I have sequenced a 7 kb part of frog mtDNA and have generated a bam file of the sequence. In IVG, I can visualize manually the per base read coverage but I need this information in an excel format (.csv or xlsx) so that I can load it into R. Please suggest me way/s to do it.
Debjyoti Dutta
I have found an answer to this problem. Using galaxy the mpileup option lets you generate a file showing variants in vcf format. Viewing the data in galaxy will show you the raw read depth per base (DP). The output file will be in vcf or bcf format but it can be converted into tabular. I loaded the tabular file in R and created a .xslx file as an output. The raw read depth per base can then be accessed via excel file.
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