@mrfox

Did you find a workaround for this? I am also facing issues, am using ExomeCNV for first time, the bamcoverage.sh does not work well as they need old version of samtools, so I tried gatk DepthofCoverage. But it gives single output files. Can you tell me how to take them as input since the input are done on chromosome wise, so do we have to separate gatk DepthofCoverage output in different chromosome files and then put them as input? If so then can you tell me how are you doing it? And then how did you tackle the problem of >500 which will not work in exomeCNV. I would appreciate some help

I gave up finally and I used VarScan2. Sorry I am not able to help on ExomeCNV.

I have used VarScan2 on my data but does not give any inferring results, I have however had some sort of success with Control-FREEC, now am trying other tools that are useful in calling somatic CNV for normal/tumor pair data. So I came across exomeCNV and want to try it but I am battling with it for over 3 days now.