« Previous AbstractA Preliminary Research Study for Distribution Characteristics and Sources of Indoor Air Pollutants in the Valuable Archive of the National Library of Korea    Next AbstractRegulation of Dauer formation by O-GlcNAcylation in Caenorhabditis elegans »

J Biol Chem

Title:		Transcriptional remodeling and G1 arrest in dioxygen stress in Saccharomyces cerevisiae
Author(s):		Lee J; Romeo A; Kosman DJ;
Address:		"Department of Biochemistry, School of Medicine and Biomedical Sciences, State University of New York, Buffalo, New York 14214, USA"
Journal Title:		J Biol Chem
Year:		1996
Volume:		271
Issue:		40
Page Number:		24885 - 24893
DOI:		10.1074/jbc.271.40.24885
ISSN/ISBN:		0021-9258 (Print) 0021-9258 (Linking)
Abstract:		"Saccharomyces cerevisiae, which lack a functional SOD1 gene, encoding the cytosolic Cu,Zn-superoxide dismutase (SOD1), exhibit a variety of metabolic defects in aerobic but not in anaerobic growth. We test here the hypothesis that some of these defects may be due to specific transcriptional changes programmed for cell survival under dioxygen stress. Analysis of the budding pattern and generation time showed that the slower proliferation of an sod1Delta mutant strain under air was due to an increase from 42 to 89 min spent in the G1 phase of the cell cycle. This delay in G1 was not due to an overall decline in biosynthetic activity since total protein and mRNA synthesis was not reduced even under 100% O2. However, rRNA synthesis was strongly decreased, e.g. by 80% in the mutant under 100% O2 (in comparison to N2). Under these conditions, the mutant permanently arrested in G1; this arrest was due to an inhibition of the Start function that prepares yeast for S phase. This Start arrest was due to an inhibition of transcription of the autoregulated G1 cyclins, CLN1 and CLN2; the transcription of the constitutive G1 cyclin, CLN3, was unaffected by the stress. Expression of a hyperstable Cln3 prevented the G1 arrest, indicating that it was due solely to the inhibition of cell cycle-dependent cyclin expression. This remodeling of transcription in oxidative stress was seen also in the inhibition of glucose derepression of SUC2 expression. In contrast, the signaling and activation of mating pheromone (FUS1) and copper-responsive (CUP1) promoter activity were not affected by dioxygen stress, while genes encoding other anti-oxidant enzymes (SOD2, CTT1 and CTA1) were strongly induced. The UBI loci, encoding ubiquitin, were particularly good examples of this pattern of negative and positive transcriptional response to the stress. UBI1-UBI3 expression was repressed in the mutant under 100% O2, while expression of UBI4 was strongly induced. The data demonstrate that extensive remodeling of transcription occurs in yeast under a strong dioxygen stress. This remodeling results in a pattern of expression of gene products needed for defense and repair, and suppression of activities associated with normal proliferative growth"
Keywords:		"Cyclins/genetics Fungal Proteins/biosynthesis *G1 Phase Gene Expression Regulation, Fungal *Oxidative Stress *Oxygen RNA, Fungal/biosynthesis/metabolism Saccharomyces cerevisiae/cytology/genetics/*metabolism *Transcription, Genetic;"
Notes:		"MedlineLee, J Romeo, A Kosman, D J eng GM46787/GM/NIGMS NIH HHS/ Research Support, U.S. Gov't, P.H.S. 1996/10/04 J Biol Chem. 1996 Oct 4; 271(40):24885-93. doi: 10.1074/jbc.271.40.24885"