Rodyti trumpą aprašą

dc.contributor.authorServienė, Elena
dc.contributor.authorLukša, Juliana
dc.contributor.authorOrentaitė, Irma
dc.contributor.authorLafontaine, Denis
dc.contributor.authorUrbonavičius, Jaunius
dc.date.accessioned2023-09-18T18:34:30Z
dc.date.available2023-09-18T18:34:30Z
dc.date.issued2012
dc.identifier.issn1932-6203
dc.identifier.other(BIS)VDU02-000012878
dc.identifier.urihttps://etalpykla.vilniustech.lt/handle/123456789/129396
dc.description.abstractBackground: Understanding how biotoxins kill cells is of prime importance in biomedicine and the food industry. The budding yeast (S. cerevisiae) killers serve as a convenient model to study the activity of biotoxins consistently supplying with significant insights into the basic mechanisms of virus-host cell interactions and toxin entry into eukaryotic target cells. K1 and K2 toxins are active at the cell wall, leading to the disruption of the plasma membrane and subsequent cell death by ion leakage. K28 toxin is active in the cell nucleus, blocking DNA synthesis and cell cycle progression, thereby triggering apoptosis. Genome-wide screens in the budding yeast S. cerevisiae identified several hundred effectors of K1 and K28 toxins. Surprisingly, no such screen had been performed for K2 toxin, the most frequent killer toxin among industrial budding yeasts. Principal Findings: We conducted several concurrent genome-wide screens in S. cerevisiae and identified 332 novel K2 toxin effectors. The effectors involved in K2 resistance and hypersensitivity largely map in distinct cellular pathways, including cell wall and plasma membrane structure/biogenesis and mitochondrial function for K2 resistance, and cell wall stress signaling and ion/pH homeostasis for K2 hypersensitivity. 70% of K2 effectors are different from those involved in K1 or K28 susceptibility. Significance: Our work demonstrates that despite the fact that K1 and K2 toxins share some aspects of their killing strategies, they largely rely on different sets of effectors. Since the vast majority of the host factors identified here is exclusively active towards K2, we conclude that cells have acquired a specific K2 toxin effectors set. Our work thus indicates that K1 and K2 have elaborated different biological pathways and provides a first step towards the detailed characterization of K2 mode of action.eng
dc.formatPDF
dc.format.extentp. 1-12
dc.format.mediumtekstas / txt
dc.language.isoeng
dc.relation.isreferencedbyScopus
dc.relation.isreferencedbyPubMed
dc.relation.isreferencedbyMEDLINE
dc.relation.isreferencedbyBIOSIS Previews
dc.relation.isreferencedbyZoological Record
dc.relation.isreferencedbyScience Citation Index Expanded (Web of Science)
dc.source.urihttp://www.plosone.org/article/info%3Adoi%2F10.1371%2Fjournal.pone.0050779
dc.titleScreening the budding yeast genome reveals unique factors affecting K2 toxin susceptibility
dc.typeStraipsnis Web of Science DB / Article in Web of Science DB
dcterms.references41
dc.type.pubtypeS1 - Straipsnis Web of Science DB / Web of Science DB article
dc.contributor.institutionVilniaus Gedimino technikos universitetas Gamtos tyrimų centras
dc.contributor.institutionGamtos tyrimų centras
dc.contributor.institutionVytauto Didžiojo universitetas Botanikos institutas Gamtos tyrimų centras
dc.contributor.institutionAcadémie Wallonie-Bruxelles, Belgium Université Libre de Bruxelles, Belgium
dc.contributor.institutionAcadémie Wallonie-Bruxelles, Belgium
dc.contributor.facultyFundamentinių mokslų fakultetas / Faculty of Fundamental Sciences
dc.subject.researchfieldN 010 - Biologija / Biology
dc.subject.researchfieldN 003 - Chemija / Chemistry
dc.subject.researchfieldN 004 - Biochemija / Biochemistry
dc.subject.enK2 toxin
dc.subject.enBiotoxins
dc.subject.enGenome
dcterms.sourcetitlePLoS ONE
dc.description.issueiss. 12
dc.description.volumevol. 7
dc.publisher.namePublic Library of Science
dc.publisher.citySan Francisco, USA
dc.identifier.doiLBT02-000046842
dc.identifier.doiVGT02-000025618
dc.identifier.doi10.1371/journal.pone.0050779
dc.identifier.elaba4691295


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