Home Protocols Cloning with Thermolabile USER Enzyme Protocol (M5507)

Cloning with Thermolabile USER Enzyme Protocol (M5507)

1. Amplify your target DNA using Taq DNA Polymerase, or any other DNA Polymerase which is not inhibited by a dU-containing template, and uracil-containing primers.

2. Assembly Reaction:
Crude PCR Sample
  10 µl
Linearized pNEB206A (20 ng)
  1 µl
Thermolabile USER Enzyme (1 unit)
  1 µl
TOTAL VOLUME
  12 µl

3. Incubate for 15 minutes at 37°C.
4. Incubate for 15 minutes at room temperature.
5. Transform chemically competent E. coli cells with 2-12 μl of the assembly reaction from Step 4.

The cloned insert can be removed by BbvCI cleavage (NEB #R0601).