Generating and Amplifying Adenoviral Constructs
From Bridges Lab Protocols
Revision as of 18:53, 14 September 2010 by Davebridges (Talk | contribs) (Added linearlization and transformation protocols)
Materials
- Targetting Construct in pAdtrack vector or the like (see Preparing an Adenoviral shRNA Clone )
- PmeI restriction enzyme (or other enzyme as required for linearization.
- PacI restriction enzyme
- Electrocompetent BJ5183-AD-1 cells (Agilent Cat#200157; or prepare yourself)
- 7.5 M ammonium acetate
- 20mg/mL glycogen
- 25:24:1 phenol/chloroform/isoamyl alcohol, pH 8.0
- 100% ethanol
- 2 mm electroporation cuvette
Protocol
see Nature Protocols, Current Protocols in Human Genetics protocols.
Linearization and Purification of Shuttle DNA
- Digest 0.2-0.5 ug plasmid DNA in 100 uL volume with 30-100U of PmeI overnight at 37C. If desired check a small amount by electrophoresis to ensure complete ligation.
- Add 100 uL ddH2O, 100 uL 7.5 M ammonium acetate and 2 uL 20 mg/ml glycogen.
- Add 300 uL 25:24:1 phenol/chloroform/isoamyl alcohol, pH 8.0.
- Remove top layer to clean tube and add 600 uL of 100% ethanol
- Centrifuge 5 min at 13 000 RPM
- Wash three times with 70% ethanol to remove residual salt.
- Dry and resuspend in 8 uL
Transformation into BJ5183-AD-1 cells
- Add 8 uL resuspended linearized plasmid to 20 uL electrocompetent cells
- Carefully transfer to ice cold 2 mm electroporation cuvette avoiding bubbles and keeping on ice
- Electroporate at pulse at 2,500 V, 200 O and 25 mF
- Resuspend in 500 uL LB and plate on 2-5 LB/Km plates
- Pick 10-20 of the smallest colonies the next day and grow in LB/Km broth
- Miniprep clones. Digest 10 uL with PacI and check size by running out both digested and undigested clones on a 0.8% agarose gel. Correct recombinants usually yield a large fragment (approximately 30 kb) and a smaller fragment of 3.0 or 4.5 kb.
- Retransform and amplify correct clone(s).