Beatriz Salas’s research while affiliated with University of Santiago Chile and other places

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Publications (1)

Scheme of template plasmids pCyaA’-Kan and pCyaA’-Cam for generation of unmarked chromosomal cyaA’ translational fusion to T3SS effectors in Salmonella. C1 and C2 are the priming sites for amplification of a DNA fragment including the cyaA’ ORF and the adjacent antibiotic resistance gene flanked by FRT sites.
Schematic representation of the procedure to generate unmarked cyaA’ translational fusions in the chromosome of Salmonella. C1 and C2 are the priming sites for amplification of a fragment of template plasmids pCyaA′-Kan and pCyaA′-Cam. H1 and H2 are specific homology regions required for insertion of the amplified fragment into a defined site in the chromosome.
Immunodetection of CyaA’ fusion proteins expressed by S. Typhimurium mutant strains grown under SPI-1- and SPI-2-inducing conditions. Bacterial strains expressing individual CyaA’ fusion proteins were grown in vitro under conditions that induce the expression of SPI-1 genes (i.e., LB medium containing 300 mM NaCl) or SPI-2 genes (i.e., N-minimal medium adjusted to pH 5.8). Bacterial lysates prepared from each culture were subjected to SDS-PAGE in 12% polyacrylamide gels. Proteins from gels were transferred to PVDF membranes, and CyaA’ fusion proteins were detected by Western blot using a commercial mouse anti-CyaA’ monoclonal antibody and anti-mouse IgG conjugated with horseradish peroxidase as secondary antibody.
T3SS-1-dependent secretion of fusion protein SipA-CyaA’. Bacterial strains expressing SipA-CyaA’ were grown in vitro under conditions that induce the expression of SPI-1 genes (i.e., LB medium containing 300 mM NaCl) or SPI-2 genes (i.e., N-minimal medium adjusted to pH 5.8). Proteins from culture supernatants and bacterial lysates were subjected to SDS-PAGE in 12% polyacrylamide gels and transferred to PVDF membranes. SipA-CyaA’ fusion protein and DnaK were detected by Western blot using a commercial mouse anti-CyaA’ monoclonal antibody or a commercial mouse anti-DnaK monoclonal antibody. In both cases, an anti-mouse IgG conjugated with horseradish peroxidase was used as secondary antibody.
Translocation of fusion protein SipA-CyaA’ into eukaryotic cells during infection. Monolayers of HeLa cells were infected with an unmarked S. Typhimurium mutant strain expressing SipA-CyaA’ using a multiplicity of infection (MOI) of 100 bacteria/cell. At different times, infected cells were lysed and the level of cAMP in the lysates was determined using a commercial ELISA kit. Graph shows mean values ± SEM from an independent assay performed in duplicate.
Novel Template Plasmids pCyaA’-Kan and pCyaA’-Cam for Generation of Unmarked Chromosomal cyaA’ Translational Fusion to T3SS Effectors in Salmonella
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February 2021

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85 Reads

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3 Citations

Paulina A. Fernández

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Marcela Zabner

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Jaime Ortega

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The type III secretion systems (T3SS) encoded in pathogenicity islands SPI-1 and SPI-2 are key virulence factors of Salmonella. These systems translocate proteins known as effectors into eukaryotic cells during infection. To characterize the functionality of T3SS effectors, gene fusions to the CyaA’ reporter of Bordetella pertussis are often used. CyaA’ is a calmodulin-dependent adenylate cyclase that is only active within eukaryotic cells. Thus, the translocation of an effector fused to CyaA’ can be evaluated by measuring cAMP levels in infected cells. Here, we report the construction of plasmids pCyaA’-Kan and pCyaA’-Cam, which contain the ORF encoding CyaA’ adjacent to a cassette that confers resistance to kanamycin or chloramphenicol, respectively, flanked by Flp recombinase target (FRT) sites. A PCR product from pCyaA’-Kan or pCyaA’-Cam containing these genetic elements can be introduced into the bacterial chromosome to generate gene fusions by homologous recombination using the Red recombination system from bacteriophage λ. Subsequently, the resistance cassette can be removed by recombination between the FRT sites using the Flp recombinase. As a proof of concept, the plasmids pCyaA’-Kan and pCyaA’-Cam were used to generate unmarked chromosomal fusions of 10 T3SS effectors to CyaA’ in S. Typhimurium. Each fusion protein was detected by Western blot using an anti-CyaA’ monoclonal antibody when the corresponding mutant strain was grown under conditions that induce the expression of the native gene. In addition, T3SS-1-dependent secretion of fusion protein SipA-CyaA’ during in vitro growth was verified by Western blot analysis of culture supernatants. Finally, efficient translocation of SipA-CyaA’ into HeLa cells was evidenced by increased intracellular cAMP levels at different times of infection. Therefore, the plasmids pCyaA’-Kan and pCyaA’-Cam can be used to generate unmarked chromosomal cyaA’ translational fusion to study regulated expression, secretion and translocation of Salmonella T3SS effectors into eukaryotic cells.

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Citations (1)

... Fernández et al. [19] report the construction of plasmids that are useful to generate chromosomal CyaA' translational fusions by homologous recombination using the Red recombination system. These fusions can be used to measure the level of expression of a gene and the secretion of a fusion to the culture supernatant by Western blot using anti-CyaA' antibodies. ...

Reference:

Special Issue: Type III Secretion Systems in Human/Animal Pathogenic Bacteria
Novel Template Plasmids pCyaA’-Kan and pCyaA’-Cam for Generation of Unmarked Chromosomal cyaA’ Translational Fusion to T3SS Effectors in Salmonella
Paulina A. Fernández

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Marcela Zabner

·

Jaime Ortega

·

[...]

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