Site-specific bacterial chromosome engineering mediated by IntA integrase from Rhizobium etli

Rogelio Hernández-Tamayo; Gonzalo Torres-Tejerizo; Susana Brom; David Romero

doi:10.1186/s12866-016-0755-y

Site-specific bacterial chromosome engineering mediated by IntA integrase from Rhizobium etli

BMC Microbiol. 2016 Jun 29;16(1):133. doi: 10.1186/s12866-016-0755-y.

Authors

Rogelio Hernández-Tamayo¹, Gonzalo Torres-Tejerizo^{1

2}, Susana Brom¹, David Romero³

Affiliations

¹ Programa de Ingeniería Genómica, Centro de Ciencias Genómicas, Universidad Nacional Autónoma de México, Apartado Postal 565-A, 62210, Cuernavaca, Morelos, Mexico.
² Departamento de Ciencias Biológicas, Instituto de Biotecnología y Biología Molecular, UNLP, CCT-La Plata-CONICET, Facultad de Ciencias Exactas, Universidad Nacional de La Plata, La Plata, Argentina.
³ Programa de Ingeniería Genómica, Centro de Ciencias Genómicas, Universidad Nacional Autónoma de México, Apartado Postal 565-A, 62210, Cuernavaca, Morelos, Mexico. dromero@ccg.unam.mx.

Abstract

Background: The bacterial chromosome may be used to stably maintain foreign DNA in the mega-base range. Integration into the chromosome circumvents issues such as plasmid replication, stability, incompatibility, and copy number variance. The site-specific integrase IntA from Rhizobium etli CFN42 catalyzes a direct recombination between two specific DNA sites: attA and attD (23 bp). This recombination is stable. The aim of this work was to develop a R. etli derivative that may be used as recipient for the integration of foreign DNA in the chromosome, adapting the IntA catalyzed site-specific recombination system.

Results: To fulfill our aim, we designed a Rhizobium etli CFN42 derivative, containing a "landing pad" (LP) integrated into the chromosome. The LP sector consists of a green fluorescent protein gene under the control of the lacZ promoter and a spectinomycin resistance gene. Between the lacZ promoter and the GFP gene we inserted an IntA attachment site, which does not affect transcription from the lac promoter. Also, a mobilizable donor vector was generated, containing an attA site and a kanamycin resistance gene; to facilitate insertion of foreign DNA, this vector also contains a multicloning site. There are no promoters flanking the multicloning site. A biparental mating protocol was used to transfer the donor vector into the landing pad strain; insertion of the donor vector into the landing pad sector via IntA-mediated attA X attA recombination thereby interrupted the expression of the green fluorescent protein, generating site-specific cointegrants. Cointegrants were easily recognized by screening for antibiotic sensitivity and lack of GFP expression, and were obtained with an efficiency of 6.18 %.

Conclusions: Integration of foreign DNA in Rhizobium, lacking any similarity with the genome, can be easily achieved by IntA-mediated recombination. This protocol contains the mating and selection procedures for creating and isolating integrants.

Keywords: Chromosomal integration; Site-specific recombination; Tyrosine recombinase.

MeSH terms

Chromosomes, Bacterial*
Conjugation, Genetic
DNA
DNA Nucleotidyltransferases / genetics
DNA Nucleotidyltransferases / metabolism
DNA Replication
Escherichia coli / genetics
Flow Cytometry
Genetic Engineering / methods*
Genetic Vectors
Green Fluorescent Proteins / genetics
Integrases / genetics*
Lac Operon
Plasmids / genetics
Promoter Regions, Genetic
Recombination, Genetic
Rhizobium etli / enzymology*
Rhizobium etli / genetics*

Substances

Green Fluorescent Proteins
DNA
DNA Nucleotidyltransferases
Integrases
Site-specific recombinase