We have been having a really difficult time with Chip-Seq experiments in which we get 70% or more of our reads located in exons.
Also, our 'control' sample of DNA isolated without antibody (which should be all of the DNA) looks very similar (in terms of aligned reads) to our sample in which only DNA attached to transcription factor pulled down with Ab should be present. That is, control and treatment look very much alike when viewing aligned reads.
However, the above is not what we get when we do PCR on the samples before they are sequenced. In this case, when doing PCR around a gene expected to have TF binding we get the expected results of DNA in specific 5' regions and not in exons when using Ab, and DNA in both exons and 5' regions when no Ab.
Has anyone had a similar problem or have any insights ? Has anyone sequenced exons when doing Chip-Seq ?
Also, our 'control' sample of DNA isolated without antibody (which should be all of the DNA) looks very similar (in terms of aligned reads) to our sample in which only DNA attached to transcription factor pulled down with Ab should be present. That is, control and treatment look very much alike when viewing aligned reads.
However, the above is not what we get when we do PCR on the samples before they are sequenced. In this case, when doing PCR around a gene expected to have TF binding we get the expected results of DNA in specific 5' regions and not in exons when using Ab, and DNA in both exons and 5' regions when no Ab.
Has anyone had a similar problem or have any insights ? Has anyone sequenced exons when doing Chip-Seq ?
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