CHARACTERIZATION OF A MINI COLE1 CLONING VECTOR

Plasmid pHA105 (formerly pAC105), a mini ColE1 plasmid containing one restriction endonuclease EcoRI site, was further characterized using restriction endonuclease analysis thereby revealing its relationship to ColE1. The polypeptides specified by plasmid pHA105 in minicells are of low molecular weight making it a useful plasmid to define cloned polypeptides larger than 16,000 daltons and its use for that purpose was demonstrated. pHA105 was used to clone two different sized fragments of DNA containing the gal operon. pHA105 was also used to reclone a 2 Mdal fragment of DNA that, when expressed, represses the synthesis of capsular polysaccharide. The repression of polysaccharide synthesis was expressed when a plasmid containing one molecule each of pHA105 and the 2 Mdal fragment was prepared (pFM100). In contrast, a plasmid containing two copies of pHA105 and one of the 2 Mdal fragment (pHA138) did not repress polysaccharide synthesis. The results demonstrate that expression of a cloned fragment gene may be prevented in certain arrangements of the vector and cloned fragment. Plasmid pHA105 fails to exhibit relaxation after treatment with sodium dodecyl sulfate in contrast to ColE1 treated in the same way. pHA105 replicates as a dimer form while ColE1 usually does not. A hypothesis that a function of a DNA-protein complex is required for monomeric DNA circle formation is discussed. © 1979.