Two genes differentially regulated in the cell cycle and by DNA-damaging agents encode alternative regulatory subunits of ribonucleotide reductase.

Elledge, Stephen J.; Davis, Ronald W.

doi:10.1101/gad.4.5.740

Cited by 284 publications

(255 citation statements)

References 41 publications

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“…This organism possesses no deoxynucleoside kinase activities, and thus, dNTP synthesis is entirely dependent on RNR (72). In S. cerevisiae, the levels of the subunits are controlled transcriptionally and the level of mRNA of the α subunit is increased during the S-phase of the cell cycle during normal growth, while the levels of mRNA for the β and β′ subunits remain largely unchanged (22,25,27,31). We have recently shown that the mRNA levels are correlated with the protein levels (D. L. Perlstein, M. Huang, and J. Stubbe, unpublished results).…”

Section: Discussionmentioning

confidence: 94%

Determination of the in Vivo Stoichiometry of Tyrosyl Radical per ββ‘ in Saccharomyces cerevisiae Ribonucleotide Reductase

et al. 2006

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The class I ribonucleotide reductases catalyze the conversion of nucleotides to deoxynucleotides and are composed of two subunits: R1 and R2. R1 contains the site for nucleotide reduction and the sites that control substrate specificity and the rate of reduction. R2 houses the essential diferric-tyrosyl radical (Y • ) cofactor. In Saccharomyces cerevisiae, two R1s, α n and , have been identified, while R2 is a heterodimer (ββ′). β′ cannot bind iron and generate the Y • ; consequently, the maximum amount of Y • per ββ′ is 1. To determine the cofactor stoichiometry in vivo, a FLAGtagged β ( FLAG β) was constructed and integrated into the genome of Y300 (MHY343). This strain facilitated the rapid isolation of endogenous levels of FLAG ββ′ by immunoaffinity chromatography, which was found to have 0.45 ± 0.08 Y • / FLAG ββ′ and a specific activity of 2.3 ± 0.5 μmol min −1 mg −1 . FLAG ββ′ isolated from MMS-treated MHY343 cells or cells containing a deletion of the transcriptional repressor gene CRT1 also gave a Y • / FLAG ββ′ ratio of 0.5. To determine the Y • /ββ′ ratio without R2 isolation, whole cell EPR and quantitative Western blots of β were performed using different strains and growth conditions. The wild-type (wt) strains gave a Y • /ββ′ ratio of 0.83-0.89. The same strains either treated with MMS or containing a crt1Δ gave ratios between 0.49 and 0.72. Nucleotide reduction assays and quantitative Western blots from the same strains provided an independent measure and confirmation of the Y • /ββ′ ratios. Thus, under normal growth conditions, the cell assembles stoichiometric amounts of Y • and modulation of Y • concentration is not involved in the regulation of RNR activity.

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Section: Discussionmentioning

confidence: 94%

Determination of the in Vivo Stoichiometry of Tyrosyl Radical per ββ‘ in Saccharomyces cerevisiae Ribonucleotide Reductase

et al. 2006

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“…6B). Because rad9 mutants show normal signaling for HU-induced RNR3 expression and are not themselves sensitive to HU (Elledge and Davis 1990), it was anticipated that rad9 mutants would have no effect on HUsensitivity of po12 mutants. Surprisingly, rad9 has a pronounced effect indicating that RAD9 may have a minor role in the response to HU arrest during S phase that is not detectable until the major pathway is knocked out.…”

Section: Transcriptional Response Of Other Checkpoint Mutants Shows Rmentioning

confidence: 99%

RAD9 and DNA polymerase epsilon form parallel sensory branches for transducing the DNA damage checkpoint signal in Saccharomyces cerevisiae.

Navas¹,

Sánchez²,

Elledge³

1996

Genes Dev.

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156

130

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In response to DNA damage and replication blocks, yeast cells arrest at distinct points in the cell cycle and induce the transcription of genes whose products facilitate DNA repair. Examination of the inducibility of RNR3 in response to UV damage has revealed that the various checkpoint genes can be arranged in a pathway consistent with their requirement to arrest cells at different stages of the cell cycle. While RADg, RAD24, and MEC3 are required to activate the DNA damage checkpoint when cells are in G1 or G2, POL2 is required to sense UV damage and replication blocks when cells are in S phase. The phosphorylation of the essential central transducer, Rad53p, is dependent on POL2 and RAD9 in response to UV damage, indicating that RAD53 functions downstream of both these genes. Mutants defective for both pathways are severely deficient in Rad53p phosphorylation and RNR3 induction and are significantly more sensitive to DNA damage and replication blocks than single mutants alone. These results show that POL2 and RAD9 function in parallel branches for sensing and transducing the UV DNA damage signal. Each of these pathways subsequently activates the central transducers Meclp/Esrlp/Sad3p and Rad53p/Mec2p/Sadlp, which are required for both cell-cycle arrest and transcriptional responses.

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“…Yeast ribonucleotide reductase, a multi-protein complex, catalyzes one step in the dNTP production pathway. It is activated both as a normal part of the cell cycle and also in response to DNA damage [21,22,23,24,25]. RNR1 mRNA levels vary considerably with the cell cycle; the peak level occurs in the G1 phase [26].…”

Section: Introductionmentioning

confidence: 99%

Dynamic SPR monitoring of yeast nuclear protein binding to a cis-regulatory element

Mao¹,

Brody²

2007

Biochemical and Biophysical Research Communications

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Gene expression is controlled by protein complexes binding to short specific sequences of DNA, called cis-regulatory elements. Expression of most eukaryotic genes is controlled by dozens of these elements. Comprehensive identification and monitoring of these elements is a major goal of genomics. In pursuit of this goal, we are developing a surface plasmon resonance (SPR) based assay to identify and monitor cis-regulatory elements. To test whether we could reliably monitor protein binding to a regulatory element, we immobilized a 16 bp region of S. Cerevisiae chromosome 5 onto a gold surface. This 16 bp region of DNA is known to bind several proteins and thought to control expression of the gene RNR1, which varies through the cell cycle. We synchronized yeast cell cultures, and then sampled these cultures at a regular interval. These samples were processed to purify nuclear lysate, which was then exposed to the sensor. We found that nuclear protein binds this particular element of DNA at a significantly higher rate (as compared to unsynchronized cells) during G1 phase. Other time points show levels of DNA-nuclear protein binding similar to the unsynchronized control. We also measured the apparent association complex of the binding to be 0.014 s −1 . We conclude that (1) SPR-based assays can monitor DNA-nuclear protein binding and that (2) for this particular cis-regulatory element, maximum DNA-nuclear protein binding occurs during G1 phase.

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Two genes differentially regulated in the cell cycle and by DNA-damaging agents encode alternative regulatory subunits of ribonucleotide reductase.

Cited by 284 publications

References 41 publications

Determination of the in Vivo Stoichiometry of Tyrosyl Radical per ββ‘ in Saccharomyces cerevisiae Ribonucleotide Reductase

Determination of the in Vivo Stoichiometry of Tyrosyl Radical per ββ‘ in Saccharomyces cerevisiae Ribonucleotide Reductase

RAD9 and DNA polymerase epsilon form parallel sensory branches for transducing the DNA damage checkpoint signal in Saccharomyces cerevisiae.

Dynamic SPR monitoring of yeast nuclear protein binding to a cis-regulatory element

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