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dc.contributor.authorSong, S.
dc.contributor.authorSemenova, E.
dc.contributor.authorSeverinov, K.
dc.contributor.authorFernández García, Laura
dc.contributor.authorBenedik, M.J.
dc.contributor.authorMaeda, T.
dc.contributor.authorWood, T.K.
dc.date.accessioned2025-08-26T11:09:10Z
dc.date.available2025-08-26T11:09:10Z
dc.date.issued2022
dc.identifier.citationSong S, Semenova E, Severinov K, Fernández-García L, Benedik MJ, Maeda T, et al. CRISPR-Cas Controls Cryptic Prophages. International Journal of Molecular Sciences. 2022;23(24).
dc.identifier.issn1422-0067
dc.identifier.otherhttps://portalcientifico.sergas.gal/documentos/65620a82f2e9e72161e172be*
dc.identifier.urihttp://hdl.handle.net/20.500.11940/20864
dc.description.abstractThe bacterial archetypal adaptive immune system, CRISPR-Cas, is thought to be repressed in the best-studied bacterium, Escherichia coli K-12. We show here that the E. coli CRISPR-Cas system is active and serves to inhibit its nine defective (i.e., cryptic) prophages. Specifically, compared to the wild-type strain, reducing the amounts of specific interfering RNAs (crRNA) decreases growth by 40%, increases cell death by 700%, and prevents persister cell resuscitation. Similar results were obtained by inactivating CRISPR-Cas by deleting the entire 13 spacer region (CRISPR array); hence, CRISPR-Cas serves to inhibit the remaining deleterious effects of these cryptic prophages, most likely through CRISPR array-derived crRNA binding to cryptic prophage mRNA rather than through cleavage of cryptic prophage DNA, i.e., self-targeting. Consistently, four of the 13 E. coli spacers contain complementary regions to the mRNA sequences of seven cryptic prophages, and inactivation of CRISPR-Cas increases the level of mRNA for lysis protein YdfD of cryptic prophage Qin and lysis protein RzoD of cryptic prophage DLP-12. In addition, lysis is clearly seen via transmission electron microscopy when the whole CRISPR-Cas array is deleted, and eliminating spacer #12, which encodes crRNA with complementary regions for DLP-12 (including rzoD), Rac, Qin (including ydfD), and CP4-57 cryptic prophages, also results in growth inhibition and cell lysis. Therefore, we report the novel results that (i) CRISPR-Cas is active in E. coli and (ii) CRISPR-Cas is used to tame cryptic prophages, likely through RNAi, i.e., unlike with active lysogens, active CRISPR-Cas and cryptic prophages may stably co-exist.en
dc.description.sponsorshipThis work was supported by funds derived from the Biotechnology Endowed Professorship at the Pennsylvania State University for T.W., from the National University Development Project at Jeonbuk National University in 2021 for S.S., and from the NIH RO1 GM10407 grant to K.S. We appreciate the feedback of Joy Muthami.en
dc.language.isoeng
dc.rightsAtribución 4.0 Internacional*
dc.rights.urihttp://creativecommons.org/licenses/by/4.0/
dc.titleCRISPR-Cas Controls Cryptic Prophages*
dc.typeArticleen
dc.authorsophosSong, T. K. S.
dc.authorsophosSemenova, E.
dc.authorsophosSeverinov, K.
dc.authorsophosFernández-García, L.
dc.authorsophosBenedik, M. J.
dc.authorsophosMaeda, T.
dc.authorsophosWood
dc.identifier.doi10.3390/ijms232416195
dc.identifier.sophos65620a82f2e9e72161e172be
dc.issue.number24
dc.journal.titleInternational Journal of Molecular Sciences*
dc.relation.projectIDBiotechnology Endowed Professorship at the Pennsylvania State University; National University Development Project at Jeonbuk National University; NIH [RO1 GM10407]
dc.relation.publisherversionhttps://www.mdpi.com/1422-0067/23/24/16195/pdf?version=1671443541;https://mdpi-res.com/d_attachment/ijms/ijms-23-16195/article_deploy/ijms-23-16195.pdf?version=1671443541es
dc.rights.accessRightsopenAccess
dc.subject.keywordAS Coruñaes
dc.subject.keywordCHUACes
dc.subject.keywordINIBICes
dc.typefidesArtículo Científico (incluye Original, Original breve, Revisión Sistemática y Meta-análisis)es
dc.typesophosArtículo Originales
dc.volume.number23


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