Linganisha mbinu
Pitia mbinu ulizochagua bega kwa bega; safu zinazotofautiana zinaangaziwa.
| Uchanganuzi wa Kuonyesha Tofauti kwa RNA-seq ya Kiini Kimoja× | Uchambuzi wa Utekelezaji Tofauti wa RNA-seq× | |
|---|---|---|
| Nyanja | Bioinformatiki | Bioinformatiki |
| Familia | Process / pipeline | Process / pipeline |
| Mwaka wa asili≠ | 2013–2015 (first scRNA-seq DE tools; refined 2015–present) | 2008–2010 (RNA-seq DE methodology established) |
| Mwanzilishi≠ | Pioneered through Seurat (Satija lab) and scde (Kharchenko lab) frameworks, building on bulk RNA-seq DE foundations | Multiple groups; foundational methods from Anders & Huber (DESeq, 2010), Robinson, McCarthy & Smyth (edgeR, 2010) |
| Aina≠ | Computational bioinformatics pipeline | Quantitative genomics pipeline |
| Chanzo asilia≠ | Butler, A., Hoffman, P., Smibert, P., Papalexi, E., & Satija, R. (2018). Integrating single-cell transcriptomic data across different conditions, technologies, and species. Nature Biotechnology, 36(5), 411–420. DOI ↗ | Love, M. I., Huber, W., & Anders, S. (2014). Moderated estimation of fold change and dispersion for RNA-seq data with DESeq2. Genome Biology, 15(12), 550. DOI ↗ |
| Majina mbadala | scRNA-seq DE, single-cell differential expression, scDE, cell-level differential expression analysis | RNA-seq DE analysis, transcriptomic differential expression, bulk RNA-seq DE, DEA |
| Zinazohusiana≠ | 5 | 6 |
| Muhtasari≠ | Single-cell RNA-seq differential expression (scRNA-seq DE) analysis identifies genes whose expression levels differ significantly between defined groups of individual cells — such as cell types, disease states, or treatment conditions. Unlike bulk RNA-seq, which averages signals across millions of cells, scRNA-seq DE operates on the transcriptome of each individual cell, enabling fine-grained characterization of cell-population-specific gene regulation and heterogeneity within seemingly homogeneous tissue. | RNA-seq differential expression (DE) analysis identifies genes whose transcript abundance differs significantly between two or more biological conditions — for example, treated versus control, or diseased versus healthy tissue. Starting from raw sequencing reads, the pipeline moves through alignment, count-based normalization, statistical modeling of count dispersion, hypothesis testing, and multiple-testing correction to produce a ranked list of differentially expressed genes accompanied by fold-change estimates and adjusted p-values. |
| ScholarGateSeti ya data ↗ |
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