Copper-specific Transcriptional Repression of Yeast Genes Encoding Critical Components in the Copper Transport Pathway

Labbé, Simon; Zhu, Zhiwei; Thiele, Dennis J.

doi:10.1074/jbc.272.25.15951

Cited by 233 publications

(299 citation statements)

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“…The high-affinity Cu(I) transport genes CTR1, CTR3, and FRE1 are transcriptionally downregulated by Cu ions and induced by Cu ion starvation. This Cu ion-dependent regulation requires a wild-type Mac1p Cu metalloregulatory transcription factor (CuMRTF) (15,24,29,48). Regulation of these genes by Mac1p is highly specific for and exquisitely sensitive to Cu ions (29).…”

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confidence: 99%

“…This Cu ion-dependent regulation requires a wild-type Mac1p Cu metalloregulatory transcription factor (CuMRTF) (15,24,29,48). Regulation of these genes by Mac1p is highly specific for and exquisitely sensitive to Cu ions (29). Deletion of the MAC1 gene results in Cu ion starvation phenotypes similar to those associated with deletions in the CTR1 and CTR3 genes, which can be corrected by added Cu ions.…”

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confidence: 99%

“…In mac1⌬ strains, transcription of CTR1 and CTR3 is undetectable and the FRE1 gene is transcribed at low levels. In addition, yeast strains which possess a dominant MAC1 up1 allele exhibit high basal levels of CTR1, CTR3, and FRE1 mRNAs, a lack of Cu-dependent repression of CTR1 and CTR3 (29), and hypersensitivity to Cu ions (24). The mutations in Mac1p that lead to a dominant MAC1 up1 allele all map to the first of two cysteine clusters found in the carboxyl-terminal half of Mac1p (16,24,48,56).…”

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Dynamic Regulation of Copper Uptake and Detoxification Genes in Saccharomyces cerevisiae

Peña

Koch

Thiele

1998

Molecular and Cellular Biology

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The essential yet toxic nature of copper demands tight regulation of the copper homeostatic machinery to ensure that sufficient copper is present in the cell to drive essential biochemical processes yet prevent the accumulation to toxic levels. In Saccharomyces cerevisiae, the nutritional copper sensor Mac1p regulates the copper-dependent expression of the high affinity Cu(I) uptake genes CTR1, CTR3, and FRE1, while the toxic copper sensor Ace1p regulates the transcriptional activation of the detoxification genes CUP1, CRS5, and SOD1 in response to copper. In this study, we characterized the tandem regulation of the copper uptake and detoxification pathways in response to the chronic presence of elevated concentrations of copper ions in the growth medium. Upon addition of CuSO 4 , mRNA levels of CTR3 were rapidly reduced to eightfold the original basal level whereas the Ace1p-mediated transcriptional activation of CUP1 was rapid and potent but transient.

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Dynamic Regulation of Copper Uptake and Detoxification Genes in Saccharomyces cerevisiae

Peña

Koch

Thiele

1998

Molecular and Cellular Biology

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172

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“…Eukaryotic Cu(I)-responsive transcription factors include AceI and MacI of the organism Saccharomyces cerevisiae. Ace1 activates the transcription of copper sequestration and detoxification genes under conditions of copper excess [3][4][5], while Mac1 activates the Ctr1 and Ctr3 high-affinity copper uptake transporters under conditions of copper depletion [6,7]. In a similar vein, copper(I) has been shown to regulate the CopY repressors in bacteria.…”

Section: Introductionmentioning

confidence: 94%

“…1. CXCX (4)(5)(6) CXC motif in CopY homologs. Phylogenetic tree of amino acid sequences similar to E. hirae CopY, obtained by BLASTing (cutoff evalue of 0.00001) CopY to 496 complete bacterial genome sequences.…”

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Stalking metal-linked dimers

Pazehoski¹,

Collins²,

Boyle³

et al. 2008

Journal of Inorganic Biochemistry

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Regulated expression of theSaccharomyces cerevisiae Fre1p/Fre2p Fe/Cu reductase related genes

Georgatsou

Alexandraki

1999

Yeast

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A new fluorescent silsequioxane precursor with tuned optical properties and controlled aggregation properties is designed. The two cyclohexyl moieties introduced in the molecular structure allow the formation of very good quality films. The J‐aggregated structure is transcribed into the solid by photoacid‐catalyzed hydrolysis–polycondensation. Aggregation of the chromophores is reduced and highly fluorescent materials are obtained. The photoacid generator lies on the surface of the homogeneous layer of the sol–gel precursor. This phase separation presents several advantages, including UV protection of the chromophore and easy removal of the PAG. The first example of chemical amplification in the photolithography of the conjugated silsesquioxane precursor is demonstrated. As hydrolysis–polycondensation could be achieved in a controlled way by UV exposure, chemically amplified photolithography is achieved by irradiating a composite film (∼110 nm thick) on silicon wafer by using a copper TEM grid as shadow mask. The pattern is produced uniformly on a miscroscopic scale of 3 mm, the photopatterned pixels remaining highly fluorescent. The sizes of the photolithographed pixels correspond to the sizes of the rectangular holes of the 300 × 75 mesh grid (hole: 63 <$>μ<$>m × 204 <$>μ<$>m).

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Copper-specific Transcriptional Repression of Yeast Genes Encoding Critical Components in the Copper Transport Pathway

Cited by 233 publications

References 39 publications

Dynamic Regulation of Copper Uptake and Detoxification Genes in Saccharomyces cerevisiae

Dynamic Regulation of Copper Uptake and Detoxification Genes in Saccharomyces cerevisiae

Stalking metal-linked dimers

Regulated expression of theSaccharomyces cerevisiae Fre1p/Fre2p Fe/Cu reductase related genes

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