Severe oxidative stress induces protein mistranslation through ...

Severe oxidative stress induces protein mistranslation through impairment of an aminoacyl-tRNA synthetase editing site Jiqiang Linga and Dieter Sölla,b,1 a

Departments of Molecular Biophysics and Biochemistry, and bDepartment of Chemistry, Yale University, New Haven, CT 06520-8114

Contributed by Dieter Söll, January 11, 2010 (sent for review December 11, 2009)

Oxidative stress arises from excessive reactive oxygen species (ROS) and affects organisms of all three domains of life. Here we present a previously unknown pathway through which ROS may impact faithful protein synthesis. Aminoacyl-tRNA synthetases are key enzymes in the translation of the genetic code; they attach the correct amino acid to each tRNA species and hydrolyze an incorrectly attached amino acid in a process called editing. We show both in vitro and in vivo in Escherichia coli that ROS reduced the overall translational fidelity by impairing the editing activity of threonyl-tRNA synthetase. Hydrogen peroxide oxidized cysteine182 residue critical for editing, leading to Ser-tRNAThr formation and protein mistranslation that impaired growth of Escherichia coli. The presence of major heat shock proteases was required to allow cell growth in medium containing serine and hydrogen peroxide; this suggests that the mistranslated proteins were misfolded. aaRS ∣ quality control ∣ ROS ∣ translational fidelity

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ellular oxidative stress arises from an excess of reactive oxygen species (ROS), such as superoxide radicals, hydrogen peroxide (H2 O2 ), hydroxyl radicals, and hypochlorous acid (1–3). High intrinsic levels of oxidative stress occur in some mammalian cells; for instance in HeLa cells over 190 proteins with sulfenic acid modifications have been identified (4). Oxidative stress has been associated with the pathogenesis and progression of many human diseases (5). Although it is well established that ROS are able to damage biomolecules like proteins, DNA, RNA, and lipids, the molecular mechanisms of how oxidative stress contributes to human diseases remain largely elusive. In addition to the cell damaging role, recent studies have shown that ROS also participate in cell signaling pathways via reversible oxidation of critical cysteine (Cys) residues of regulatory proteins, such as OxyR and Hsp33 (6–8). Extensive studies have revealed that oxidative stress impacts cells at least partially through targeting the protein quality control machinery (9, 10). Protein quality control refers to the cellular regulation of protein folding and degradation (11). Aberrant proteins resulting from translation errors or posttranslational damage are normally misfolded; they then undergo unfolding and refolding by chaperones, degradation by proteases or the proteasome, or aggregation to cause deleterious effects to cells (11, 12). Oxidatively damaged proteins are carefully monitored by chaperones and are rapidly degraded (10, 13). Nevertheless, during severe oxidative stress conditions or in aged cells, the protein quality control capacity becomes saturated by the large amount of misfolded proteins, and protein aggregation prevails (5, 11). In addition to posttranslational damage, misfolded proteins can also be caused by errors in translation (12). Surprisingly, little is known as to whether oxidative stress affects translational fidelity, leading to an increased level of misfolded proteins. Fidelity in protein synthesis (with an error rate of one in 103 –104 ) is maintained via correct codon-anticodon recognition on the ribosome and accurate pairing of each amino acid with its 4028–4033 ∣ PNAS ∣ March 2, 2010 ∣ vol. 107 ∣ no. 9

cognate tRNA by the aminoacyl-tRNA synthetase (aaRS) (14, 15). An aaRS catalyzes aminoacylation in two steps: (a) activation of the amino acid with ATP to form an aminoacyl adenylate (aa-AMP), and (b) subsequent transfer of the amino acid moiety from aa-AMP to the tRNA (16). The error rate of tRNA selection by an aaRS is as low as one in 106 due to the complexity of tRNA molecules and a kinetic proofreading mechanism (16, 17). In contrast, selection of the correct amino acid is more challenging for the aaRS. While the aminoacylation active site excludes most noncognate amino acids, the enzyme activates certain amino acids or analogues that are structurally similar to the cognate amino acid (15) (Fig. 1). For example, threonyl-tRNA synthetase (ThrRS) misactivates serine (Ser) (18). Such errors are further corrected by a proofreading activity named editing (18–26). A double-sieve model that suggested that the active and editing sites are structurally distinct (27) was later confirmed by biochemical and structural analyses (28, 29). The editing activity of aaRSs is critical for maintaining the overall translational accuracy, as misacylated tRNAs that escape the editing step are effectively used by the ribosome (30–33). AaRS editing deficiency causes growth defects in bacteria (23, 34, 35), apoptosis in mammalian cells (36), and neurodegeneration in mice (12), mainly due to an increased level of misfolded proteins. In HeLa cells a number of aaRS enzymes (ThrRS, glutamyl-tRNA synthetase, and methionyl-tRNA synthetase) have been found to contain sulfenic acid modifications (4). Here we show that oxidative stress directly impaired the editing site of ThrRS, resulting in protein mistranslation. The lack of major heat shock proteases severely exacerbated the growth defect caused by mistranslation, suggesting that oxidative stress-induced mistranslation may harm cells through accumulation of misfolded proteins. Thus, our work revealed a previously unknown pathway through which ROS affects faithful protein synthesis. Results H2 O2 Induces ThrRS Editing Defect and Ser-tRNAThr Formation. Active site cysteines have been found susceptible to oxidation by ROS (6, 37), prompting us to search in the editing sites of aaRSs for critical Cys residues. Previous studies have revealed that ThrRS depends on a Cys residue (Fig. S1) for efficient editing and that replacing the editing site Cys with other amino acids causes Ser to be misacylated to tRNAThr species (18, 38). To study the impact of ROS on aminoacylation and editing activities, we tested Escherichia coli ThrRS in an ATP consumption assay, which would determine the overall editing activity of an aaRS against a noncognate amino acid. AaRSs hydrolyze ATP to form aa-AMP and aa-tRNA. In the presence of editing activity, aa-AMP or Author contributions: J.L. and D.S. designed research; J.L. performed research; J.L. and D.S. analyzed data; J.L. and D.S. wrote the paper. The authors declare no conflict of interest. 1

To whom correspondence should be addressed. E-mail: [email protected]

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aa-tRNA is subjected to hydrolysis, which initiates multiple rounds of ATP consumption. We showed that ThrRS could effectively misactivate (Table 1) and edit Ser (Fig. 2A), while the ATP consumption rate in the presence of Thr is negligible. Treating ThrRS with 4 mM H2 O2 for 5 min significantly reduced the ATP consumption rate, and addition of dithiothreitol (DTT) after H2 O2 treatment restored the editing activity, demonstrating that ThrRS oxidation by H2 O2 is reversible. A reduced ATP consumption rate could result from a decrease in either aminoacylation or editing efficiency. To distinguish the two possibilities, we employed pyrophosphate exchange and aminoacylation assays. The pyrophosphate exchange assay measures the radioactivity transferred from pyrophosphate to ATP during reversible amino acid activation and has been traditionally used to determine amino acid activation rates (39). Treatment of ThrRS with 1–4 mM H2 O2 did not affect the number of active sites or activation of Thr and Ser (Table 1, Fig. S2A), and the steady-state threonylation activities were similar in the presence or absence of H2 O2 (Table 2, Fig. 2B). In contrast, 0.2 mM H2 O2 started to cause Ser to be misacylated to tRNAThr (Fig. 2C). Treating H2 O2 oxidized ThrRS with DTT suppressed the misacylation activity (Fig. 2D). Together, these data reveal that the ThrRS editing activity is impaired by H2 O2 treatment, likely through reversible oxidation of the editing site Cys. Oxidation of the Editing Site Cys182 Residue. Oxidation of Cys resi-

dues can generate several products, e.g., disulfides, sulfenic (SOH), sulfinic (SO2 H), and sulfonic (SO3 H) acids (Fig. S3) (6). To analyze the oxidation product, we used sodium arsenite (NaAsO2 ), which specifically reduces sulfenic acids (40), to treat H2 O2 -oxidized ThrRS. NaAsO2 partially restored the editing efficiency of H2 O2 -treated ThrRS (Fig. 2D), suggesting that a Cys residue was at least partially modified to a sulfenic acid. In ThrRS, Cys182 has been shown to be essential for editing (38, 41). The C182A ThrRS variant displayed misacylation activity in the absence of ROS, confirming the critical role of Cys182 in editing (Fig. S2). Treatment of ThrRS C182A with H2 O2 did not further enhance misacylation. Using Ellman’s reagent 5, 5′dithiobis-(2-nitrobenzoic acid) (42), we determined that the wildtype (WT) ThrRS contained 1.9
0.1 free thiols per monomer,

H2 O2 Causes Missense Suppression of the β-Lactamase Gene in E. coli.

In vitro experiments clearly demonstrated that H2 O2 could damage the ThrRS editing site, resulting in misacylation of Ser to tRNAThr . To test whether such mistakes are conveyed to protein synthesis in vivo, a β-lactamase reporter system was employed to detect misincorporation of Ser at Thr codons. Previous studies have shown that Ser68 is critical for the activity of TEM β-lactamase and that an editing-defective ThrRS rescues the lactamase activity of the S68T variant via misincorporation of Ser at the codon Thr68 (33). E. coli strain XL1-blue expressing the WT β-lactamase could grow on ampicillin (Amp) plates with or without H2 O2 , while the strain expressing the S68T variant displayed Amp resistance only in the presence of H2 O2 (Fig. 3). Replacing the Ser68 codon (AGC) with a near-cognate asparagine codon (AAC) abolished the lactamase activity, which could not be rescued by H2 O2 . Colonies expressing S68T β-lactamase that appeared on plates with Amp and H2 O2 were streaked on Amp plates without H2 O2 and showed no growth. This confirmed that H2 O2 -induced β-lactamase activity from the S68T variant was not due to changes at the DNA level but was rather caused by ThrRS editing defects and missense suppression of the ACA codon68 with Ser. H2 O2 -Induced Ser-tRNAThr Formation Causes Protein Mistranslation.

ThrRS editing deficiency results in large-scale protein mistranslation, with Ser randomly inserted at Thr codons. To investigate the impact of H2 O2 -induced protein mistranslation, we tested the growth of E. coli strains in minimal media. The XL1-blue strain displayed a longer lag phase in the presence of 0.8 mM H2 O2 (Fig. 4A). Addition of Ser to the growth medium further prolonged the lag phase in the presence of H2 O2 but did not affect the growth in the absence of H2 O2 ; this suggests that oxidative stress-induced mistranslation has a negative effect on bacterial growth. The Ser toxicity in the presence of H2 O2 was suppressed by addition of Thr. In vitro experiments have shown that the ThrRS aminoacylation active site prefers Thr over Ser (Table 1). Therefore, in vivo, Thr would decrease the level of Ser-tRNAThr and improve translational accuracy under oxidative stress conditions. The inhibitory effect of Ser in the presence of H2 O2 was observed only in the lag phase but not in the exponential growth

Table 1. Pyrophosphate exchange activities of E. coli ThrRS with or without H2 O2 treatment Thr H2 O2 treated Yes No

Ser

kcat (sec−1 )

K M (mM)

kcat ∕K M (mM−1 sec−1 )

kcat (sec−1 )

K M (mM)

kcat ∕K M (mM−1 sec−1 )

Selectivity

11 ± 1 13 ± 1

0.082 ± 0.003 0.090 ± 0.015

130 ± 10 140 ± 30

10 ± 1 12 ± 1

58 ± 7 53 ± 11

0.17 ± 0.03 0.23 ± 0.05

760 610

These values are the average of three repeats with standard deviations indicated.

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Fig. 1. Double-sieve model of editing by aaRSs. The aaRS aminoacylation active site as the first sieve accepts the cognate (shown in green) and structurally similar near-cognate (i.e., Ser for ThrRS, shown in red) amino acids but rejects the majority of noncognate amino acids. The editing site serves as the second sieve to hydrolyze only the misactivated products (aminoacyl adenylate or aa-tRNA). The correct aa-tRNA is excluded from the editing site and participates in protein synthesis.

whereas the C182A variant contained only 1.0
0.1 free thiol per monomer. Treating the WT ThrRS with H2 O2 decreased the number of free thiols to 0.7
0.1, consistent with oxidation of roughly one Cys residue. This reveals that Cys182 is one of the two Cys residues exposed to solvent and is thus likely the target for oxidation. To confirm Cys182 oxidation, the WT ThrRS was treated with 1 mM H2 O2 , dialyzed to remove residue H2 O2 , digested with chymotrypsin, and subjected to mass spectrometry [liquid chromatography (LC) MS/MS] analyses. The MS data revealed that Cys182 was oxidized to a Cys sulfinic acid (Fig. S4), a higher order oxidation product derived from Cys sulfenic acids. In an attempt to detect Cys sulfenic acids, we labeled the oxidized ThrRS with dimedone and 7-chloro-4-nitrobenz-2oxa-1,3-diazole (NBD-Cl), respectively, which forms adducts with protein sulfenic acids (43, 44). LC MS/MS analyses did not identify dimedone or NBD-labeled Cys derivatives, suggesting that the sulfenic acid form of Cys182 is transient and can be further oxidized to Cys sulfinic acids or even disulfides.

Fig. 2. ROS cause editing defect and misacylation by WT ThrRS. (A) Total editing activity of ThrRS (1.5 μM) in the presence of tRNAThr transcript (2 μM) and cold Ser (10 mM) or cold Thr (10 mM). Treatment of ThrRS with H2 O2 (4 mM) at 37 °C for 5 min significantly reduces ThrRS editing efficiency. Subsequent treatment with DTT (11 mM) recovers the editing activity. (B) Threonylation (25 μM [14 C]Thr, 5 mg∕ml total E. coli tRNA containing 15 μM tRNAThr ) by ThrRS (37.5 nM). Treating ThrRS with H2 O2 (4 mM) and/ or DTT (11 mM) does not affect the aminoacylation activity. (C) Serylation (30 μM [14 C]Ser, 5 mg∕ml total E. coli tRNA containing 15 μM tRNAThr ) by ThrRS (2.3 μM) in the presence and absence of H2 O2 . Treatment of ThrRS with H2 O2 (0.2–4 mM) at 37 °C for 5 min induces Ser-tRNAThr formation; 0.2 mM is the lowest H2 O2 concentration at which misacylation is detected. (D) Serylation (30 μM [14 C]Ser, 5 mg∕ml total E. coli tRNA containing 15 μM tRNAThr ) by ThrRS (2.3 μM) is suppressed by DTT and sodium arsenite. ThrRS is treated with H2 O2 (1 mM) at 37 °C for 5 min and followed by addition of DTT (11 mM) or sodium arsenite (11 mM). tRNA is added last to initiate the aminoacylation reaction.

phase. E. coli cells exposed to H2 O2 trigger an OxyR stress response pathway that decreases the intracellular H2 O2 level and enhances chaperone activities (1). The prolonged lag phase may reflect the time cells take to reduce the initial H2 O2 levels, repair damage, and better tolerate an increased level of aberrant proteins. Proteases Protect E. coli from the Deleterious Effects of Mistranslation. Mistranslated proteins are more susceptible to misfolding

and degradation by proteases. We reasoned that oxidative stress-induced protein mistranslation might lead to an increased level of misfolded proteins. While the WT E. coli strain MG1655 appeared to tolerate a higher level of oxidative stress and H2 O2 -induced mistranslation (Fig. 4B), the growth of KY2350, a protease-deficient derivative of MG1655, was inhibited by H2 O2 and an excess of Ser in minimal media (Fig. 4C). Addition of Thr was only able to partially rescue the growth defect of KY2350 in the presence of H2 O2 . It is reasonable to speculate that due to the lack of protease activities in KY2350, the misfolded proteins resulting from mistranslation would overwhelm the protein quality control machinery and form harmful aggregates. A dose-response growth curve analysis revealed that Ser exhibited an inhibitory effect on KY2350 in the presence of 200–1,000 μM H2 O2 , suggesting that ThrRS editing activity might be partially impaired by a minimal level of 200 μM H2 O2 in the media (Fig. S5A).

Discussion Physiological Impact of ROS-Induced ThrRS Editing Defect. A common

type of stress in organisms from all three domains of life is oxidative stress accompanied by an increasing level of ROS. Here we show that H2 O2 can oxidize a critical editing site Cys of ThrRS, resulting in Ser-tRNAThr formation and protein mistranslation. The minimal H2 O2 concentration required to impair ThrRS editing is about 200 μM both in vitro and in vivo (Figs. 2 and 3 and Fig. S5A). The initial bacterial defense against peroxide stress senses low in vivo concentrations (20 mM) is unclear (46, 47). At the concentrations required to induce protein mistranslation (0.2–0.5 mM) H2 O2 does not significantly kill E. coli as indicated by a survival assay (Fig. 4B), suggesting that ROS-induced mistranslation might be bacteriostatic but not bactericidal.

phosphatases (7, 8). A common switch for ROS-signaled pathways is the reversible oxidation of Cys residues, which allows the sensor protein to detect the flux of cellular ROS levels. The active site Cys residues in signaling proteins are often first oxidized to sulfenic acids, which can be stabilized by forming disulfide bonds with intramolecular or intermolecular thiols (6, 51). Both sulfenic acids and disulfide bonds are reducible by cellular reductants such as thioredoxin and glutaredoxin (6). Oxidation of ThrRS results in misincorporation of Ser, a common site for phosphorylation, at Thr codons. It is thus possible that regulation of editing activity by ROS might involve signaling pathways.

Oxidation of Cys Residues in ThrRS by H2 O2. Chemical and mass spectrometry experiments suggested that Cys182 of ThrRS was oxidized to a Cys sulfenic acid by H2 O2 , which could be reduced by sodium arsenite or DTT. While DTT completely restored the editing activity of the oxidized ThrRS, sodium arsenite only partially rescued the editing efficiency (Fig. 2). It is therefore possible that the Cys sulfenic acid further forms a disulfide, which is reducible by DTT but not by sodium arsenite. The ThrRS editing site residues (including Cys182 and several histidines) are similar to the active sites of Cys proteases (38), which are known to form sulfenic acids (6), further supporting the notion that a Cys sulfenic acid forms in the oxidized ThrRS editing site. In addition to the editing site Cys, the aminoacylation active site contains a Cys (Cys334) involved in zinc binding (48), which might also be oxidized by ROS. However, under tested conditions neither the aminoacylation activity nor the selectivity for Thr over Ser was changed upon ThrRS oxidation (Tables 1 and 2), suggesting that the ROS damage of ThrRS mainly causes an editing defect.

Editing and Protein Synthesis Fidelity. Four decades have passed since editing has been initially discovered, yet the physiological roles of editing are only beginning to be understood (15). The editing activities of many aaRSs are strictly conserved in all three domains of life, implying a critical role of editing throughout evolution. Disruption of the editing activity in certain aaRSs causes bacterial growth defects and apoptosis in mammalian cells (34, 36). Furthermore, an editing site mutation in alanyl-tRNA synthetase only slightly enhances misacylation but leads to an increased level of protein misfolding and severe neurodegeneration in sticky mice (12). Terminally differentiated neurons are particularly sensitive to misfolded proteins, presumably because such cells cannot dilute misfolded proteins through cell division. Further, the nervous system produces a high level of ROS, as

ROS, Cell Damage, and Signaling. ROS causes protein oxidation which generates carbonyls, indicators of damaged proteins (10). A moderate level of carbonylation enhances degradation of damaged proteins by proteases and the proteasome, but heavily oxidized proteins can form aggregates and harm cells (10, 13) (Fig. 5). The protein synthesis machinery might also be affected by ROS. For example, glutamyl-tRNA synthetase oxidized by H2 O2 is shown to be a substrate for the thiol-disulfide oxidoreductase DsbA (49); three HeLa cell aaRSs (ThrRS, glutamyltRNA synthetase, and methionyl-tRNA synthetase) have been found to carry sulfenic acid modifications (4); recently it has also been shown that ROS increase translational errors by causing methionine to be misacylated to noncognate tRNAs (50). Increasing evidence has supported that ROS play regulatory roles as cell signals (7, 37, 51). Among the well-characterized ROS sensor proteins are OxyR, Hsp33, and protein tyrosine Ling and Söll

Fig. 5. Model for oxidative stress-induced mistranslation. ROS cause editing defects to ThrRS, leading to global protein mistranslation. While certain mistranslated proteins may participate in signal transduction, the majority of incorrectly made proteins are misfolded, overwhelming the protein quality control system. Accumulation of protein aggregates will eventually damage the cell. PNAS ∣

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Fig. 4. Growth curves of E. coli strains in the presence (closed symbols) and absence (open symbols) of H2 O2 (0.8–1 mM). (A) E. coli strain XL1-blue. (B) WT E. coli strain MG1655. (C) E. coli strain KY2350, a protease-deficient derivative of MG1655. Squares, minimal media without Ser or Thr; circles, minimal media with Ser (5 mM) but without Thr; triangles, minimal media with Ser (5 mM) and Thr (5 mM). Plots represent the average of three repeats with standard deviations indicated.

neurons are low in antioxidant capacity and consume more oxygen for energy production than other cells (5). Recent studies have shown that in HeLa cells with high oxidative stress levels, ThrRS contains sulfenic acid modifications (4), suggesting that mammalian ThrRSs are susceptible to oxidation. It remains unclear whether oxidative stress affects ThrRS aminoacylation fidelity in mammalian cells. Although editing is a crucial activity, loss of editing can be beneficial under certain extreme conditions (33, 52). For example, when the cognate amino acid is depleted, the growth rate of Acinetobacter baylyi increased in the presence of an editing-defective isoleucyl-tRNA synthetase (52). It has also been shown that E. coli can survive certain selective pressures only if the protein mistranslation level is increased (30, 33). The interplay between stresses, editing, and adaptation of organisms during evolution raises a variety of questions in the field of protein synthesis quality control. The proposed pathway of ROS-induced mistranslation provides a fascinating example of such interactions between organisms and stresses. Experimental Procedures Strains, Plasmids, and Protein Expression. E. coli strain MG1655 and its protease-deficient derivative KY2350 [ΔhslV U, ΔðclpPX-lonÞ] (53) were gifts from M. Kanemori (HSP Research institute, Kyoto, Japan). ThrRS was cloned into pET28a expression vector (Novagen) with an N-terminal six-His tag. Expression of ThrRS was induced at 37 °C for 4 h with 0.5 mM isopropyl β-D-1-thiogalactopyranoside (IPTG) in E. coli strain BL21-codon plus in Luria-Bertani (LB) media. His-tagged ThrRS were purified according to standard procedures. β-lactamase gene variants were cloned into a pTech vector with a constitutive lipoprotein (lpp) promoter and a chloramphenicol (Cm) resistance gene.

sphate exchange experiment contained 100 mM Na-HEPES pH 7.2, 30 mM KCl, 10 mM MgCl2 , 2 mM KF, 2 mM ATP, 2 mM [32 P]-pyrophosphate (10 mCi∕ml in the stock and 1 cpm∕pmole in the final reaction), 10–1,000 μM Thr or 5–500 mM Ser, and 150 nM ThrRS. Aminoacylation experiments were done in the presence of 100 mM Na-HEPES pH 7.2, 30 mM KCl, 10 mM MgCl2 , 2 mM ATP, 25 μM [14 C]-Thr (44 μCi∕ml or 190 cpm∕pmole) or 30 μM [14 C]-Ser (49 μCi∕ml or 180 cpm∕pmole), 2–14 μM tRNA transcript or 5 mg∕ml total tRNA (from E. coli MRE 600, Roche), and 37–2,300 nM ThrRS. For mass spectrometry analyses, ThrRS was oxidized with 1 mM H2 O2 for 5 min at 37 °C. The remaining H2 O2 was removed by extensive dialysis, and the resulting sample was labeled with 5 mM dimedone (Sigma-Aldrich) or 1 mM NBD-Cl (SigmaAldrich) for 1 h at room temperature in the anaerobic chamber. LC MS/MS was performed on labeled ThrRS at W. M. Keck Foundation Biotechnology Research Lab at Yale University. In Vivo Assays. For growth curve measurement, the minimal media contained 48 mM Na2 HPO4 , 22 mM KH2 PO4 , 8.5 mM NaCl, 23 mM NH4 Cl, 2 mM MgSO4 , 0.1 mM CaCl2 , 1% glucose, 0.1 mM thiamine, 20 μg∕ml of each amino acid except Cys, Thr, and Ser, and indicated concentrations of Ser, Thr, and H2 O2 . E. coli cells were grown in LB media overnight, collected with centrifugation, washed twice with minimal media, diluted to A600 ∼ 0.02, and grown at 37 °C in minimal media. In the β-lactamase reporter assay, E. coli XL1-blue cells expressing β-lactamase variants were grown in LB media with 25 μg∕ml Cm overnight, collected with centrifugation, washed twice with minimal media, and streaked on minimal medium plates with 25 μg∕ml Cm, 30 μg∕ml Amp, with or without 0.3 mM H2 O2 . Plates were grown at 37 °C for 24–48 h.

In Vitro Assays. AaRS experiments were performed as described (23, 54). The ATP consumption reaction mix contained 2 U∕ml of yeast pyrophosphatase (Roche), 10 mM Ser, 2–14 μM cognate tRNA, 2 mM [γ-32 P]ATP (10 mCi∕ml in the stock, and 5 cpm∕pmole in the final reaction), 100 mM Na-HEPES (pH 7.2), 30 mM KCl, 10 mM MgCl2 , and 1.5 μM ThrRS. The pyropho-

ACKNOWLEDGMENTS. We thank Dr. M. Kanemori for E. coli strains, Dr. M. Ibba for insightful discussion on the project, A. Lieberman for experimental support, Dr. D. Su and L. Randau for critical reading of the manuscript, and other members of Söll lab for help. This work was supported by a grant from the National Institute of General Medical Sciences and a Brown-Coxe Postdoctoral Fellowship.

1. Farr SB, Kogoma T (1991) Oxidative stress responses in Escherichia coli and Salmonella typhimurium. Microbiol Rev 55:561–585. 2. Finkel T, Holbrook NJ (2000) Oxidants, oxidative stress and the biology of ageing. Nature 408:239–247. 3. Winter J, Ilbert M, Graf PC, Ozcelik D, Jakob U (2008) Bleach activates a redoxregulated chaperone by oxidative protein unfolding. Cell 135:691–701. 4. Leonard SE, Reddie KG, Carroll KS (2009) Mining the thiol proteome for sulfenic acid modifications reveals new targets for oxidation in cells. ACS Chem Biol 4:783–799. 5. Mariani E, Polidori MC, Cherubini A, Mecocci P (2005) Oxidative stress in brain aging, neurodegenerative and vascular diseases: An overview. J Chromatogr B 827:65–75. 6. Poole LB, Karplus PA, Claiborne A (2004) Protein sulfenic acids in redox signaling. Annu Rev Pharmacol Toxicol 44:325–347. 7. Veal EA, Day AM, Morgan BA (2007) Hydrogen peroxide sensing and signaling. Mol Cell 26:1–14. 8. Barford D (2004) The role of cysteine residues as redox-sensitive regulatory switches. Curr Opin Struct Biol 14:679–686. 9. Stadtman ER (1992) Protein oxidation and aging. Science 257:1220–1224. 10. Nyström T (2005) Role of oxidative carbonylation in protein quality control and senescence. EMBO J 24:1311–1317. 11. Balch WE, Morimoto RI, Dillin A, Kelly JW (2008) Adapting proteostasis for disease intervention. Science 319:916–919. 12. Lee JW, et al. (2006) Editing-defective tRNA synthetase causes protein misfolding and neurodegeneration. Nature 443:50–55. 13. Dukan S, et al. (2000) Protein oxidation in response to increased transcriptional or translational errors. Proc Natl Acad Sci USA 97:5746–5749. 14. Ogle JM, Ramakrishnan V (2005) Structural insights into translational fidelity. Annu Rev Biochem 74:129–177. 15. Ling J, Reynolds N, Ibba M (2009) Aminoacyl-tRNA synthesis and translational quality control. Annu Rev Microbiol 63:61–78. 16. Ibba M, Söll D (2000) Aminoacyl-tRNA synthesis. Annu Rev Biochem 69:617–650. 17. Guth EC, Francklyn CS (2007) Kinetic discrimination of tRNA identity by the conserved motif 2 loop of a class II aminoacyl-tRNA synthetase. Mol Cell 25:531–542. 18. Dock-Bregeon A, et al. (2000) Transfer RNA-mediated editing in threonyl-tRNA synthetase: The class II solution to the double discrimination problem. Cell 103:877–884.

19. Baldwin AN, Berg P (1966) Transfer ribonucleic acid-induced hydrolysis of valyladenylate bound to isoleucyl ribonucleic acid synthetase. J Biol Chem 241:839–845. 20. Beebe K, Ribas de Pouplana L, Schimmel P (2003) Elucidation of tRNA-dependent editing by a class II tRNA synthetase and significance for cell viability. EMBO J 22:668–675. 21. Fersht AR, Kaethner MM (1976) Enzyme hyperspecificity: Rejection of threonine by the valyl-tRNA synthetase by misacylation and hydrolytic editing. Biochemistry 15:3342–3346. 22. Yarus M (1972) Phenylalanyl-tRNA synthetase and isoleucyl-tRNA Phe: A possible verification mechanism for aminoacyl-tRNA. Proc Natl Acad Sci USA 69:1915–1919. 23. Roy H, Ling J, Irnov M, Ibba M (2004) Post-transfer editing in vitro and in vivo by the beta subunit of phenylalanyl-tRNA synthetase. EMBO J 23:4639–4648. 24. Beuning PJ, Musier-Forsyth K (2000) Hydrolytic editing by a class II aminoacyl-tRNA synthetase. Proc Natl Acad Sci USA 97:8916–8920. 25. Chen JF, Guo NN, Li T, Wang ED, Wang YL (2000) CP1 domain in Escherichia coli leucyltRNA synthetase is crucial for its editing function. Biochemistry 39:6726–6731. 26. Lincecum TL, Jr., et al. (2003) Structural and mechanistic basis of pre- and posttransfer editing by leucyl-tRNA synthetase. Mol Cell 11:951–963. 27. Fersht AR (1977) Editing mechanisms in protein synthesis. Rejection of valine by the isoleucyl-tRNA synthetase. Biochemistry 16:1025–1030. 28. Schmidt E, Schimmel P (1994) Mutational isolation of a sieve for editing in a transfer RNA synthetase. Science 264:265–267. 29. Nureki O, et al. (1998) Enzyme structure with two catalytic sites for double-sieve selection of substrate. Science 280:578–582. 30. Min B, et al. (2003) Protein synthesis in Escherichia coli with mischarged tRNA. J Bacteriol 185:3524–3526. 31. Nangle LA, de Crécy-Lagard V, Döring V, Schimmel P (2002) Genetic code ambiguity. Cell viability related to the severity of editing defects in mutant tRNA synthetases. J Biol Chem 277:45729–45733. 32. Ling J, Yadavalli SS, Ibba M (2007) Phenylalanyl-tRNA synthetase editing defects result in efficient mistranslation of phenylalanine codons as tyrosine. RNA 13:1881–1886. 33. Ruan B, et al. (2008) Quality control despite mistranslation caused by an ambiguous genetic code. Proc Natl Acad Sci USA 105:16502–16507.

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45. Aslund F, Zheng M, Beckwith J, Storz G (1999) Regulation of the OxyR transcription factor by hydrogen peroxide and the cellular thiol-disulfide status. Proc Natl Acad Sci USA 96:6161–6165. 46. Miller RA, Britigan BE (1997) Role of oxidants in microbial pathophysiology. Clin Microbiol Rev 10:1–18. 47. Imlay JA, Linn S (1987) Mutagenesis and stress responses induced in Escherichia coli by hydrogen peroxide. J Bacteriol 169:2967–2976. 48. Sankaranarayanan R, et al. (2000) Zinc ion mediated amino acid discrimination by threonyltRNA synthetase. Nat Struct Biol 7:461–465. 49. Leichert LI, Jakob U (2004) Protein thiol modifications visualized in vivo. PLoS Biol 2:e333. 50. Netzer N, et al. (2009) Innate immune and chemically triggered oxidative stress modifies translational fidelity. Nature 462:522–526. 51. D’Autreaux B, Toledano MB (2007) ROS as signalling molecules: Mechanisms that generate specificity in ROS homeostasis. Nat Rev Mol Cell Biol 8:813–824. 52. Bacher JM, Waas WF, Metzgar D, Crécy-Lagard V, Schimmel P (2007) Genetic code ambiguity confers a selective advantage on Acinetobacter baylyi. J Bacteriol 189:6494–6496. 53. Kanemori M, Yanagi H, Yura T (1999) The ATP-dependent HslVU/ClpQY protease participates in turnover of cell division inhibitor SulA in Escherichia coli. J Bacteriol 181:3674–3680. 54. Ling J, Roy H, Ibba M (2007) Mechanism of tRNA-dependent editing in translational quality control. Proc Natl Acad Sci USA 104:72–77.

BIOCHEMISTRY

34. Bacher JM, Crécy-Lagard V, Schimmel PR (2005) Inhibited cell growth and protein functional changes from an editing-defective tRNA synthetase. Proc Natl Acad Sci USA 102:1697–1701. 35. Karkhanis VA, Mascarenhas AP, Martinis SA (2007) Amino acid toxicities of Escherichia coli that are prevented by leucyl-tRNA synthetase amino acid editing. J Bacteriol 189:8765–8768. 36. Nangle LA, Motta CM, Schimmel P (2006) Global effects of mistranslation from an editing defect in mammalian cells. Chem Biol 13:1091–1100. 37. Poole LB, Nelson KJ (2008) Discovering mechanisms of signaling-mediated cysteine oxidation. Curr Opin Chem Biol 12:18–24. 38. Dock-Bregeon AC, et al. (2004) Achieving error-free translation: The mechanism of proofreading of threonyl-tRNA synthetase at atomic resolution. Mol Cell 16:375–386. 39. Francklyn CS, First EA, Perona JJ, Hou YM (2008) Methods for kinetic and thermodynamic analysis of aminoacyl-tRNA synthetases. Methods 44:100–118. 40. Kim SO, et al. (2002) OxyR: A molecular code for redox-related signaling. Cell 109:383–396. 41. Waas WF, Schimmel P (2007) Evidence that tRNA synthetase-directed proton transfer stops mistranslation. Biochemistry 46:12062–12070. 42. Ellman GL (1959) Tissue sulfhydryl groups. Arch Biochem Biophys 82:70–77. 43. Benitez LV, Allison WS (1974) The inactivation of the acyl phosphatase activity catalyzed by the sulfenic acid form of glyceraldehyde 3-phosphate dehydrogenase by dimedone and olefins. J Biol Chem 249:6234–6243. 44. Ellis HR, Poole LB (1997) Novel application of 7-chloro-4-nitrobenzo-2-oxa-1,3-diazole to identify cysteine sulfenic acid in the AhpC component of alkyl hydroperoxide reductase. Biochemistry 36:15013–15018.

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vol. 107 ∣

no. 9 ∣

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