Construction and Physiological Analysis of a Xanthomonas Mutant To Examine the Role of the oxyR Gene in Oxidant-Induced Protection against Peroxide Killing

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Journal of Bacteriology, August 1998, p. 3988-3991, Vol. 180, No. 15
0021-9193/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Construction and Physiological Analysis of a Xanthomonas Mutant To Examine the Role of the oxyR Gene in Oxidant-Induced Protection against Peroxide Killing

Skorn Mongkolsuk,¹^,²^,^* Rojana Sukchawalit,¹ Suvit Loprasert,¹ Wipa Praituan,¹ and Apichat Upaichit²

Laboratory of Biotechnology, Chulabhorn Research Institute, Lak Si, Bangkok 10210,¹ and Department of Biotechnology, Faculty of Science, Mahidol University, Rama 6 Rd, Bangkok 10400,² Thailand

Received 19 March 1998/Accepted 26 May 1998

	ABSTRACT

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We constructed and characterized a Xanthomonas campestris pv. phaseoli oxyR mutant. The mutant was hypersensitive to H₂O₂and menadione killing and had reduced aerobic plating efficiency.The oxidants' induction of the catalase and ahpC genes was alsoabolished in the mutant. Analysis of the adaptive responses showedthat hydrogen peroxide-induced protection against hydrogen peroxidewas lost, while menadione-induced protection against hydrogenperoxide was retained in the oxyR mutant. These results show thatX. campestris pv. phaseoli oxyR is essential to peroxide adaptationand revealed the existence of a novel superoxide-inducible peroxideprotection system that is independent of OxyR.

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Inducible stress responses are important components of bacterial survival under stressful conditions. Exposure to a low levelof one stress can induce a protective response against subsequentexposure to lethal levels of the same (adaptive response) or unrelated(cross-protective response) stresses (3, 5, 7, 23,32). OxyR, a global regulator for peroxide stress response,is a bifunctional protein that acts as a peroxide sensor and atranscription activator in response to oxidative stress (2,31, 33). It regulates many genes involved in the scavengingof peroxides (i.e., catalase and alkyl hydroperoxide reductase[ahpR] [5, 30]) and the prevention and repair of oxidativedamage for macromolecules (i.e., glutathione reductase and dps)(5, 17, 19, 29).

The inducible adaptive and cross-protective responses against peroxide killing could play important roles in plant-microbeinteractions. Active plant defense response against microbes involvesincreased production of H₂O₂, organic peroxides, and superoxides(14). These reactive oxygen species can inhibit growth and killinvading microbes. During initial interactions, bacteria are exposedto low-concentration mixtures of superoxide anions and peroxides(14). These could induce protection against subsequent exposureto higher concentrations of reactive oxygen species that prolongbacterial survival in the plant and may affect disease progression.Moreover, normal aerobic metabolism also generates significantquantities of reactive oxygen species (8, 9), which haveto be rapidly detoxified.

We have isolated and characterized an oxyR from Xanthomonas campestris pv. phaseoli (15, 22). The gene has unique organizationand transcription regulation (1, 16, 23). This fact, coupledwith observations that many aspects of Xanthomonas oxidative stressresponse differ from those of other bacteria (1, 16), leadsus to investigate OxyR function in X. campestris pv. phaseoli.

Construction of the oxyR mutants. Inactivation of the oxyR gene was achieved by insertion of a KpnI-digested gentamicin resistance gene from pUCGM (27) intoa KpnI site located in the coding region of oxyR on plasmid pUC18(15). The new recombinant plasmid, designated poxyR::Gm, waselectroporated into X. campestris pv. phaseoli as previously described(21). Transformants were selected on SB (0.5% yeast extract,0.5% peptone, 0.5% sucrose, 0.1% glutamic acid; pH 7.0) platescontaining 15 µg of gentamicin per ml. Gm^r colonies were subsequently scored for an Ap^s phenotype. Many colonies had Ap^s Gm^r phenotypes, indicating an exchange of the mutated oxyR for itsfunctional counterpart. These colonies were selected for furthercharacterization by both Southern and Western analyses, whichconfirmed that the mutated oxyR had replaced the functional genein these cells with an Ap^s Gm^r phenotype (data not shown).

Physiological characterization of the mutant. We noticed that the oxyR mutants formed smaller colonies than did the parental strain on SB plates. Mutations in genes involvedin oxidative stress response often lead to defects in aerobicplating efficiency (18, 34). All of the X. campestris pv.phaseoli oxyR mutant strains tested showed a 10⁴ decrease in aerobic plating efficiency on SB plates comparedto that for the parental strain. This effect could be reversedby the addition of 10 mM sodium pyruvate (18, 24, 34) toSB plates (Fig. 1), suggesting that accumulation of peroxidesin the oxyR mutants probably caused the defect. To test the hypothesis,plasmids containing Xanthomonas genes involved in oxidative stressprotection were transformed into the mutant and their platingefficiency was determined. The results are shown in Fig. 1. Ahigh level of superoxide dismutase (pUFR-SOD [28]) or microaerobicgrowth conditions had no effect on the plating efficiency of themutant. An increased level of enzymes directly involved in peroxidemetabolism (e.g., monofunctional catalase [pkat] [21] and AhpRsubunits C and F [pUFR-ahpCF]) restored the plating efficiencyof the mutant so that it was close to that of the parental strain.An increased level of catalase was less efficient than AhpR atcomplementing the defect, probably due to the inability of catalaseto metabolize organic peroxide. Unexpectedly, increased levelsof AhpF (pUFR-ahpF) alone restored the level of plating efficiencysimilar to the level attained by overexpression of catalase, whilehigh levels of AhpC (pahpC [15]) alone were not as effective(Fig. 1). Purified AhpC and AhpF can use both H₂O₂ and organicperoxide as substrates (25, 26). On the other hand, we haveobserved in X. campestris pv. phaseoli that increased expressionof either ahpC (15) or ahpC-ahpF in vivo does not increase resistanceto H₂O₂ killing. We interpreted these data as evidence that oxyRmutants accumulate both H₂O₂ and organic peroxides, consistentwith the observation in Escherichia coli that oxyR mutants havehigher levels of peroxides than a wild-type strain (9). Thisfact and increased susceptibility to oxidative damage during theearly stages of colony formation when bacterial density is low(17) could have been responsible for the lower aerobic platingefficiency seen for the mutants.

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FIG. 1. Plating efficiency of an oxyR mutant harboring various expression plasmids containing genes involved in oxidative stress response or conditions that affected oxidative stress. In all experiments, a mid-log-phase X. campestris pv. phaseoli oxyR mutant grown in SB was serially diluted and plated on SB plates with or without 10 mM pyruvate. Plating efficiency is defined as the number of cells on SB plates divided by the number of cells on SB plates with pyruvate. Pyr, X. campestris pv. phaseoli oxyR mutant on 10 mM pyruvate SB plates; Mic, the mutant was plated on SB plates and incubated in an anaerobic jar under microaerobic conditions (Oxoid gas generating kit); UFR, X. campestris pv. phaseoli oxyR mutant harboring only pUFR047 (4) expression vector; C, pahpC (15); F, pahpF (ahpF subunit of X. campestris pv. phaseoli [15] in pUFR047); CF, pahpCF (ahpC and ahpF [15] in pUFR047); Kat, pkat (21); Sod, psod (Xanthomonas sod [28] coding region in pUFR047).

Next we qualitatively determined the sensitivity of the log-phase oxyR mutant to killing concentrations of various oxidantsby a killing zone method (15). Essentially, 6 µl of indicatedconcentrations of oxidants applied to 6-mm-diameter paper discswas subsequently placed on lawns of cells. Experiments were performedin triplicate. To ensure reproducibility, only log-phase cellswere used. The killing zones for H₂O₂ (500 mM), menadione (MD)(500 mM), tert butyl hydroperoxide (tBOOH) (500 mM), and cumenehydroperoxide (CuOOH) (500 mM), respectively, were 13, 17, 11,and 16 mm for a wild-type X. campestris pv. phaseoli and 34, 42,13, and 18 mm for an oxyR mutant. The oxyR mutant showed increasedsensitivity to all oxidants tested, with MD and H₂O₂ causing themost severe effects. The high sensitivity of the oxyR mutant toH₂O₂ was expected, but the hypersensitivity to MD implied thatits killing mechanism could partly be mediated via superoxideanion metabolism to H₂O₂ (11, 12). By contrast to an E. colioxyR mutant, the X. campestris pv. phaseoli oxyR mutant had onlya minor increase in sensitivity to organic peroxide killing. Thiscould be due to presence of an additional novel organic peroxide-protectivesystem (ohr) in X. campestris pv. phaseoli that may functionallycompensate for regulatory defects of AhpC (20).

Regulation of oxidant induction of catalase and AhpC by oxyR. We have observed in Xanthomonas that the peroxide-scavenging enzymes, catalase and AhpC, are highly induced by low concentrationsof peroxides and superoxide generators (1, 22). However,the regulator of these responses could not be identified. Experimentswere performed to determine catalase and AhpC levels in responseto low concentrations of oxidants in X. campestris pv. phaseoliand X. campestris pv. phaseoli oxyR. The results are shown inFig. 2. In X. campestris pv. phaseoli, H₂O₂, tBOOH, and MD inducedboth catalase and AhpC to high levels, consistent with previousobservations (1, 16, 21). However, induction of both enzymesby all oxidants tested did not occur in the oxyR mutant. Thisfinding is consistent with a notion that OxyR is acting as a peroxidesensor and a transcription activator of genes for peroxide-scavengingenzymes. These functions are conserved for oxyR in all bacteriathus far studied (28, 31, 33, 34). An increase in thebasal level of AhpC in the oxyR mutant was observed. This couldbe due to OxyR in its reduced form functioning as a repressorof ahpC; thus, in the absence of OxyR, this leads to an increasein ahpC expression (20). The induction of these peroxide-scavengingenzymes by a superoxide generator (MD) was likely to occur viathe breakdown of superoxide anion to H₂O₂ that, in turn, activatedOxyR, not via a superoxide sensor transcription activator proteinsuch as SoxRS (11, 12).

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FIG. 2. Levels of AhpC and catalase activities in response to various oxidants in X. campestris pv. phaseoli (Xp) and an X. campestris pv. phaseoli oxyR mutant (Xp oxyR). Mid-log-phase X. campestris pv. phaseoli or an X. campestris pv. phaseoli oxyR mutant grown in SB was induced with 100 µM H₂O₂ (H) or tBOOH (T) or 20 µM MD (M) for 30 min. Various concentrations of oxidants were chosen to give maximum induction and minimal effects on X. campestris pv. phaseoli growth. Uninduced (U) and induced samples were collected by centrifugation, and lysates were prepared as previously described (21). AhpC levels (A) were determined by Western immunoblotting with an anti-E. coli AhpC (22, 30). Forty micrograms of total protein was loaded into each lane, and immunodetection was performed according to the method of Mongkolsuk et al. (22). At the right of each panel is indicated whether lysates were from X. campestris pv. phaseoli or an X. campestris pv. phaseoli oxyR mutant. Catalase levels were determined spectrophotometrically (21). (B) Closed and open bars represent catalase activities of X. campestris pv. phaseoli and the X. campestris pv. phaseoli oxyR mutant, respectively. Letters above the lanes (A) or below the bars (B) indicate that lysates were prepared from uninduced or oxidant-induced cultures, respectively. Experiments were performed three times, and typical results are shown.

Basal levels of catalase and AhpC in the mutant appeared to be sufficient for normal aerobic growth. The lack of an inductionmechanism for peroxide-scavenging enzymes and the increased oxidantsensitivity of oxyR mutants support the interpretation that up-regulationof these scavenging enzymes is important to bacterial survivalunder stressful conditions. Consistent with this notion, oxyRsuppressor mutants with high levels of AhpC-AhpF and catalaseshave been isolated (10).

oxyR roles in adaptive and cross-protective responses. In Xanthomonas, peroxide and superoxide anions induce protective responses to peroxide killing (23). These responses aremediated by OxyR in E. coli (32), and the oxyR mutant was usedto investigate whether the situation in Xanthomonas was similar.The results of the experiment are shown in Fig. 3. H₂O₂ inducedprotection against H₂O₂ killing in wild-type X. campestris pv.phaseoli. This response was abolished in the oxyR mutant (Fig.3A). In contrast to previous observations with other bacteria(6, 10, 18), MD could induce protection against H₂O₂ andtBOOH killing in both the parental strain and the oxyR mutant(Fig. 3B and C). The data indicate that OxyR is essential to peroxideadaptation and also to the existence of a novel superoxide-inducibleperoxide-protective system independent of OxyR. This novel peroxide-protectivesystem does not depend on up-regulation of the well-known peroxide-scavengingenzymes catalase and AhpR, since their induction by superoxideanions was abolished in the oxyR mutant (Fig. 2).

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FIG. 3. Adaptive and cross-protective responses against peroxide killing in X. campestris pv. phaseoli and an X. campestris pv. phaseoli oxyR mutant. Log-phase uninduced X. campestris pv. phaseoli ( $open circle$ ) and an X. campestris pv. phaseoli oxyR mutant ( $triangle$ ) and oxidant-induced (30-min treatment with either 100 µM H₂O₂ [A] or 50 µM MD [B and C]) X. campestris pv. phaseoli ( $bullet$ ) and X. campestris pv. phaseoli oxyR mutant ( $black-triangle$ ) grown in SB were treated with killing concentrations of either 30 mM H₂O₂ (A and B) or 100 mM tBOOH (C) as previously described (15). At the indicated times, aliquots of cells were removed and washed twice before viable cells were counted (23). Experiments were repeated three times, and representative results are shown.

It is noteworthy that resistance levels to peroxide killing in the MD-induced oxyR strain were similar to those attained bythe similarly induced parental strain, even though the uninducedoxyR mutant was more sensitive than the parental strain to peroxidekilling. Thus, the novel superoxide-inducible peroxide-protectivesystem is likely to play a crucial role in protection againstperoxide killing in X. campestris pv. phaseoli. We believe thissystem differs from the starvation-induced or the general stress-protectivesystems (13). In Xanthomonas, MD does not induce protectionagainst itself or against a nonoxidative stress such as heat killing(23). We are investigating the mechanism of this novel superoxideanion-induced peroxide-protective system.

	ACKNOWLEDGMENTS

We thank G. Storz for her helpful comments and an anti-AhpC antibody and T. Flegel for reviewing the manuscript. This researchwas supported by grants from Chulabhorn Research Institute, ThaiResearch Fund BRG-10-40, and a career development award, RCF 01-40-005,from NASTDA to S.M.

	FOOTNOTES

^* Corresponding author. Mailing address: Laboratory of Biotechnology, Chulabhorn Research Institute, Lak Si, Bangkok 10210,Thailand. Phone: (662) 574-0622. Fax: (662) 574-2027. E-mail:scsmk{at}mucc.mahidol.ac.th.

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	ALL ASM JOURNALS

1.	Chamnongpol, S., P. Vattanaviboon, S. Loprasert, and S. Mongkolsuk. 1995. Atypical oxidative stress regulation of a Xanthomonas oryzae pv. oryzae monofunctional catalase. Can. J. Microbiol. 41:541-547.
2.	Christman, M. F., R. W. Morgan, F. S. Jacobson, and B. N. Ames. 1985. Positive control of a regulon for a defense against oxidative stress and some heat shock proteins in Salmonella typhimurium. Cell 41:753-762[Medline].
3.	Crockford, A. J., C. Behncke, and H. D. Williams. 1996. The adaptation of Rhizobium leguminosarum pv. phaseoli to oxidative stress and its overlap with other environmental stress responses. Microbiology 142:331-336.
4.	DeFeyter, R., C. I. Kado, and D. W. Gabriel. 1990. Small, stable shuttle vectors for use in Xanthomonas. Gene 88:65-72[Medline].
5.	Demple, B. 1991. Regulation of bacterial oxidative stress genes. Annu. Rev. Genet. 25:315-337[Medline].
6.	Dukan, S., and D. Touati. 1996. Hypochlorous acid stress in Escherichia coli: resistance, DNA damage, and comparison with hydrogen peroxide stress. J. Bacteriol. 178:6145-6150[Abstract/Free Full Text].
7.	Farr, S. B., and T. Kogoma. 1991. Oxidative stress responses in Escherichia coli and Salmonella typhimurium. Microbiol. Rev. 55:561-585[Abstract/Free Full Text].
8.	Gonzalez-Flecha, B., and B. D. Demple. 1995. Metabolic sources of hydrogen peroxide in aerobically growing Escherichia coli. J. Biol. Chem. 270:13681-13687[Abstract/Free Full Text].
9.	Gonzalez-Flecha, B., and B. D. Demple. 1997. Homeostatic regulation of intracellular hydrogen peroxide concentration in aerobically growing Escherichia coli. J. Bacteriol. 179:382-388[Abstract/Free Full Text].
10.	Greenberg, J. T., and B. Demple. 1988. Overproduction of superoxide-scavenging enzymes in Escherichia coli suppresses spontaneous mutagenesis and sensitivity to redox-cycling agents in oxyR mutants. EMBO J. 7:2611-2617[Medline].
11.	Greenberg, J. T., and B. Demple. 1989. A global response induced in Escherichia coli by redox-cycling agents overlaps with that induced by peroxide stress. J. Bacteriol. 171:3933-3939[Abstract/Free Full Text].
12.	Hassan, H. M., and I. Fridovich. 1979. Intracellular production of superoxide radical and of hydrogen peroxide by redox active compounds. Arch. Biochem. Biophys. 196:385-395[Medline].
13.	Kolter, R., D. A. Siegele, and A. Tormo. 1993. The stationary phase of bacterial life cycle. Annu. Rev. Microbiol. 48:855-874.
14.	Levine, A., R. Tenhaken, R. Dixon, and C. Lamb. 1994. H₂O₂ from oxidative burst orchestrates the plant hypersensitive disease resistance response. Cell 79:583-593[Medline].
15.	Loprasert, S., S. Atichartpongkun, W. Whangsuk, and S. Mongkolsuk. 1997. Isolation and analysis of the Xanthomonas alkyl hydroperoxide reductase gene and the peroxide sensor regulator genes ahpC and ahpF-oxyR-orfX. J. Bacteriol. 179:3944-3949[Abstract/Free Full Text].
16.	Loprasert, S., P. Vattanaviboon, W. Praituan, S. Chamnongpol, and S. Mongkolsuk. 1996. Regulation of oxidative stress protective enzymes, catalase and superoxide dismutase in Xanthomonas $---$ a review. Gene 179:33-37[Medline].
17.	Ma, M., and J. W. Eaton. 1992. Multicellular oxidant defense in unicellular organisms. Proc. Natl. Acad. Sci. USA 89:7924-7928[Abstract/Free Full Text].
18.	Maciver, I., and E. J. Hansen. 1996. Lack of expression of the global regulator OxyR in Haemophilus influenzae has a profound effect on growth phenotype. Infect. Immun. 64:4618-4629[Abstract].
19.	Martinez, A., and R. Kolter. 1997. Protection of DNA during oxidative stress by the nonspecific DNA binding protein Dps. J. Bacteriol. 179:5188-5194[Abstract/Free Full Text].
20.	Mongkolsuk, S. Unpublished observations.
21.	Mongkolsuk, S., S. Loprasert, P. Vattanaviboon, C. Chanvanichayachai, S. Chamnongpol, and N. Supsamran. 1996. Heterologous growth phase- and temperature-dependent expression and H₂O₂ toxicity protection of a superoxide-inducible monofunctional catalase gene from Xanthomonas oryzae pv. oryzae. J. Bacteriol. 178:3578-3584[Abstract/Free Full Text].
22.	Mongkolsuk, S., S. Loprasert, W. Whangsuk, M. Fuangthong, and S. Atichartpongkun. 1997. Characterization of transcription organization and analysis of unique expression patterns of an alkyl hydroperoxide reductase C gene (ahpC) and the peroxide regulator operon ahpF-oxyR-orfX from Xanthomonas campestris pv. phaseoli. J. Bacteriol. 179:3950-3955[Abstract/Free Full Text].
23.	Mongkolsuk, S., P. Vattanaviboon, and W. Praituan. 1997. Induced adaptive and cross-protection responses against oxidative stress killing in a bacterial phytopathogen. Xanthomonas oryzae pv. oryzae. FEMS Microbiol. Lett. 146:212-217.
24.	Nath, K. A., E. O. Ngo, R. P. Hebbel, A. J. Croatt, B. Zhou, and L. M. Nutter. 1995. Alpha-ketoacids scavenge H₂O₂ in vitro and in vivo and reduced menadione-induced DNA injury and cytotoxicity. Am. J. Physiol. 268:C227-C236[Abstract/Free Full Text].
25.	Niimura, Y., L. B. Poole, and V. Massey. 1995. Amphibacillus xylanus NADH oxidase and Salmonella typhimurium alkyl hydroperoxide reductase flavoprotein components show extremely high scavenging activity for both alkyl hydroperoxide and hydrogen peroxide in the presence of S. typhimurium alkyl hydroperoxide reductase 22 kDa protein component. J. Biol. Chem. 270:25645-25650[Abstract/Free Full Text].
26.	Poole, L. B., and H. R. Ellis. 1996. Flavin-dependent alkyl hydroperoxide reductase from Salmonella typhimurium. 1. Purification and enzymatic activities of overexpressed AhpF and AhpC proteins. Biochemistry 35:56-64[Medline].
27.	Schweizer, H. D. 1993. Small broad-host-range gentamycin resistance cassettes for site-specific insertion and deletion mutagenesis. BioTechniques 15:831-834[Medline].
28.	Smith, S. G., T. J. Wilson, J. M. Dow, and M. J. Daniels. 1996. A gene for superoxide dismutase from Xanthomonas campestris pv. campestris and its expression analysis during bacterial-plant interactions. Mol. Plant-Microbe Interact. 9:584-593[Medline].
29.	Storz, G., and S. Altuvia. 1994. OxyR regulon. Methods Enzymol. 234:217-223[Medline].
30.	Storz, G., F. S. Jacobson, L. A. Tartaglia, R. W. Morgan, L. A. Silveira, and B. N. Ames. 1989. An alkyl hydroperoxide reductase induced by oxidative stress in Salmonella typhimurium and Escherichia coli: genetic characterization and cloning of ahp. J. Bacteriol. 171:2049-2055[Abstract/Free Full Text].
31.	Storz, G., L. A. Tartaglia, and B. N. Ames. 1990. Transcriptional regulator of oxidative stress-inducible genes: direct activation by oxidation. Science 248:189-194[Abstract/Free Full Text].
32.	Tartaglia, L. A., G. Storz, S. B. Farr, and B. N. Ames. 1991. The bacterial adaptation to hydrogen peroxide stress, p. 155-169. In H. Sies (ed.), Oxidative stress, oxidants and antioxidant. Academic Press, New York, N.Y.
33.	Tolendano, M. B., I. Kullik, F. Trinh, P. T. Baird, T. D. Scheider, and G. Storz. 1994. Redox-dependent shift of OxyR-DNA contacts along an extended DNA binding site: a mechanism for differential promoter selection. Cell 78:897-909[Medline].
34.	Zhang, Y., S. Dhandayuthapani, and V. Deretic. 1996. Molecular basis for the exquisite sensitivity of Mycobacterium tuberculosis to isoniazid. Proc. Natl. Acad. Sci. USA 93:13212-13216[Abstract/Free Full Text].