If you are using magnetic beads, you don't need to do centrifugation. it would be separated by a magnet only. In the case of agarose beads, you would need centrifugation.

6 in-depth lecture slides couldn't help with what you did in 4 minutes! Thank you so much.

BEST EXPLANATION I'VE GOTTEN! THANK YOU!

Very good explanation, thank you so much, and the diagrams are so neatly-drawn too! Was so confused about co-IP and IP before this haha. Thank you!

You save me! Really thank you Your video is precious!!

The best explanation l have found. Thank you

Great video! Super clear and easy to follow... I also liked your diagrams. Thanks for sharing

Lovely diagrams and nice clear explanation!

hello! thank you very much for posting these explanations on youtube. just watched the long term potentiation (LTP) and this one about CO-IP and it helped me a lot! just subscribed :)

Im a medical student,Thank you so much for this video❤️❤️❤️❤️it helps a lott!

Very useful and excellent explanation. Thanks a lot 👌

Can you please explain how beta actin will be present in the lysates when we only pulled our protein of interest with the beads, all other proteins will be in the supernatant which we will discard or not use for this particular gel. We will run only those proteins which are in pellet and i think beta actin wont be presnt in pellet?

This was PERFECT! Thank you! Also you have very nice handwriting!

Thank you so much for the clear explanation! You saved my course!!!!

thanks this is short, concise and logical, made it easy to understand

OH MY GOD THIS IS SO GOOD!!!!!!!!!!!!!!!!!!!! THANK YOU!!!!!!!!!!!!!

Thanks a lot. your videos are really helpful for young researchers.

If we dont know which protein is interacted with Protein A then how we can use the antibody against the unknown protein. In this case we can only go for sequencing the SDS PAGE bands interacted with Protein A

Thanks for explanation! It was really helpful

YOU SIR ARE GENIUS !

Lourd la vidéo, ça m'a mis bien 👍

very helpful video, the only video explains co-IP with western blot!

thanks a lot! from Argentina!!

a very straightforward video ! thanks a lot !

Love your hand drawing!

Nicely explained explained. Could have been better if the importance of running input in the same gel was also given.

Very nice presentation

Co-immunoprecipitation (Co-IP) is a popular technique to identify physiologically relevant protein-protein interactions by using target protein-specific antibodies to indirectly capture proteins that are bound to a specific target protein.

THANKS! NOW I CAN UNDERSTAND A PAPER THAT I HAVE TO READ xD

Thank you so much for this clear explanation!

Explained very clearly thank you!

4:53 how will you get any B-actin band from an immunoprecipitated sample? if b-actin is present this simply means that b-actin is also interacting with the protein A, which is WRONG!

Thank you man, it will facilitate my presentation. You are the best :))

Super useful, thank you !!

Helpful 👌

The difference between Pull-down and CoIp is that pull-down using solution from eluted beads, and CoIp uses the precipitate after centrifuge. Then both of them go to SDS-PAGE, is that right?

good job brah...keep uploading

I don't understand why we need a second antibody for protein B! Would it not show anyway on the SDS Page? Or did I miss something?!

Where is protein A on the blot? How is A not blotted?

So helpful, thanks!

It's fantastic thanks!

Thank you for this video.

Thanks for the very nice video. But I have a question. How can we detect unknown protein bound to the know protein in co immunoprecipitation ?

thank you

how do you justify the pH of the buffer to make sure that protein A and B are not dissociated?

Thank you, sir :)

thank you!

thank you brother!

Thanks

r u from Presidency? very good keep up the good work bro..👍

How we select antibody for a protein, How we can sure that our antibody interact with our protein??

Do you have this information from a source? If so, which one? Can you send me the link please

actin is used just to make sure the proteins you are testing presence for were loaded correctly on the blot?

great explanation

Amazing explanation, however, isn't this an in-vitro technique? Literally everything is happening outside of the body, in a test tube etc. Thanks, nonetheless.

Who teaches better? A. Your professor majored in biotechnology with 10+ years teaching experience Or B. A random indian boi on youtube

does this only work for covalent interactions?

you save me!

Do you pull down beta actin too with the beads? How do you get beta actin in an IP blot?

tell me are u from India? what is that accent??? i need to know

Sir it is in vitro technique????

QuickQuestion You are studying 3 proteins (A, B and C). You hypothesize that A binds to B (forming a complex AB) but not C. From the scientific literature you know that B does not interact with C. 1) You are able to obtain 100% pure preparations of proteins A, B and C. Which experimental technique would you use to prove/disprove your hypothesis? Describe the experiment and the expected results

What is the purpose of using beta actin in this assay sir?

good presetation, except some accent, but it's good. thanks.

so by this way you describe yo identify the complex AB not their interaction as say !!!

what is this accent ?