Xer Site-Specific Recombination,an Efficient Tool To Introduce Unmarked Deletions into Mycobacteria

Genetic manipulation of mycobacteria still represents a serious challenge due to the lack of tools and selection markers. In this report, we describe the development of an intrinsically unstable excisable cassette for introduction of unmarked mutations in both Mycobacterium smegmatis and Mycobacterium tuberculosis.Mycobacterium tuberculosis causes about 2 million deaths worldwide every year (15). Over the last few years, M. tuberculosis pathogenesis characterization at a molecular level required the development of efficient genetic tools for recombination and mutagenesis. The employment of replicating temperature-sensitive and suicide plasmids (14), specialized transducing mycobacteriophages (1, 9), and a recombineering system based on two exogenous recombinases (24) improved the ability to obtain mycobacterial mutants by homologous recombination. However, the availability of only few selection markers represents a real problem when multiple knockouts are required for the study of redundant gene families in mycobacteria. A way to circumvent this problem is by the production of unmarked mutations, which can be obtained by homologous recombination and selection for sequential crossing-over events using both positive and negative markers for counterselection of the different allelic exchange events (13), or by a different approach relying on sequence-specific recombination systems allowing the excision of the positive selection marker after it has been used to select for the recombination event (19).Three different sequence-specific recombinase systems have been successfully used with mycobacteria: the TnpR/res system of the γδ transposon (1), the Flp/FRT system of Saccharomyces cerevisiae (18, 20), and the LoxP/cre systems from bacteriophage P1 (11, 19). While the Flp/FRT and the Lox/cre systems were shown to work efficiently in both slow- and fast-growing mycobacteria, the Tnp/res system was proved to be efficient only in fast-growing species. All of these systems require a first step during which the expression of an exogenous resolvase or recombinase from a replicative plasmid allows the excision of the resistant marker and a second step to eliminate the replicative plasmid, making the procedure very time-consuming, particularly when working with slow-growing mycobacteria.Recently, a new sequence-specific recombinase system based on the endogenous Xer recombinases (Xer-cise) was shown to be amenable for genetic manipulation and construction of unmarked deletion mutants in Escherichia coli and Bacillus subtilis (4). In this system, the antibiotic resistance cassette, flanked by dif sites, is intrinsically unstable since the endogenous recombinases XerC and XerD recognize and resolve the dif sites that border the cassette. This method, relying on endogenous recombinases, does not require the introduction and the subsequent removal of replicating plasmids carrying exogenous genes, making it extremely simple and practical.E. coli XerC and XerD recombinases are essential for chromosome segregation during cell division, as their role is to resolve chromosome dimers to monomers recognizing the 28-bp dif sequence present at the replication terminus region (8). The Xer site-specific recombination system is very well conserved in prokaryotes with circular chromosomes, and homologues of XerC and XerD have been identified among Gram-negative and Gram-positive bacteria (16).In this report, we adapted the Xer-cise technique to mycobacteria, demonstrating that it can be employed as a practical and efficient genetic tool for manipulating both M. tuberculosis and Mycobacterium smegmatis.