Direct Cloning of Blunt-end PCR Fragments
BioTechniques 13:613
- Phenol extract the PCR product
- Ethanol precipitate
- Treat for 1hr at 37C with 10 units of T4 DNA polynucleotide kinase and 10 units T4
DNA polymerase I(NEB) in a 100ul reaction volume containing 50mM Tris-HCl
pH7.5, 10mM MgCl2, 1mM DTT, 50 ug/ml BSA, 1mM ATP, 200uM each dNTP.
I run the entire thing out on a 1.3% agarose TAE gel, cut a trough in front
of the band, pour in some 0.7% LMP agarose(BRL), run the product into it
and excise.
The PCR product in the LMP can be used for ligations directly, without
purification. The ligations take place at room temp on the benchtop.
I prepare the vector with minimal digestion (~2hr) then treat it with
shrimp alkaline phosphatase(USB). I usually prepare a stock of this vector
to have on hand, so I know it is good and will have a low background.
You may also want to try using an EcoRV cut vector instead of a Sma cut
vector.
- Remove the oil with Diethylether.
- To 40 ul of the PCR
reaction add 50 ul of H2O. Add 10 U T4 PNK, 10 U klenow, ATP (to 1 mM)
and some more dNTPs (usually 4 ul of 1.25 mM...whatever) and icubate at 37
oC for 30 min.
- Phenol/chloroform extract
- chloroform/IAA extrac
- EtOH precipitate
you can then just "shotgun" clone this DNA. However, if you have several
non-specific bands then you may want to gel purify the fragment first.
One point to note....
We have given up blunt end cloning into Sma I sites where possible.
Several people have reported problems with Sma I cut DNA. By choice we
clone into EcoRV sites.