2021
DOI: 10.1080/21505594.2021.1893008
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Enhancing the chemical transformation of Candida parapsilosis

Abstract: Candida parapsilosis is a leading cause of invasive mycoses and the major cause of nosocomial fungaemia amongst low and very low birth weight neonates. However, the molecular and physiological characteristics of this fungus remain understudied. To advance our knowledge about the pathobiology of this pathogen, we sought to develop and validate an effective method for chemical transformation of C. parapsilosis . Chemical transformation is the primary procedure for introducing fo… Show more

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Cited by 8 publications
(7 citation statements)
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“…The previously investigated yeast species S. cerevisiae , C. gattii C. albicans and C. dubliniensis each encode only two Zip-type cellular zinc importers. In S. cerevisiae , C. gattii and C. dubliniensis , the Zap1 transcription factor is responsible for the regulation of Zip importers in response to environmental zinc levels [2527]. Candida albicans Zap1 also regulates the zinc regulon in this species [35].…”
Section: Discussionmentioning
confidence: 99%
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“…The previously investigated yeast species S. cerevisiae , C. gattii C. albicans and C. dubliniensis each encode only two Zip-type cellular zinc importers. In S. cerevisiae , C. gattii and C. dubliniensis , the Zap1 transcription factor is responsible for the regulation of Zip importers in response to environmental zinc levels [2527]. Candida albicans Zap1 also regulates the zinc regulon in this species [35].…”
Section: Discussionmentioning
confidence: 99%
“…For reintegration, CpZRT21 and CpZRC1 were introduced into the CpNEUT5 L neutral locus using the Gateway cloning method as adapted to C. parapsilosis by Németh et al [26]. For functional restoration, CpZRC1 with a CaTDH3 promoter was introduced into the mutant strain Δ/Δ CpZRC1 by transformation as described by Németh et al [27].…”
Section: Methodsmentioning
confidence: 99%
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“…Yeast cells were transformed with 5 μg of the relevant plasmid and either 25 μL of unpurified repair template for editing the gene (eRT) or 5 μg of purified repair template for deleting the gene (delRT), using the lithium acetate method described in (47), with minor modifications (starting OD600nm of YPD culture 0.1 instead of 0.05). Transformants were selected onto YPD agar plates containing 200 μg/mL nourseothricin (Jena Bioscience GmbH, Germany) and screened by colony PCR to confirm the presence of the mutation (Table S2).…”
Section: Methodsmentioning
confidence: 99%
“…Yeast cells were transformed with 5 μg of the relevant plasmid and either 25 μL of unpurified repair template for editing the gene (eRT) or 5 μg of purified repair template for deleting the gene (delRT), using the lithium acetate method described in (47), with minor modifications (starting OD 600nm of YPD culture 0.1 instead of 0.05).…”
Section: Transformation Of Candida Parapsilosismentioning
confidence: 99%