Hi,
If we want to study interaction of two proteins in transcription, can we use mixture of antibodies in ChIP-seq experiment? Is there any references that I can read?
Thanks,
I do not see a computational aspect of this question, so you may be better off asking elsewhere. That being said, I cannot see how using a mixture of antibodies would allow you to study the interaction of two proteins in transcription. If you have two antibodies that each target a different transcription factors, your ChIP would pull down DNA fragments bound by either of the two transcription factors. It would to my knowledge not give you any information on which transcription factor(s) bound which fragment.
If you want to understand to which extent the two transcription factors target the same set of downstream genes, I think they way to go is to do separate ChIP-seq experiments for the two transcription factors and then subsequently computationally analyze which promotors are bound by both transcription factors.
Again, there is no computational aspect to this, but some people do sequential IP to get at protein interactions, see e g http://nar.oxfordjournals.org/content/32/19/e151.full
In principle you can. There is no specific reason why the mixture of antibodies would not work. And since you will eventually access the precipitated sequences themselves you might be able to make an educated guess which precipitated sequence comes from what transcription factor binding.
In ChIP-on-chip this is not unheard of. Since the chips are expensive to run you will want to maximize the amount of information you get from a single array. The trade off is likely different for ChIP-seq.
There may be specific reasons to combine antibodies though. Suppose it is really a complex you are looking at, and the binding of protein A is conditional for the binding of protein B, then you will only get signals for both TFs combined. This is something you might in fact want to study using 2 antibodies. Although you will still have to evaluate the binding sequences for each of them, you might even find that protein B doesn't have a binding sequence of it's own but only piggy backs on protein A.
I think you are right, the 2 antibodies alone are not sufficient for problems like this. You will want to combine that with other wetlab approaches, like using labeled anti-antibodies for detection of the complexes after separating those on a 2D gel. There might be smarter ways to do the same. In my example knockout of protein A should remove any ChIP effects for both A and B
But here is a real life example. Suppose the second TF is not really a TF but only complexes with the first. Then you will only see binding of the second antibody when you also see binding of the first, but not the other way around. Also you will only see effects on expression when both antibodies bind and thus the TF was bound and complexed. Or sometimes opposite effects if the complex is formed, from what you would see with the first antibody alone.
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Is there a bioinformatics/computational biology aspect to this question? If not, it would be better to ask in a molecular biology forum.