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. 1984 Dec;32(3):481-5.
doi: 10.1016/0378-1119(84)90022-2.

The pIC plasmid and phage vectors with versatile cloning sites for recombinant selection by insertional inactivation

Free article

The pIC plasmid and phage vectors with versatile cloning sites for recombinant selection by insertional inactivation

J L Marsh et al. Gene. 1984 Dec.
Free article

Abstract

The versatility of insertional inactivation of beta-galactosidase activity for subcloning and sequencing has been enhanced by combining a chemically synthesized oligonucleotide which specifies nine 6-bp-cutter restriction sites including BglII, XhoI, NruI, ClaI, SacI and EcoRV in various configurations with existing polylinkers to create a set of highly versatile cloning sites. These improved polylinkers have been inserted into plasmids (the pICs) for routine cloning of double-stranded DNA, and into chimeric phage/plasmids (the pICEMs) for biological production of single stranded DNA. The most versatile polylinker specifies 17 restriction sites in the beta-galactosidase alpha-complementing gene fragment. One of the new polylinkers was inserted into M13 DNA to produce a vector (M13mIC7) with nine cloning sites.

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