Did the bioanalyzer show the ChIP-DNA in a good size range (~100-700bp)?

Personally I don't understand why Illumina's ChipSeq kit uses an agarose gel band extraction. Even if you are pretty good at extracting DNA from agarose, it is good way to lose >90% of the DNA.

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Phillip

Hi Phillip,
thank you for your answer
yes the size of the fragment was fine according to the bioanalyser.
Did you succesfully run Chip seq without the gel extraction step?

thanks
Olivier

Any chance you could post the bioanalyzer chromatogram of your input DNA? I ask because we always run this as QC, but I never see example chromatograms in ChipSeq kit manuals of this step. (They always have a picture of the library, after PCR amplification, instead.)

We switched to the Bioo ChipSeq kit -- it doesn't use a gel extraction kit. I think that as a result of this it is able to specify 1 ng of input DNA.

That said, the libraries we made from the Illumina ChIPseq kit starting with 5ng of DNA were in the 40-60% duplicate read range. We did once make a set of libraries that had a similar level of duplication to yours -- but in most cases those started with an amount of DNA below the level of detection of the Qubit. (For one ul -- if we had used the entire sample, for fluorimetry we may have been able to detect its concentration. But there was no point doing that...)

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Phillip

bioanalyser data here:

sorry, the previous link is not working.
here:http://imgur.com/a/CRUzA

That is input? Wow, that looks great.

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Phillip