Entering edit mode
14 months ago
Meghna
▴
10
I am trying to convert FASTA sequences for SARS CoV-2 from GISAID into read counts matrix for RNA-seq analysis. I tried doing the same on galaxy after assigning dummy scores to my fasta file to convert it to fastqc format and then aligning my reads with hisat 2 to the SARS cov-2 Wuhan genome but when I finally try to find the counts with FeatureCounts and put the Annotation file for SaRS Cov 2 from GENCODE I am not getting any mapped reads. All my reads are showing unmapped. I am really clueless on how to do it.Will be really grateful if someone can help me out
Sometimes I feel like the word "convert" needs to be banned on the forum. Can you convert a carrot into a salad? Or a piece of paper into an education? In the same way, you cannot convert a "fasta" into anything. Please use the right words. And when you go on a quest to understand the word you need to describe the process, answers will become clear to you without you having to ask anyone.
You mean RNA seq?
Yes I wanted to do RNA seq analysis with data from GISAID but thats a DNA data so it won't be possible