Genomic analysis of Salmonella isolated from surface water and animal sources in Chile reveals new T6SS effector protein candidates

dc.contributor.authorAmaya, Fernando A.
dc.contributor.authorBlondel, Carlos J.
dc.contributor.authorReyes Méndez, Felipe.
dc.contributor.authorRivera, Dácil
dc.contributor.authorMoreno Switt, Andrea I.
dc.contributor.authorToro, Magaly
dc.contributor.authorBadilla, Consuelo
dc.contributor.authorSantiviago, Carlos A.
dc.contributor.authorPezoa Aros, David Antonio.
dc.contributor.otherFacultad de Medicina Veterinaria y Agronomíaes
dc.date.accessioned2025-04-22T18:44:37Z
dc.date.available2025-04-22T18:44:37Z
dc.date.issued2024
dc.description.abstractType VI Secretion Systems (T6SS), widely distributed in Gram-negative bacteria, contribute to interbacterial competition and pathogenesis through the translocation of effector proteins to target cells. Salmonella harbor 5 pathogenicity islands encoding T6SS (SPI-6, SPI-19, SPI-20, SPI-21 and SPI-22), in which a limited number of effector proteins have been identified. Previous analyses by our group focused on the identification of candidate T6SS effectors and cognate immunity proteins in Salmonella genomes deposited in public databases. In this study, the analysis was centered on Salmonella isolates obtained from environmental sources in Chile. To this end, bioinformatics and comparative genomics analyses were performed using 695 genomes of Salmonella isolates representing 44 serotypes obtained from surface water and animal sources in Chile to identify new T6SS effector proteins. First, T6SS gene clusters were identified using the SecreT6 server. This analysis revealed that most isolates carry the SPI-6 T6SS gene cluster, whereas the SPI-19 and SPI-21 T6SS gene clusters were detected in isolates from a limited number of serotypes. In contrast, the SPI-20 and SPI-22 T6SS gene clusters were not detected. Subsequently, each ORF in the T6SS gene clusters identified was analyzed using bioinformatics tools for effector prediction, identification of immunity proteins and functional biochemical prediction. This analysis detected 20 of the 37 T6SS effector proteins previously reported in Salmonella. In addition, 4 new effector proteins with potential antibacterial activity were identified in SPI-6: 2 Rhs effectors with potential DNase activity (PAAR-RhsA-NucA_B and PAAR-RhsA-GH-E) and 2 effectors with potential RNase activity (PAAR-RhsA-CdiA and RhsA-CdiA). Interestingly, the repertoire of SPI-6 T6SS effectors varies among isolates of the same serotype. In SPI-19, no new effector protein was detected. Of note, some Rhs effectors of SPI-19 and SPI-6 present C-terminal ends with unknown function. The presence of cognate immunity proteins carrying domains present in bona fide immunity proteins suggests that these effectors have antibacterial activity. Finally, two new effectors were identified in SPI-21: one with potential peptidoglycan hydrolase activity and another with potential membrane pore-forming activity. Altogether, our work broadens the repertoire of Salmonella T6SS effector proteins and provides evidence that SPI-6, SPI-19 and SPI-21 T6SS gene clusters harbor a vast array of antibacterial effectors.es
dc.facultadFacultad de Medicina Veterinaria y Agronomía
dc.format.extent17 páginas
dc.format.extent6.610Mb
dc.format.mimetypePDF
dc.identifier.citationFrontiers in Microbiology, 15, 17 p.es
dc.identifier.doi10.3389/fmicb.2024.1496223
dc.identifier.issn1664-302X
dc.identifier.urihttp://repositorio.udla.cl/xmlui/handle/udla/1766
dc.identifier.urihttps://www.frontiersin.org/journals/microbiology
dc.language.isoen_USes
dc.publisherFrontiers Mediaes
dc.rightsCreative Commons Attribution License (CC BY)
dc.sourceFrontiers in Microbiology
dc.subjectEffectores
dc.subjectImmunity proteines
dc.subjectT6SSes
dc.subject.lcshChile
dc.subject.lcshSalmonella
dc.titleGenomic analysis of Salmonella isolated from surface water and animal sources in Chile reveals new T6SS effector protein candidateses
dc.typeArtículoes
dc.udla.indexWoS
dc.udla.indexScopus
dc.udla.privacidadDocumento públicoes

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