Entering edit mode
9.4 years ago
manekineko
▴
150
Hi,
I have used default options in Galaxy (just set the Mean Inner Distance between Mate Pairs to 50 which I did not sure it is ok) to map my RNA-seq library to Human genome hg38. Is there a way to check is the mapping good and ok, for example check a housekeeping gene or a gene what I can see how should look like in IGV?
just open your bam file in IGV and check several genes. Don't forget to index it before open it in IGV (samtools index alignment_file.bam)
I see this - http://s22.postimg.org/4s9xmq4u9/Screen_Shot_2015_07_27_at_17_51_47.png
but cannot decide if it is normal or not for RNA-seq (as I work mainly with miRNAs not with RNA-seq so far :)
Seems OK to me. Are your data stranded?
R1 read is forwarded and R2 is reverse.
I mainly was worried for setting mean-inner-mate option in tophat as I have problems calculating it. I just know that my reads are 101bp, and the RNA was selected from fragments 300-400.So do not know how much a wrong
-r
option will harm the mapping. I see from the mapping there is a lot reads overlapping mates