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Akula, Nirmala NIH/NIMH [C]
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190
@akula-nirmala-nihnimh-c-5007
Last seen 5.1 years ago
Based on the previous threads when using DESeq the reads should not be
double counted. I am following pipeline for RNA-seq analysis and would
like to know any suggestions/comments regarding the pipeline:
1. Mapping the reads using Tophat
2. Convert Tophat output.bam to Sam
3. Create bed file from Sam file
4. Use CoverageBed along with reference genome for counting the
reads
5. Sum count of reads from all exons in a transcript
6. DESeq to analyze the counts/transcript
Thank you very much
Nirmala
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