The extent splicing is regulated at single-cell resolution has remained controversial due to both available data and methods to interpret it. We apply the SpliZ, a new statistical approach, to detect cell-type-specific splicing in >110K cells from 12 human tissues. Using 10X Chromium data for discovery, 9.1% of genes with computable SpliZ scores are cell-type-specifically spliced, including ubiquitously expressed genes MYL6 and RPS24. These results are validated with RNA FISH, single-cell PCR, and Smart-seq2. SpliZ analysis reveals 170 genes with regulated splicing during human spermatogenesis, including examples conserved in mouse and mouse lemur. The SpliZ allows model-based identification of subpopulations indistinguishable based on gene expression, illustrated by subpopulation-specific splicing of classical monocytes involving an ultraconserved exon in SAT1. Together, this analysis of differential splicing across multiple organs establishes that splicing is regulated cell-type-specifically.
RNA splicing programs define tissue compartments and cell types at single-cell resolution.
RNA剪接程序以单细胞分辨率定义组织区室和细胞类型
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作者:Olivieri Julia Eve, Dehghannasiri Roozbeh, Wang Peter L, Jang SoRi, de Morree Antoine, Tan Serena Y, Ming Jingsi, Ruohao Wu Angela, Quake Stephen R, Krasnow Mark A, Salzman Julia
| 期刊: | Elife | 影响因子: | 6.400 |
| 时间: | 2021 | 起止号: | 2021 Sep 13; 10:e70692 |
| doi: | 10.7554/eLife.70692 | 研究方向: | 细胞生物学 |
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