CLONING PROBLEM!!! - no DNA after ligation!!!!! (May/18/2010 )

hello everyone!!!!!

I have a problem with my cloning. I cut my vector with BamHI, I do heat inactivation, I purify it with a Nucleospin column and then I run a gel, where I have enough DNA. After that I make the ligation and next day I run a small amount of the ligation and I see no vector at all!!!!

Any ideas??????? Thank you!!!!!

How much DNA are you loading on your gel. Two things are different about your post-ligation gel band -- it likely has much less DNA (you've diluted it and run only a fraction), and likely your ligation has produced complex products which are spread out over the gel, making individual bands difficult to see. 10-20 ng per band is typically easy to see on a gel. Less than that is tricky. Running a post-ligation gel is not the easiest way to tell if a ligation is working (except for very controlled circumstances).

And you can't heat inactivate BamHI.

phage434 on May 18 2010, 02:00 PM said:

Actually that was the only ay to check if there is any DNA in my ligation reaction, because I get no colonies after the electroporation and I have checked every step one by one. So, I run 4ul from a 10ul ligation reaction.

biochemistry23 on May 18 2010, 01:24 PM said:

Use your ligation reaction as template for PCR. Use primers specific to the vector just outside the cloning site. A small product indicates empty vector, a larger product indicates an insertion, no product points to no ligation.

What concentrations of DNA are you adding to your ligation reactions?

fishdoc on May 18 2010, 08:30 PM said:

I usually add 100ng of the vector.

biochemistry23 on May 18 2010, 04:10 PM said:

You're not inserting anything, just trying to ligate the empty vector?

fishdoc on May 19 2010, 01:08 AM said:

Exactly! I am just trying to religate the vector in order to check me new ligase.