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Hi all,
I am using HTseq-count to count reads in my bam files. I used ncbi mouse annotation file.
I wonder which feature type (third column of gff3 file) I should use?
My understanding of how htseq count reads is that if I choose 'exon', then it will count reads only mapping to exons and sum those up for a gene. If I choose 'gene', it will count all the reads mapping to introns and exons of that gene. Theoretically, for RNAseq I should choose exons, and ignore reads mapping to introns.
In my sample, I know I knock out the gene ext1. I tried both choices and used DEseq2 to do differential expression analysis. In my results which I chose the 'gene' feature, the ext1 gene was the most significant gene. However, in the results for choosing 'exon', there are over 200 genes more significant than ext1. So now I am confused, it seems that the 'gene' feature are better than 'exon'? Anyone has this situation before? thanks.
I am using HTseq-count to count reads in my bam files. I used ncbi mouse annotation file.
I wonder which feature type (third column of gff3 file) I should use?
My understanding of how htseq count reads is that if I choose 'exon', then it will count reads only mapping to exons and sum those up for a gene. If I choose 'gene', it will count all the reads mapping to introns and exons of that gene. Theoretically, for RNAseq I should choose exons, and ignore reads mapping to introns.
In my sample, I know I knock out the gene ext1. I tried both choices and used DEseq2 to do differential expression analysis. In my results which I chose the 'gene' feature, the ext1 gene was the most significant gene. However, in the results for choosing 'exon', there are over 200 genes more significant than ext1. So now I am confused, it seems that the 'gene' feature are better than 'exon'? Anyone has this situation before? thanks.
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