Entering edit mode
5.5 years ago
sabaghianamir70
▴
70
Hi every one. i did rna seq analysis. in PER3 gene and PER4 pseudogene i didnt get any counts, but in IGV i saw some small peaks which means they have some counts, even very low, but still they have !!. i want to know is there any way i can get any counts from that ? were my options in my aligner wrong or what else ?
i used blood samples. and used with trimmomatic, STAR, featureCounts
may be there is a low MAPQ for those reads . Use
samtools view in.bam "chr1:234-567"to explore the reads in the region of the gene.Duplicate of What is the best tool for estimate the counts of genes with very low expression rate ?
i know these two are similar. but im make my point more clear this time. thank you anyway
Did you try
salmon? I think it is still the best option to make use of problematic reads such as multimappers.since i working in galaxy plat form . working with galaxy is a little confusing and different from other tools i used. because it using data without needing to aligner. what the exact steps of Salmon ? i mean after trimming. we use salmon and featureCounts? i dont know what workflow should i use
Why don't you just try it first? It's right there on Galaxy. Try it and then you can come back with specific questions.