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| Peak-kaldelse i single-cell ChIP-seq× | Single-cell sekvensjustering× | |
|---|---|---|
| Fagområde | Bioinformatik | Bioinformatik |
| Familie | Process / pipeline | Process / pipeline |
| Oprindelsesår≠ | 2019 | 2013–2016 |
| Ophavsperson≠ | Grosselin et al.; Ku et al. (parallel independent development) | Adapted from bulk RNA-seq aligners; single-cell extensions by Dobin et al. (STAR) and 10x Genomics Cell Ranger team |
| Type≠ | Epigenomic profiling pipeline | Computational pipeline step |
| Oprindelig kilde≠ | Grosselin, K., Durand, A., Marsolier, J., Poitou, A., Marangoni, E., Nemati, F., ... & Vallot, C. (2019). High-throughput single-cell ChIP-seq identifies heterogeneity of chromatin states in breast cancer. Nature Genetics, 51(6), 1060-1066. link ↗ | Dobin, A., Davis, C. A., Schlesinger, F., Drenkow, J., Zaleski, C., Jha, S., Batut, P., Chaisson, M., & Gingeras, T. R. (2013). STAR: ultrafast universal RNA-seq aligner. Bioinformatics, 29(1), 15–21. DOI ↗ |
| Aliasser | scChIP-seq peak calling, single-cell chromatin profiling, scChIC-seq analysis, single-cell epigenomic peak detection | scRNA-seq alignment, single-cell read mapping, scSeq alignment, cell barcode-aware alignment |
| Relaterede≠ | 5 | 1 |
| Resumé≠ | Single-cell ChIP-seq peak calling is a bioinformatics pipeline that identifies genomic regions enriched for histone modifications or transcription factor binding in individual cells. By profiling chromatin states at single-cell resolution, it reveals epigenomic heterogeneity hidden in bulk ChIP-seq experiments, enabling researchers to map regulatory landscapes across distinct cell populations within a complex tissue sample. | Single-cell sequence alignment is the computational step that maps millions of short sequencing reads produced by single-cell RNA-seq experiments back to a reference genome or transcriptome. Unlike bulk RNA-seq alignment, each read carries a cell barcode and a Unique Molecular Identifier (UMI) that together identify the originating cell and the individual RNA molecule. Accurate alignment and barcode demultiplexing are prerequisites for constructing the cell-by-gene count matrix that drives all downstream single-cell analyses. |
| ScholarGateDatasæt ↗ |
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