrow-derived cells to reveal changes in the cis- and trans-regulatory landscape across cell types and under stimulatory conditions at single-cell resolution. Altogether, we describe a total of 510,123 single-cell profiles, demonstrating the scalability and flexibility of this droplet-based platform.
Droplet-based combinatorial indexing for massive-scale single-cell chromatin accessibility.
基于液滴的组合索引用于大规模单细胞染色质可及性分析
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作者:Lareau Caleb A, Duarte Fabiana M, Chew Jennifer G, Kartha Vinay K, Burkett Zach D, Kohlway Andrew S, Pokholok Dmitry, Aryee Martin J, Steemers Frank J, Lebofsky Ronald, Buenrostro Jason D
| 期刊: | Nature Biotechnology | 影响因子: | 41.700 |
| 时间: | 2019 | 起止号: | 2019 Aug;37(8):916-924 |
| doi: | 10.1038/s41587-019-0147-6 | 研究方向: | 细胞生物学 |
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