The Saccharomyces cerevisiae Proteome of Oxidized Protein Thiols

Moan, Natacha Le; Clément, Gilles; Maout, Sophie Le; Tacnet, Frédérique; Toledano, Michel B.

doi:10.1074/jbc.m513346200

Cited by 149 publications

(72 citation statements)

References 56 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…4) and concluded from these results that E. coli cells are exposed to a considerable amount of ROS during aerobic growth. This observation agrees with earlier reports in both E. coli (10) and yeast cells (22) and provides an excellent explanation for the essential roles that the thioredoxin and glutaredoxin systems play in maintaining the reducing character of pro-and eukaryotic cytoplasm (23).…”

Section: Oxicat Provides a Quantitative Assessment Of The Cellular Redoxsupporting

confidence: 82%

“…This mechanism might contribute to the Pasteur effect in bacteria, which describes the influence of oxygen on the glucose metabolism (27). Similar observations have recently also been made in aerobically growing yeast cells, where a large proportion of glycolytic enzymes including GapA were shown to be oxidatively modified in vivo (22).…”

Section: Oxicat Provides a Quantitative Assessment Of The Cellular Redoxsupporting

confidence: 58%

“…It is via reversible thiol modifications that transcriptional (e.g., OxyR, Yap1) and posttranslational (e.g., Hsp33, Prx-2) responses are triggered and that physiological processes (e.g., GapA) start to change during oxidative stress conditions (9). To identify target proteins that use redoxsensitive thiol groups to modulate their protein activity, the monitoring of relative changes in the overall thiol oxidation state (10,11,13,15,22) or the selective identification of proteins with distinct thiol modifications (12, 37) is an invaluable approach. Previously established methods, however, were unable to directly quantify the extent of thiol-modified protein and identify the cysteines affected.…”

Section: Discussionmentioning

confidence: 99%

See 2 more Smart Citations

Quantifying changes in the thiol redox proteome upon oxidative stress in vivo

Leichert

Gehrke

Gudiseva

et al. 2008

Proc. Natl. Acad. Sci. U.S.A.

486

542

View full text Add to dashboard Cite

Antimicrobial levels of reactive oxygen species (ROS) are produced by the mammalian host defense to kill invading bacteria and limit bacterial colonization. One main in vivo target of ROS is the thiol group of proteins. We have developed a quantitative thiol trapping technique termed OxICAT to identify physiologically important target proteins of hydrogen peroxide (H 2O2) and hypochlorite (NaOCl) stress in vivo. OxICAT allows the precise quantification of oxidative thiol modifications in hundreds of different proteins in a single experiment. It also identifies the affected proteins and defines their redox-sensitive cysteine(s). Using this technique, we identified a group of Escherichia coli proteins with significantly (30 -90%) oxidatively modified thiol groups, which appear to be specifically sensitive to either H 2O2 or NaOCl stress. These results indicate that individual oxidants target distinct proteins in vivo. Conditionally essential E. coli genes encode one-third of redoxsensitive proteins, a finding that might explain the bacteriostatic effect of oxidative stress treatment. We identified a select group of redox-regulated proteins, which protect E. coli against oxidative stress conditions. These experiments illustrate that OxICAT, which can be used in a variety of different cell types and organisms, is a powerful tool to identify, quantify, and monitor oxidative thiol modifications in vivo.chaperone ͉ proteomics ͉ thiol modification

show abstract

Section: Oxicat Provides a Quantitative Assessment Of The Cellular Redoxsupporting

confidence: 82%

Section: Oxicat Provides a Quantitative Assessment Of The Cellular Redoxsupporting

confidence: 58%

Section: Discussionmentioning

confidence: 99%

See 1 more Smart Citation

Quantifying changes in the thiol redox proteome upon oxidative stress in vivo

Leichert

Gehrke

Gudiseva

et al. 2008

Proc. Natl. Acad. Sci. U.S.A.

486

542

View full text Add to dashboard Cite

show abstract

“…In another systematic study focused onto the oxidation of protein thiols in yeast, the oxidized proteome of unstressed cells was identified [44]. In this survey, among 200 mostly cytoplasmatic proteins, cysteines were reported to be oxidized at a various extent.…”

Section: Vdacs and Rosmentioning

confidence: 99%

Swapping of the N‐terminus of VDAC1 with VDAC3 restores full activity of the channel and confers anti‐aging features to the cell

et al. 2010

View full text Add to dashboard Cite

a b s t r a c tVoltage-dependent anion-selective channels (VDACs) are pore-forming proteins allowing the permeability of the mitochondrial outer membrane. The VDAC3 isoform is the least abundant and least active in a complementation assay performed in a yeast strain devoid of porin-1. We swapped the VDAC3 N-terminal 20 amino acids with homologous sequences from the other isoforms. The substitution of the VDAC3 N-terminus with the VDAC1 N-terminus caused the chimaera to become more active than VDAC1. The VDAC2 N-terminus improved VDAC3 activity, though to a lesser extent. The VDAC3 carrying the VDAC1 N-terminus was able to complement the lack of the yeast porin in mitochondrial respiration and in modulation of reactive oxygen species (ROS). This chimaera increased life span, indicating a more efficient bioenergetic metabolism and/or a better protection from ROS.

show abstract

“…In bacteria and yeast, where Gpx is a minor scavenger or absent altogether, the evidence of protein thiol oxidation by physiological doses of H 2 O 2 is not strong. High H 2 O 2 doses have typically been employed in proteomics studies that detect oxidized proteins (121,122). One wonders, then, whether glutaredoxins and thioredoxins are actually needed only when H 2 O 2 stress is of such long duration as to compensate for the sluggish reactivity of protein thiols; whether they repair a small cohort of extremely reactive thiolate enzymes that have so far escaped detection; whether thiolate oxidations are primarily driven by reactions with oxygen or hydroxyl radicals, rather than H 2 O 2 ; or whether disulfide stress arises in natural environments from a different types of stressor, mimicked by thiol agents such as diamide.…”

Section: 52mentioning

confidence: 99%

Cellular Defenses against Superoxide and Hydrogen Peroxide

Imlay

2008

Annu. Rev. Biochem.

1,335

1,310

View full text Add to dashboard Cite

Life evolved in an anaerobic world; therefore, fundamental enzymatic mechanisms and biochemical pathways were refined and integrated into metabolism in the absence of any selective pressure to avoid reactivity with oxygen. After photosystem 2 appeared, environmental oxygen levels rose very slowly. During this time microorganisms acquired oxygen tolerance by jettisoning enzymes that use glycyl radicals and low-potential iron-sulfur clusters, which can be directly poisoned by oxygen. They also developed mechanisms to defend themselves against O 2 − and hydrogen peroxide, partially reduced oxygen species that are generated as inadvertent by-products of aerobic metabolism. These species are more chemically reactive than is molecular oxygen itself. Contemporary organisms have inherited both the vulnerabilities and the defenses of these ancestral microbes. Current research seeks to identify these, and bacteria comprise an exceptionally accessible experimental system that has provided the many of the answers. This manuscript reviews recent developments and identifies remaining puzzles.

show abstract

The Saccharomyces cerevisiae Proteome of Oxidized Protein Thiols

Cited by 149 publications

References 56 publications

Quantifying changes in the thiol redox proteome upon oxidative stress in vivo

Quantifying changes in the thiol redox proteome upon oxidative stress in vivo

Swapping of the N‐terminus of VDAC1 with VDAC3 restores full activity of the channel and confers anti‐aging features to the cell

Cellular Defenses against Superoxide and Hydrogen Peroxide

Contact Info

Product

Resources

About