Has anyone had trouble shearing formaldehyde crosslinked chromatin to small enough fragments to go into Illumina library prep? Our protocol calls for shearing to 200-300 bp fragments after crosslinking but it seems that we can't breakup the chromatin to anything less the ~800 bp by Bioanalyzer. We have tried traditional sonicator and Covaris. What are we doing wrong?
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Hi,
I wonder which protocol you used to shear chromatin using Covaris? I have attached our two updated protocols. One is for using SDS based buffers, and one is for using non-ionic detergent based buffers. Please prepare your samples according to one of the protocols, and let me know how it works for you.
Thank you
Hamid
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Hi,
The new SDS-based buffer protocol works just as well now, so you are welcome to try either protocol. My suggestion would be to use a sample volume of 500ul in the TC12 tubes.
What is the cell type, and cell number you are using in this experiment?
Thank you
Hamid
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To me it sounds like you've overcrosslinked your chromatin. What is your crosslink strategy?
Also, I know with the bioruptor the tube choice makes a difference. Some tubes barely let any of the sonic energy through the tube wall. The TPX tubes from diagenode so far are the best. Since the TPX plastic is used in high sound frequency applications so it makes sense that it is the best.
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hmmm. Interesting. We crosslink (thymocytes) at 1x10^6 cell/mL in 1% formaldehyde for 10 min in a 37 degree air incubator with rotation. Then quench with 0.125M glycine for 10 min on ice.
Your conditions seem mild enough. But I can't help but think they are somehow overcrosslinked. Have your conditions worked in the past and give you a more reasonable 300bp avg frag size?
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by GATTACATLove this - good data definitely starts from good input, and poor input can only give relatively poor data. I particularly like the mention of Nanodrop/absorbance based methods for quantification. It's such a toss up if you'll get an accurate reading or what amounts to a randomly generated number, and a lot of library/sequencing related issues can be traced back to poor quant.
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by SEQadmin2
I’m not a sequencing expert. I’m a purification scientist who uses NGS to evaluate workflows my group develops. With this perspective, we think about the sample first and the NGS workflow second. The sequencer is an exceptionally honest reporter, but it can only report on what you give it, so whether you get clean, interpretable data from an NGS workflow is largely determined before you begin.
Here are nine questions we think about, in roughly the order they matter, before...-
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