Step 2.2: Count generation
Protocol 2
Counts are already generated and can be skipped
Bibliography
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RNA-Seq data processing and gene expression analysis
Gene/transcript level counts generation
Below are two protocols for generation of gene- and transcript-level counts. Protocol 1 focuses on the classical alignment-based approach, whereas Protocol 2 uses recent advances in accelerated kmer-based 'pseudo-alignment'[1-3](#footnote1) approaches for assigning reads to transcripts, which has some distinct advantages to alignment methods but rely on having a comprehensive and reliably annotated transcriptome:
- Protocol 1: Alignment-based approach
- Protocol 2: Estimated counts using graph-based or similar approaches
Bibliography
- Patro, R., Mount, S. M., & Kingsford, C. (2014). Sailfish enables alignment-free isoform quantification from RNA-seq reads using lightweight algorithms. Nature biotechnology, 32(5), 462.
- Bray, N. L., Pimentel, H., Melsted, P., & Pachter, L. (2016). Near-optimal probabilistic RNA-seq quantification. Nature biotechnology, 34(5), 525.
- Patro, R., Duggal, G., Love, M. I., Irizarry, R. A., & Kingsford, C. (2017). [Salmon provides fast and bias-aware quantification of transcript expression. Nature methods, 14(4), 417.
Reads enumeration
Here, this step depends on the protocol you followed in the previous step:
Collecting & Tabulating stats
Again, this depends on the protocol you chose from the begining:
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This work is licensed under a Creative Commons Attribution-NonCommercial-ShareAlike 4.0 International License.
This work is licensed under a Creative Commons Attribution-NonCommercial-ShareAlike 4.0 International License.