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10.4 years ago
tejaswikoganti
▴
70
Hello,
I am trying to run Varscan somatic command for the first time. I have single tumor-normal mpileup file with reads only for certain regions on chr 17 and with a tumor purity of 50%. My command looks like this -
java -jar Varscan.jar somatic file.mpileup OUTPUT --mpileup 1 --tumor-purity 0.5
I encountered an error saying
Error: Invalid format or not enough samples in mpileup:
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I am not sure if this is because my file is really small. Has anybody else faced this problem?
Thank you!
Tejaswi
Hey Charles,
Can varscan somatic call be stored in vcf format. Because i could get output only in .snp and .indel.
Since some other downstream tools use vcf format. What tools did you use after u called somatic mutations.
thanks !
I just manually convert the file format for annotation in ANNOVAR.
I am only aware of the mpileup commands (mpileup2snp, mpileup2indel, mpileup2cns) having a parameter to produce .vcf files. However, I didn't develop the program, so it is possible that I missed something.
Thanks Charles !
I wanted to extract the read count that support the reference/variant call for each Normal/Tumor pair, to see if the variant is occurring in all or few libraries. There is readCount script from Varscan
But the problem is that I have assembled all Normal/Tumor for 5 patients in the same file. Do you know some easy way on how to get read count supporting reference/variant frequency for each patient. If not, I might just have to redo mpileup for each normal/tumor pair.
Thanks!
I would recommend asking your question on a VarScan discussion group.
I think the separate
.pileupfiles will work, but I'm guessing that this function won't really save you much time (since the pileup files already contain a coverage column). However, I honestly haven't tried this particular function.