Multicopy Integration of Heterologous Genes, Using the Lactococcal Group II Intron Targeted to Bacterial Insertion Sequences

Rawsthorne, Helen; Turner, Kevin N.; Mills, David A.

doi:10.1128/aem.02992-05

Cited by 28 publications

(35 citation statements)

References 39 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…Colony PCRs were carried out as previously described (42 (31) developed by the DOE Joint Genome Institute. 16S rRNA-based dendrograms were generated using tools available on the Ribosomal Database Project website (4).…”

Section: Methodsmentioning

confidence: 99%

Role of Hypermutability in the Evolution of the GenusOenococcus

et al. 2008

Self Cite

View full text Add to dashboard Cite

Oenococcus oeni is an alcohol-tolerant, acidophilic lactic acid bacterium primarily responsible for malolactic fermentation in wine. A recent comparative genomic analysis of O. oeni PSU-1 with other sequenced lactic acid bacteria indicates that PSU-1 lacks the mismatch repair (MMR) genes mutS and mutL. Consistent with the lack of MMR, mutation rates for O. oeni PSU-1 and a second oenococcal species, O. kitaharae, were higher than those observed for neighboring taxa, Pediococcus pentosaceus and Leuconostoc mesenteroides. Sequence analysis of the rpoB mutations in rifampin-resistant strains from both oenococcal species revealed a high percentage of transition mutations, a result indicative of the lack of MMR. An analysis of common alleles in the two sequenced O. oeni strains, PSU-1 and BAA-1163, also revealed a significantly higher level of transition substitutions than were observed in other Lactobacillales species. These results suggest that the genus Oenococcus is hypermutable due to the loss of mutS and mutL, which occurred with the divergence away from the neighboring Leuconostoc branch. The hypermutable status of the genus Oenococcus explains the observed high level of allelic polymorphism among known O. oeni isolates and likely contributed to the unique adaptation of this genus to acidic and alcoholic environments.Two species of lactic acid bacteria (LAB), Oenococcus oeni and the recently identified Oenococcus kitaharae, are described within the Oenococcus genus (12, 50). O. oeni, formerly Leuconostoc oenos (7), plays an important role in the elaboration of wine, where it is often added as a starter culture to carry out the malolactic conversion (28). Given the economic importance of this conversion, the taxonomic structure of this species has been studied in detail, the result of which indicates that the species is quite homogeneous (22,44,51,59). Recently, however, multilocus sequence typing (MLST) of 18 strains revealed a high level of allelic diversity in O. oeni, which has a panmictic population structure where lines of clonal descent are difficult to define (5). Panmictic populations are often characterized by high levels of horizontal transfer and recombination among strains, and this was posited as a cause of the genomic diversity and evolution of O. oeni (5). On the basis of 16S rRNA analysis, Yang and Woese (56) proposed an accelerated evolution of the Leuconostoc group in general and of O. oeni in particular. This work was confirmed by recent phylogenetic comparisons of concatenated ribosomal and RNA polymerase subunits (29).A recent comparative genomic analysis of O. oeni PSU-1 with other sequenced LAB indicated that O. oeni PSU-1 lacks the genes mutS and mutL (29, 30), which encode two key enzymes in the mismatch repair (MMR) pathway. The MMR pathway is an excision repair system that corrects many types of base pair mismatches (14,24,35,36,39). While there are some differences among MMR systems in different bacteria, the presence of mutS and mutL homologs is required. The MutS protein recognize...

show abstract

Section: Methodsmentioning

confidence: 99%

Role of Hypermutability in the Evolution of the GenusOenococcus

et al. 2008

Self Cite

View full text Add to dashboard Cite

show abstract

“…In bacteria, targetrons designed using the algorithm are commonly inserted into chromosomal target sites at frequencies of 1 to 100% of colonies without selection, and insertions can be detected either by colony PCR screening or by using a genetic marker inserted in the intron (30,47). Targetrons have been used in bacteria to obtain targeted gene disruptions, including conditional disruptions (11,21,30,45), insertion ("knocking in") of cargo genes at desired chromosomal locations (11,34), introduction of point mutations by making a targeted double-strand break that stimulates homologous recombination with a cotransformed DNA (21), and generation of whole-genome knockout libraries (46,47).…”

mentioning

confidence: 99%

Gene Targeting in Gram-Negative Bacteria by Use of a Mobile Group II Intron (“Targetron”) Expressed from a Broad-Host-Range Vector

Yao

Lambowitz

2007

Appl Environ Microbiol

View full text Add to dashboard Cite

Mobile group II introns ("targetrons") can be programmed for insertion into virtually any desired DNA target with high frequency and specificity. Here, we show that targetrons expressed via an m-toluic acidinducible promoter from a broad-host-range vector containing an RK2 minireplicon can be used for efficient gene targeting in a variety of gram-negative bacteria, including Escherichia coli, Pseudomonas aeruginosa, and Agrobacterium tumefaciens. Targetrons expressed from donor plasmids introduced by electroporation or conjugation yielded targeted disruptions at frequencies of 1 to 58% of screened colonies in the E. coli lacZ, P. aeruginosa pqsA and pqsH, and A. tumefaciens aopB and chvI genes. The development of this broad-host-range system for targetron expression should facilitate gene targeting in many bacteria.Mobile group II introns ("targetrons") have been used for targeted gene disruption and site-specific DNA insertion in diverse gram-negative and gram-positive bacteria, including Escherichia coli (21, 30), Shigella flexneri (21), Salmonella enterica serovar Typhimurium (21), Lactococcus lactis (11), Clostridium perfringens (3), and Staphylococcus aureus (45). Group II introns are useful for gene targeting because they can be programmed for insertion into virtually any desired DNA target with high frequency and specificity (22,30). This ability derives from their unique DNA integration mechanism, called retrohoming, in which the intron RNA is inserted via reverse splicing directly into a DNA target site and is then reverse transcribed by the intron-encoded protein (IEP) (reviewed in reference 23). Retrohoming is mediated by a ribonucleoprotein (RNP) particle that is formed during RNA splicing and contains the IEP and excised intron lariat RNA. RNPs initiate mobility by using both the IEP and base pairing of the intron RNA to recognize DNA target sequences, with the latter contributing most of the target specificity (10,16,17,41). Consequently, it is possible to retarget group II introns for insertion into preselected sites simply by modifying the base-pairing sequences in the intron RNA (16,22,28,30).DNA target site interactions for the L. lactis Ll.LtrB group II intron used in the present work are shown in Fig. 1A (16, 28, 30, 41). The DNA target site positions recognized by base pairing of the intron RNA span positions Ϫ12 to ϩ2 from the intron insertion site and are denoted intron-binding sites 1 and 2 (IBS1 and IBS2) in the 5Ј exon (E1) and ␦Ј in the 3Ј exon (E2). The complementary intron RNA sequences are located in two different RNA stem loops and are denoted exon-binding sites 1 and 2 (EBS1 and EBS2) and ␦ sequences (sequences adjacent to EBS1). The IEP (LtrA protein) recognizes additional positions in the distal 5Ј exon and 3Ј exon regions of the DNA target site, interactions that are important for local DNA melting and bottom-strand cleavage for generating the primer for reverse transcription of the inserted intron RNA (key positions recognized by the IEP are underlined in Fig. 1A) (22, 23). ...

show abstract

“…The recent advances toward the development of efficient gene expression systems in L. lactis and the established safety profile of L. lactis based on long-term use in dairy food processing has led to new potential applications in protein production, therapeutic drug delivery, and vaccine delivery (5,27,30,38).…”

mentioning

confidence: 99%

Production of a Particulate Hepatitis C Vaccine Candidate by an Engineered Lactococcus lactis Strain

Parlane

Grage

Lee

et al. 2011

Appl Environ Microbiol

View full text Add to dashboard Cite

Vaccine delivery systems based on display of antigens on bioengineered bacterial polyester inclusions can stimulate cellular immune responses. The food-grade Gram-positive bacterium Lactococcus lactis was engineered to produce spherical polyhydroxybutyrate (PHB) inclusions which abundantly displayed the hepatitis C virus core (HCc) antigen. In mice, the immune response induced by this antigen delivery system was compared to that induced by vaccination with HCc antigen displayed on PHB beads produced in Escherichia coli, to PHB beads without antigen produced in L. lactis or E. coli, or directly to the recombinant HCc protein.Vaccination site lesions were minimal in all mice vaccinated with HCc PHB beads or recombinant protein, all mixed in the oil-in-water adjuvant Emulsigen, while vaccination with the recombinant protein in complete Freund's adjuvant produced a marked inflammatory reaction at the vaccination site. Vaccination with the PHB beads produced in L. lactis and displaying HCc antigen produced antigen-specific cellular immune responses with significant release of gamma interferon (IFN-␥) and interleukin-17A (IL-17A) from splenocyte cultures and no significant antigen-specific serum antibody, while the PHB beads displaying HCc but produced in E. coli released IFN-␥ and IL-17A as well as the proinflammatory cytokines tumor necrosis factor alpha (TNF-␣) and IL-6 and low levels of IgG2c antibody. In contrast, recombinant HCc antigen in Emulsigen produced a diverse cytokine response and a strong IgG1 antibody response. Overall it was shown that L. lactis can be used to produce immunogenic PHB beads displaying viral antigens, making the beads suitable for vaccination against viral infections.The food-grade Gram-positive bacterium, Lactococcus lactis has been increasingly considered as a production host for recombinant therapeutic proteins (6, 9, 49). The recent advances toward the development of efficient gene expression systems in L. lactis and the established safety profile of L. lactis based on long-term use in dairy food processing has led to new potential applications in protein production, therapeutic drug delivery, and vaccine delivery (5,27,30,38).Recently, it was shown that L. lactis can be engineered to produce spherical polyhydroxybutyrate (PHB) inclusions which display the Staphylococcus aureus protein A-derived IgG binding region, the Z domain, and that these can be isolated for in vitro use in purification of IgG (26). This was achieved by establishing the PHB biosynthesis pathway in L. lactis and by overproducing a Z domain-PHB synthase fusion protein which remained attached to the PHB inclusion surface. The PHB synthase represents the only essential enzyme required for PHB inclusion formation (39,40). This strategy utilized protein engineering of the PHB synthase from Ralstonia eutropha for the display of various protein-based functions, such as technical enzymes, binding domains, or a fluorescent protein, at the surfaces of PHB beads as had been previously established in recombinant Escherichi...

show abstract

Multicopy Integration of Heterologous Genes, Using the Lactococcal Group II Intron Targeted to Bacterial Insertion Sequences

Cited by 28 publications

References 39 publications

Role of Hypermutability in the Evolution of the GenusOenococcus

Role of Hypermutability in the Evolution of the GenusOenococcus

Gene Targeting in Gram-Negative Bacteria by Use of a Mobile Group II Intron (“Targetron”) Expressed from a Broad-Host-Range Vector

Production of a Particulate Hepatitis C Vaccine Candidate by an Engineered Lactococcus lactis Strain

Contact Info

Product

Resources

About