Hi all,
Not sure if this is the proper forum, but here goes. We did our first RNAseq analysis of a fungal genome. We had 2 conditions (stress and non-stressed) and 2 time points with three biological replicates of each condition and time point. One of the time points was also represented on a microarray experiment (Aglilent arrays) done with the same genome under the same conditions.
I used edgeR to determine the DE genes. There were ~1200 genes DE on the microarray and ~2000 DE for the same time point in the RNAseq experiment. The overlap of DE genes was 590/1200. However the direction of the change was often different between them.
My questions:
1) If anyone done a comparison between an Agilient microarray and RNAseq, what sort of concordance was observed?
2) The edgeR was done after RPKM normalization. How much does that affect the number of DE genes? I have the BAM files from the Bowtie alignment so I can redo the edgeR starting from non-normalized counts.
3) Is it even worth spending time trying to determine the level of concordance because these technologies are too different to compare?
I did see a recent paper in BMC Genomics comparing Affy exon arrays with RNAseq and they found a fairly high level of concordance.
Thanks in advance for any thoughts, comments or advice.
Regards,
Maureen
Not sure if this is the proper forum, but here goes. We did our first RNAseq analysis of a fungal genome. We had 2 conditions (stress and non-stressed) and 2 time points with three biological replicates of each condition and time point. One of the time points was also represented on a microarray experiment (Aglilent arrays) done with the same genome under the same conditions.
I used edgeR to determine the DE genes. There were ~1200 genes DE on the microarray and ~2000 DE for the same time point in the RNAseq experiment. The overlap of DE genes was 590/1200. However the direction of the change was often different between them.
My questions:
1) If anyone done a comparison between an Agilient microarray and RNAseq, what sort of concordance was observed?
2) The edgeR was done after RPKM normalization. How much does that affect the number of DE genes? I have the BAM files from the Bowtie alignment so I can redo the edgeR starting from non-normalized counts.
3) Is it even worth spending time trying to determine the level of concordance because these technologies are too different to compare?
I did see a recent paper in BMC Genomics comparing Affy exon arrays with RNAseq and they found a fairly high level of concordance.
Thanks in advance for any thoughts, comments or advice.
Regards,
Maureen
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