Quantitation of Ergosterol Content: Novel Method for Determination of Fluconazole Susceptibility of
            <i>Candida albicans</i>

Arthington-Skaggs, Beth A.; Jradi, Hoda; Desai, Tejal A.; Morrison, Christine J.

doi:10.1128/jcm.37.10.3332-3337.1999

Cited by 312 publications

(168 citation statements)

References 28 publications

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“…Ergosterol assays were carried out on 40 mL of yeast cultures grown in SC medium following treatment with atorvastatin and supplements. Ergosterol was extracted according to the method of Arthington-Skaggs et al (1999), involving digestion of the cell pellet in an alcoholic potassium hydroxide solution, followed by sterol extraction with n-heptane. The heptane layer was collected, diluted (up to fivefold) in 100% ethanol and scanned spectrophotometrically between 240 and 300 nm (Arthington-Skaggs et al, 1999) using a Shimadzu UV-1601 spectrophotometer.…”

Section: Quantitation Of Intracellular Ergosterol Contentmentioning

confidence: 99%

Atorvastatin-induced cell toxicity in yeast is linked to disruption of protein isoprenylation

Callegari

Andrews

Lopes

2010

FEMS Yeast Research

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Statins, used to treat hypercholesterolemia, are one of the most frequently prescribed drug classes in the developed world. However, a significant proportion of users suffer symptoms of myotoxicity, and currently, the molecular mechanisms underlying myotoxicity remain ambiguous. In this study, Saccharomyces cerevisiae was exploited as a model system to gain further insight into the molecular mechanisms of atorvastatin toxicity. Atorvastatin-treated yeast cells display marked morphological deformities, have reduced cell viability and are highly vulnerable to perturbed mitochondrial function. Supplementation assays of atorvastatin-treated cells reveal that both loss of viability and mitochondrial dysfunction occur as a consequence of perturbation of the sterol synthesis pathway. This was further investigated by supplementing statin-treated cells with various metabolites of the sterol synthesis pathway that are believed to be essential for cell function. Ergosterol, coenzyme Q and a heme precursor were all ineffective in the prevention of statin-induced mitochondrial disruption and cell death. However, the addition of geranylgeranyl pyrophosphate and farnesyl pyrophosphate significantly restored cell viability, although these did not overcome petite induction. This highlights the pleiotropic nature of statin toxicity, but has established protein prenylation disruption as one of the principal mechanisms underlying statin-induced cell death in yeast.

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Section: Quantitation Of Intracellular Ergosterol Contentmentioning

confidence: 99%

Atorvastatin-induced cell toxicity in yeast is linked to disruption of protein isoprenylation

Callegari

Andrews

Lopes

2010

FEMS Yeast Research

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“…Ergosterol levels were assayed using a modification of the sterol quantitation methods of Arthington-Skaggs et al (1999) and Breivik & Owades (1957). Yeast strains were grown to stationary phase in 50 mL of minimal medium in the presence or absence of simvastatin.…”

Section: Ergosterol Assaysmentioning

confidence: 99%

Simvastatin reduces ergosterol levels, inhibits growth and causes loss of mtDNA inCandida glabrata

Westermeyer

Macreadie

2007

FEMS Yeast Research

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Statins are widely used for lowering cholesterol levels through their action on 3-hydroxy-3-methylglutaryl-CoA (HMG-CoA) reductase. Yeasts use HMG-CoA reductase for the same enzymatic step as humans, but in yeasts the main end-product of the pathway is ergosterol rather than cholesterol. We considered that insights into the effects of statins in humans could be gained by examination of the effects of simvastatin on the petite-positive yeast Candida glabrata. Simvastatin was found to inhibit growth, and this was associated with lower ergosterol levels. As simvastatin-treated cultures of yeast were passaged, the frequencies of petite cells (respiratory-deficient yeast mutants with deletions in the mitochondrial genome) increased with time and with simvastatin concentration. DNA staining of the petite mutants showed that they were devoid of mtDNA, suggesting a defect in the maintenance of mtDNA. These observations in C. glabrata may provide further insights into the molecular effects of statins in humans undergoing treatment for hypercholesterolemia. In addition, if C. glabrata is a valid model for studying statin treatments, it would be very useful for the preliminary screening of agents to reduce statin side-effects.

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“…Ergosterol content was measured as described (Arthington-Skaggs et al, 1999;Yarden et al, 2014). Briefly, 1 ml of conidial suspensions (10 7 conidia/ml) were inoculated in 100 ml of SDB and incubated at room temperature for 3 days with aeration.…”

Section: Ergosterol Measurementsmentioning

confidence: 99%

The Thm1 Zn(II)₂Cys₆ transcription factor contributes to heat, membrane integrity and virulence in the insect pathogenic fungus Beauveria bassiana

Huang

Keyhani

Zhao

et al. 2019

Environmental Microbiology

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Summary The ability to withstand heat and cell wall stress is critical for successful infection of target hosts by many pathogenic fungi. We report on the characterization of BbThm1 (transcription factor for heat and membrane integrity), a Zn(II)2Cys6 (Gal4‐like) family member, which regulates resistance to heat (32°C) and specific detergents in the insect pathogenic fungus, Beauveria bassiana. BbThm1 gene knock‐out mutants showed severely impaired growth/resistance at 32°C and to SDS, but mild to moderate phenotypic responses to other stresses including oxidative, osmotic and cell‐wall targeting compounds, or to various fungicides. Shifts in cell wall properties, adhesion and decreased viability were noted for the ΔBbThm1 mutant. Susceptibility to SDS but not heat could be rescued by exogenous ergosterol. Insect bioassays revealed decreased virulence of the ΔBbThm1 mutant against Galleria mellonella both topically and via intrahemocoel injection assays that correlated with impaired in insecta hyphal body formation and altered host immune prophenol oxidase (PO) activation. Transcriptomic analyses of the wild‐type and ΔBbThm1 mutants revealed up‐regulation of hydrolases but down‐regulation of a wide range of basic metabolic processes. These data reveal fine tune aspects of the transcription factor network that regulates specific stress responses to contribute to the overall pathogenic process.

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Quantitation of Ergosterol Content: Novel Method for Determination of Fluconazole Susceptibility of Candida albicans

Cited by 312 publications

References 28 publications

Atorvastatin-induced cell toxicity in yeast is linked to disruption of protein isoprenylation

Atorvastatin-induced cell toxicity in yeast is linked to disruption of protein isoprenylation

Simvastatin reduces ergosterol levels, inhibits growth and causes loss of mtDNA inCandida glabrata

The Thm1 Zn(II)₂Cys₆ transcription factor contributes to heat, membrane integrity and virulence in the insect pathogenic fungus Beauveria bassiana

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Quantitation of Ergosterol Content: Novel Method for Determination of Fluconazole Susceptibility of Candida albicans

Cited by 312 publications

References 28 publications

Atorvastatin-induced cell toxicity in yeast is linked to disruption of protein isoprenylation

Atorvastatin-induced cell toxicity in yeast is linked to disruption of protein isoprenylation

Simvastatin reduces ergosterol levels, inhibits growth and causes loss of mtDNA inCandida glabrata

The Thm1 Zn(II)2Cys6 transcription factor contributes to heat, membrane integrity and virulence in the insect pathogenic fungus Beauveria bassiana

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The Thm1 Zn(II)₂Cys₆ transcription factor contributes to heat, membrane integrity and virulence in the insect pathogenic fungus Beauveria bassiana