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I am planning for to do a ChIP-seq with chromatin prepared from embryonic sample(E7.5 mouse embryo). For fixing the protein-DNA complex I have used 1% Formaldehyde @ 37 C for 10min.
Sonication cycle= 30 seconds ON and 30 seconds
No of cycles= 60
But still after such high number of cycles I am unable to get the desired fragment size of 200-400bp for ChIP seq.
What could be the possible modification I could do to improve the current situation?
Sonication cycle= 30 seconds ON and 30 seconds
No of cycles= 60
But still after such high number of cycles I am unable to get the desired fragment size of 200-400bp for ChIP seq.
What could be the possible modification I could do to improve the current situation?
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