COSMID LIBRARY

1. Isolate chromosomal DNA by using the CTAB protocols in current Pr M R.
2. Make a CsCl preparation of pLAFr3 (or other appropriate cosmid).
3. Cut pLAFr with BamHI phenol ext. + ETOH preparation.
4. Partially digest a sample of chromosomal DNA as per Maniatis protocol (pp. 9.24 - 9.28) in order to maximize production of 20 kb plasmid.
5. Scale up the conditions (all of the conditions!!) to obtain 200 - 500 µg of cut DNA.
6. Prepare a 10 - 40% sucrose gradient as per Maniatis (pp. 2.85 - 2.87).
7. Pool fractions containing 20 kb fragments and, after adding 3 vol. of sterile dH₂O, prep. the DNA.
8. Set up ligations (Maniatis p. 3.29) to maximize the formation of concatomers.
9. Package via "Packagene" protocol. Plate the infected bacteria on LB Tet. plates. Remember: if you are using pLAFr, you are looking for colonies, NOT PLAQUES, since it is a cosmid.
10. Check a randomly selected group of transformants for the presence of inserts by restriction analysis.

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Updated 01 December 2000.