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**huguesparri** · 02-23-2010, 01:48 AM

Hello jb1,
Size selection on a ChIP Seq library preparation occurs before the PCR.
Adapters sequence at this step are only 68nt long (34*2). So your DNA fragment of interest is 132 +/-25 nt long.
As you can see, it's close to the maximum enrichment size of your fragmentation.
Moreover, even if at the end of the sonication the maximum enrichment size is beetween 150 and 300 pb (and even higher), there is a lot of lower size DNA in the smear.
In the end, as long as your fragmentation is random, libraries generated this way are ok and reprensentative of your total ChIPed material.

**jb1** · 02-23-2010, 02:10 PM

Thanks for your reply, that really clears things up. I will aim for fragments of 132bp on sonication!

**huguesparri** · 02-23-2010, 02:33 PM

You can also try to cut your gel at higher size (like 250+/-25) to be sure to be in the enriched region.
It shouldn't affect the sequencing process.

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