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Implementation of a CRISPR-Based System for Gene Regulation in Candida albicans.

dc.contributor.authorRomán González, Elvira
dc.contributor.authorComan, Ioana V.
dc.contributor.authorPrieto Prieto, Antonio Daniel
dc.contributor.authorAlonso Monge, Rebeca María Del Mar
dc.contributor.authorPla Alonso, Jesús
dc.date.accessioned2023-06-17T13:23:59Z
dc.date.available2023-06-17T13:23:59Z
dc.date.issued2019-02-13
dc.description.abstractClustered regularly interspaced short palindromic repeat (CRISPR) methodology is not only an efficient tool in gene editing but also an attractive platform to facilitate DNA, RNA, and protein interactions. We describe here the implementation of a CRISPR-based system to regulate expression in the clinically important yeast By fusing an allele of Cas9 devoid of nuclease activity to a transcriptional repressor (Nrg1) or activator (Gal4), we were able to show specific repression or activation of the tester gene , encoding the cytosolic catalase. We generated strains where a 1.6-kbp upstream regulatory region of controls the expression of the green fluorescent protein (GFP) and demonstrated the functionality of the constructs by quantitative PCR (qPCR), flow cytometry, and analysis of sensitivity/resistance to hydrogen peroxide. Activation and repression were strongly dependent on the position of the complex in this regulatory region. We also improved transcriptional activation using an RNA scaffolding strategy to allow interaction of inactive variants of Cas9 (dCas9) with the RNA binding protein MCP (monocyte chemoattractant protein) fused to the VP64 activator. The strategy shown here may facilitate the analysis of complex regulatory traits in this fungal pathogen. CRISPR technology is a new and efficient way to edit genomes, but it is also an appealing way to regulate gene expression. We have implemented CRISPR as a gene expression platform in using fusions between a Cas9 inactive enzyme and specific repressors or activators and demonstrated its functionality. This will allow future manipulation of complex virulence pathways in this important fungal pathogen.en
dc.description.departmentDepto. de Microbiología y Parasitología
dc.description.facultyFac. de Farmacia
dc.description.refereedTRUE
dc.description.sponsorshipMinisterio de Economía, Comercio y Empresa (España)
dc.description.sponsorshipComunidad de Madrid
dc.description.statuspub
dc.eprint.idhttps://eprints.ucm.es/id/eprint/55654
dc.identifier.doi10.1128/mSphere.00001-19
dc.identifier.issn2379-5042
dc.identifier.officialurlhttps//doi.org/10.1128/mSphere.00001-19
dc.identifier.relatedurlhttps://www.asm.org/
dc.identifier.urihttps://hdl.handle.net/20.500.14352/13368
dc.issue.number1
dc.journal.titlemSphere
dc.language.isoeng
dc.publisherAmerican Society for Microbiology
dc.relation.projectIDBIO2015-05777
dc.relation.projectIDINGEMICS (S2017/BMD-36919
dc.rightsAtribución 3.0 España
dc.rights.accessRightsopen access
dc.rights.urihttps://creativecommons.org/licenses/by/3.0/es/
dc.subject.cdu579
dc.subject.cdu576
dc.subject.keywordCRISPR
dc.subject.keywordCandida albicans
dc.subject.keywordGal4
dc.subject.keywordRNA scaffold
dc.subject.keywordCatalase
dc.subject.keywordGene activation
dc.subject.keywordGene repression
dc.subject.keywordGenetic tool
dc.subject.ucmBiología celular (Farmacia)
dc.subject.ucmMicrobiología (Farmacia)
dc.subject.unesco3302.03 Microbiología Industrial
dc.titleImplementation of a CRISPR-Based System for Gene Regulation in Candida albicans.en
dc.typejournal article
dc.volume.number4
dspace.entity.typePublication
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