Hi I am doing RNA editing analysis using REDItools. I have two data sets one is mRNAseq reads of 150bp and other is total RNAseq reads of 101 bps. Sample size is below 5 in each dataset and would like to combine them. Since alu index calculation is influenced by length i can not combine for calculating alu index . But I could do that for significance of differential RNA editing site calculation using wilcoxon rank test as we just use the frequency of editing in a particular site. Please let me know if this is right approach. can we combine them at all?