CLONING

 

Digestion and dephosphorylation of vector:

 

20 µl:

2 µl 10xrestriction buffer

2-4 µg vector

1 µl of each restriction enzyme

37C, ≥1h.

 

+ 75 µl ddw

5 µl 1M Tris-HCl pH 8.5

2 µl alkaline phosphatase (AP, Boehringer)

37C, ≥1h.

(If blunt or 3'overhangs, after incubation add 1µl AP and incubate at 50C for another 1 h.)

 

+ 5 µl 0.2M EDTA (pH 8)

Extract with Phenol:CHCl₃ (PCA) (leave 5-10 µl aqueous phase behind).

+ 10 µl 3M NaAc pH 6.0

1 µl 20 mg/ml glycogen

275 µl 100% EtOH

Ice ≥ 5 min

Spin 14,000 rpm, 15-30 min at 4C

Remove EtOH

Wash with 70% EtOH

Dry pellet

Dissolve at 0.1 mg/ml in Te buffer (10 mM Tris-HCl pH 8, 0.1 mM EDTA)

 

 

Preparation of insert:

 

PCR product:

Purify PCR product from agarose gel

To 50 µl of gel purified PCR product add:

5 µl 10xrestriction buffer

1-2 µl of each restriction enzyme

37C, ≥1h.

 

+ 45 µl ddw

5 µl 0.2M EDTA (pH 8)

Extract with PCA.

+ 10 µl 3M NaAc pH 6.0

1 µl 20 mg/ml glycogen

275 µl EtOH

Ice, ≥5 min.

Spin 14,000 rpm, 15-30 min

Remove EtOH.

Wash with 70% EtOH.

Dissolve in Te buffer (e.g. 10 µl Te for a 20 µl PCR rxn)

 

 

Plasmid insert:

20 µl:

2 µl 10xrestriction buffer

2-5 µg plasmid

1 µl of each restriction enzyme

37C, ≥1h.

 

+ 5 µl 5xDNA load buffer

Purify DNA fragment from agarose gel

Elute in 30 µl Te

 

 

Oligo insert:

Phosphorylate each oligo (in sepearate rxns):

10 µl:

1 µl 10xPNK

1 µl 50 mM DTT

200 pmole DNA oligo

2 µl 2 mM ATP

1 µl Polynucleotide kinase

37C, ≥1h.

 

Anneal by mixing the two phosphorylation rxns

95C, 2 min

RT, 5 min

Ice.

This will give an annealed oligo concentration of 10 µM.

Use 0.001-0.1 pmole for a ligation. The amount has to  be titrated every time as too high an oligo concentration results in multiple inserts.

 

 

Ligation:

 

10 µl:

1 µl 10xT4 DL

1 µl 50 mM DTT

1 µl 2 mM ATP

1 µl cut, cipped vector (≈0.1 mg/ml)

2-5 µl cut insert/PCR product or 0.001-0.1 pmole annealed, phosphorylated oligos (Titrate every time!)

0.2 units T4 DNA ligase (Boehringer)

 

RT, ≥4h.

 

Transform 2.5 µl to competent E. coli DH5a cells and plate on selection medium

Store remainder of ligation at -20C.

 

Buffers:

Te:

10 mM Tris-HCl pH 8

0.1 mM EDTA

 

10xT4 DL:

660 mM Tris-HCl pH 7.5

66 mM MgCl₂

 

10xPNK

500 mM Tris-HCl pH 7.5

100 mM MgCl₂

 

 

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JLA; Aug. 1, 2007