Dear All,
I have a ~2300 bp insert with Snabl and NotI respectively( 5 prime to 3 prime). I need to use pPIC9 expression vector which is 8 kb in size. I co digested pPIC9 with SnabI and NotI, gel purified and ligate with my insert. 50 ng of vector and 4:1 insert to vector molar ratio i used for the ligation. Initial incubation at 25 for 2 hours following over night incubation at 4 degree . I took 5 ul of ligation mixture after 48 hours ligation period, transformed in DH5aplha, mini preped and screened with Snabl and NotI. I got nothing. This is the third time I am doing. SnabI produce blunt end where Notl produces sticky end. Can you share your opinion? Am I doing anything wrong?