| Article ID | Journal | Published Year | Pages | File Type |
|---|---|---|---|---|
| 2090299 | Journal of Microbiological Methods | 2011 | 7 Pages |
Molecular tools for Gram-positive bacteria such as Mycobacterium are less well-developed than those for Gram-negatives such as Escherichiacoli. This has slowed the molecular-genetic characterisation of Mycobacterium spp, which is unfortunate, since this genus has high medical, environmental and industrial significance. Here, we developed a new Mycobacterium shuttle vector (pMycoFos, 12.5 kb, KmR) which combines desirable features of several previous vectors (controllable copy number in E. coli, inducible gene expression in Mycobacterium) and provides a new multiple cloning site compatible with large inserts of high-GC content DNA. Copy number control in E. coli was confirmed by the increased KmR of cultures after arabinose induction and the greater DNA yield of vector from arabinose-induced cultures. Measurement of beta-galactosidase activity in pMycoFos clones carrying the lacZ gene showed that in Mycobacterium smegmatis mc2-155, expression was inducible by acetamide, but in E. coli EPI300, the expression level was primarily determined by the vector copy number. Examination of protein profiles on SDS–PAGE gels confirmed the beta-galactosidase assay results. Construction of a fosmid library with the new vector confirmed that it could carry large DNA inserts. The new vector enabled the stable cloning and expression of an ethene monooxygenase gene cluster, which had eluded previous attempts at heterologous expression.
► A new cloning vector for Mycobacterium spp has been made which combines the desirable features of several previous vectors. ► The new vector provides plasmid copy number control in E. coli and inducible expression of cloned genes in Mycobacterium. ► The properties of the new vector were confirmed by beta-galactosidase assays and SDS–PAGE using a cloned lacZ gene. ► The ability of the new vector to carry large DNA inserts was confirmed. ► The vector enabled expression of a monooxygenase enzyme which had resisted previous attempts at cloning and expression.
