I am also looking for CNV detection in twin sequencing whole exom data. I found this project http://code.google.com/p/condr/

That looks very bare-bones but seems workable as long as you know what you're doing. Have you had any success running this? Do you think it would work for whole-genome sequencing input? Also, what kind of input does it take? I have aligned BAM.

I have illumina whole exom sequencing with nimblegen exom v2 enrichment. Paired end about 65bps. What type of data do you have? I don't have BAM alignment but I will use galaxy to get it. I havn't tried this code yet. I am going it if i find it appropriate. Did you get any results with CNVnator?

I have data from whole genome sequencing done using 90 bps paired-end reads. I have aligned it using bowtie with parameters specified by the authors of CNVer, who have suggested a CNV-focused alignment. The params are -v 2 -a -m 600 --best --strata

Upon converting from SAM to BAM after alignment, I installed root (that was quite the chore but somehow it worked). I then ran CNVnator using two bam files as the "tree" inputs, each one representing one set of the paired ends. Unfortunately I received an error that I am unable to decipher. I will post it here in a minute in a separate post. I'm not sure what I am doing wrong...I e-mailed the author, so hopefully I can figure out the issue. Apparently SegSeq is quite a good CNV tool, but very difficult to implement. If you or anyone else have success with something that would be useful for twin CNV comparisons, please share (I will do the same). Thanks.

Here is the error:

Assuming BAM file ...
terminate called after throwing an instance of 'std::bad_alloc'
what(): St9bad_alloc
/campus/apps/amd64_linux26/packages/torque-2.4.8/var/mom_priv/jobs/7319.localhost.localdomain.SC:
line 10: 30301 Aborted ./cnvnator -root
/output_folder/BAM_output.root -tree /input_folder/input_file1.bam
/input_folder/input_file2.bam

So you have samples sequencing data from twin? you interested in finding shared cnv or nonconcordant cnv? can you clarify?

I am interested in finding both, but the most important ones we want are nonconcordant CNV's. One twin has cancer, the other does not. We want to know CNV's responsible for this. It also would help to call concordant ones simply for validation however.

Has anyone had any success with FREEC? This seems to have the capability to do the trick.

do you know if they are monozygotic or dizygotic twin? either case they would be very similar genotypically. Theoritically how much of their exom would be concordant based on knowing the'r twin? taking into account sequencing noise? how much background noise do you think there is generally in exom sequencing?