Involvement of Carbon Source and Acetyl Phosphate in the External-pH-Dependent Expression of Porin Genes in Escherichia coli

doi:10.1128/JB.182.1.198-202.2000

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Journal of Bacteriology, January 2000, p. 198-202, Vol. 182, No. 1
0021-9193/0/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Involvement of Carbon Source and Acetyl Phosphate in the External-pH-Dependent Expression of Porin Genes in Escherichia coli

Martine Heyde, Patrick Laloi,^* and Raymond Portalier

Unité de Microbiologie et Génétique, UMR CNRS 5577, Université Lyon I, F-69622 Villeurbanne Cedex, France

Received 6 July 1999/Accepted 14 October 1999

	ABSTRACT

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The porin composition of the Escherichia coli cell envelope was analyzed during growth at different external pHs (pHo) asa function of the acetyl phosphate (AcP) level ( $Delta$ ackA pta or ackAmutant, pyruvate or glucose as the carbon source) in the presenceor absence of EnvZ. Our results indicate that the AcP level isinfluenced by the pHo, leading to modulation of the amount ofOmpR-P and subsequent pHo-dependent expression of ompF and ompC.We also propose the existence of a specific signal, independentof EnvZ and AcP, leading to OmpR phosphorylation in response topyruvate.

	TEXT

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The outer membrane of Escherichia coli contains two porin proteins, OmpF and OmpC, that control the permeability of smallhydrophilic molecules across the outer membrane. The total amountof OmpF and OmpC proteins is fairly constant, but their relativelevel varies with environmental factors, including osmolarityand external pH (pHo) (14, 15). Medium with high osmolarityor low pH favors the synthesis of OmpC, and medium with low osmolarity(LO) or high pH increases the OmpF level and reduces the OmpClevel (6, 7, 19, 20). Osmoregulation of the ompF andompC genes is mediated at the transcriptional level by the EnvZ-OmpRtwo-component regulatory system (2). EnvZ is the osmosensorable to sense changes in external osmolarity. It undergoes autophosphorylationat His 274 and transfers the phosphate group to Asp55 of OmpR.EnvZ also acts as an OmpR phosphate (OmpR-P) phosphatase (8).OmpR-P is a transcriptional effector of both porin genes (14).The level of OmpR-P relies on the ratio of kinase to phosphataseEnvZ activity. In vivo, the level of OmpR-P increases as osmolarityis raised (3, 16). The current genetic model for porin regulationpredicts that a low level of OmpR-P stimulates the transcriptionof the ompF gene through binding to a high-affinity site and ahigh level of OmpR-P represses ompF through binding to a low-affinitysite (5). ompC transcription is stimulated by OmpR-P throughthe binding to a low-affinity site (14). The high degree ofhomology between sensors and regulator proteins of two-componentregulatory systems favors the possibility of phosphorylation ofa regulator protein by a noncognate histidine kinase but alsoby low-molecular-weight phosphodonor molecules (21). Such cross-regulationwas demonstrated to occur in vivo between CreC and PhoB (in theabsence of PhoR), EnvZ and PhoB (in the absence of OmpR), andPhoB and acetyl phosphate (AcP) (in the absence of PhoR and CreC)(10, 23). EnvZ-independent mechanisms can also lead to OmpRphosphorylation and to osmolarity-dependent ompF expression inan envZ null mutant (3). In vitro, OmpR was demonstrated tobe phosphorylated by the noncognate histidine kinase CheA (9)and by low-molecular-weight phosphate donors such as AcP (5).In vivo experiments show that ompF transcription is dependentupon AcP synthesis only when EnvZ is absent (8, 11; S.-K.Kim and B. Wanner, personal communication). However, in the presenceof EnvZ, the OmpC level has been demonstrated to increase as AcPaccumulates (12, 18). All of these results suggest that cross-regulationwould occur in vivo between OmpR and other kinase-independent,AcP-dependentmechanisms.

The role of EnvZ and OmpR-P in pHo regulation of porin expression has not yet been elucidated. Preliminary results suggesta role for EnvZ in ompF and ompC pHo regulation (19). However,in the absence of EnvZ, ompF expression is still pHo dependent,being higher during growth at low pHo than during growth at highpHo (6).

In this study, ompF and ompC transcription was analyzed under slightly acidic (pHo 6) or alkaline (pHo 7.8) growth conditionswith glucose or pyruvate as the carbon source and in the presenceof a pta or ackAmutation.

Bacterial strains, media, and growth conditions. All of the strains used are derivatives of E. coli K-12 and are listed in Table 1. P1 vir lysates and transduction experimentswere performed as previously described by Miller (13). Selectionand identification are indicated in Table 1.

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TABLE 1. E. coli strains used in this study

LO minimal medium was used because, as previously shown by Thomas and Booth (19), we observed that ompF transcription dependson pHo only during growth in LO minimal medium. The LO minimalmedium used in this study is a derivative of both the S mediumdescribed by Thomas and Booth (19) and the A medium describedby Miller (13). It contained 49.2 mM KH₂PO₄-K₂HPO₄, 1 mM trisodiumcitrate, 0.4 mM MgSO₄, 7.6 mM (NH₄)₂SO₄, and 3 µM thiamine hydrochloride.It was adjusted to pH 6 or 7.8 by mixing appropriate volumes ofphosphate solutions (43 mM KH₂PO₄ and 6.2 mM K₂HPO₄ for pH 6 and4.2 mM KH₂PO₄ and 45 mM K₂HPO₄ for pH 7.8). At pH 6, 40 mM NaClwas added to compensate for the change in medium osmolarity causedby the different balance of potassium and phosphate ions. Identicalresults were obtained whether 40 mM NaCl was added or not in themedium. Minimal media were supplemented with 0.04% glucose or0.1% pyruvate, which was the carbon source. These sugar concentrationsallow identical growth conditions with a doubling time of about2 h and a concentration of about 5 × 10⁸ cells ml¹ in stationary growth phase. Overnight subcultures, grown in LBbroth (13) at 30°C, were used to inoculate LO medium adjustedto different pH values. These cultures were incubated at 30°Cuntil stationary phase was reached. At this point, the differentbuffered cultures were diluted with the same fresh medium to anoptical density at 600 nm of 0.02. These new cultures were aeratedand incubated at 30°C until they reached an optical density at600 nm of 0.2 to 0.3. Until this cell density was reached, thepH of the growth medium remainedconstant.

Effect of carbon source on ompF and ompC pHo regulation. Strains GPH8252 and GPH8259, carrying the ompF-lacZ or the ompC-lacZ operon fusion, respectively, were grown in LO minimalmedium adjusted to pH 6 or 7.8 with pyruvate or glucose as thecarbon source. $beta$ -Galactosidase expression in toluene-treated cellswas assayed (Fig. 1A and C and 2A and C; parent strains) as describedby Miller (13). One unit of enzyme activity was defined as theamount of enzyme which hydrolyzed 1 nmol of substrate per minwith 3 mM o-nitrophenyl- $beta$ -D-galactopyranoside as the substrate.In the parent EnvZ⁺ strain, with pyruvate as the carbon source, ompF transcriptionwas induced 1.7-fold during growth at pHo 7.8 compared with growthat pHo 6 (Fig. 1A, parent strain) but this induction was not apparentwith glucose (Fig. 1C, parent strain). Figure 2A and C show thatin the parent EnvZ⁺ strain with pyruvate or glucose, ompC was induced 1.5- and 2-fold,respectively, during growth at pHo 6 compared with growth at pHo7.8. ompC induction during growth at pHo 6 with glucose or pyruvateindicates that the OmpR-P level would be higher at pHo 6 thanat pHo 7.8. Identical levels of ompF expression at both pHos inglucose are not inconsistent with different OmpR-P levels. Weassume that at pHo 6, the OmpR-P level would lead to ompF repressionand at pHo 7.8, a lower OmpR-P level would lead to ompF activation,resulting in the same ompF expression at both pHos.

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FIG. 1. Expression of ompF at pHos 6 and 7.8 in parental and mutant (ackA pta or ackA) strains in the presence or absence of EnvZ. Strains were grown in LO medium with pyruvate or glucose as the carbon source. Panels: A and C, GPH8252 parent strain, GPH8255 $Delta$ (ackA pta) strain, and GPH8257 ackA200 strain; B and D, GPH8268 parent strain, GPH8273 $Delta$ (ackA pta) strain, and GPH8274 ackA200 strain. The data are mean values ± standard deviations from three independent experiments.

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FIG. 2. Expression of ompC at pHos 6 and 7.8 in parental and mutant (ackA pta or ackA) strains in the presence or absence of EnvZ. Strains were grown in LO medium with pyruvate or glucose as the carbon source. Panels: A and C, GPH8259 parent strain, GPH8282 $Delta$ (ackA pta) strain, and GPH8280 ackA200 strain; B and D, GPH8285 parent strain, GPH8293 $Delta$ (ackA pta) strain, and GPH8291 ackA200 strain. The data are mean values ± standard deviations from two to four independent experiments.

In the absence of EnvZ, with pyruvate, ompF expression (strain GPH8268) was slightly decreased but still induced at pHo 7.8,as in the EnvZ⁺ strain (compare Fig. 1B to A, parent strains). With glucose,the absence of EnvZ led to a decrease in ompF expression mainlyat pHo 7.8. Consequently, ompF expression became higher at pHo6 than at pHo 7.8 (compare Fig. 1D to C, parent strains). Theseresults indicate that in the absence of EnvZ, ompF expressionis still influenced by the pHo and the carbon source. With pyruvateor glucose, ompC was still expressed, albeit at a lower levelthan in the EnvZ⁺ strain (compare Fig. 2B to A and D to C, parent strains). Thisresidual expression was more important in pyruvate than in glucoseand was pHo dependent. These data show that in the absence ofEnvZ, ompC expression is also influenced by both the pHo and thecarbon source. So, without EnvZ, OmpR would be phosphorylatedby an EnvZ-independent mechanism and OmpR-P would accumulate becauseof the lack of EnvZ phosphatase activity. ompC expression levelsindicate that the OmpR-P level would be higher at low than athigh pHo and in pyruvate than in glucose. In pyruvate, OmpR phosphorylationwould allow OmpR-P levels high enough to repress ompF and stronglyactivate ompC. In glucose, compared to pyruvate, OmpR phosphorylationwould be weaker and the OmpR-P accumulation would allow ompF activationand lower ompCactivation.

From our results collected with and without EnvZ, we can deduce that both EnvZ activities would not be responsible for thepHo regulation and the carbon source-dependent activation of poringenes. In addition to the kinase activity of EnvZ, OmpR phosphorylationwould require pHo- and carbon source-dependentmechanisms.

Role of noncognate histidine kinase in ompF pHo regulation. In an EnvZ-deficient strain, ompF transcription remained pHo dependent (Fig. 1B and D, parent strains). Since CheA was demonstratedto phosphorylate OmpR in vitro (9), we investigated the physiologicalrelevance of cross-regulation between noncognate kinases (PhoR,CheA, and CreC) and OmpR when EnvZ is absent and the role thatthis cross-regulation may play in the pHo regulation of ompF.The $beta$ -galactosidase activities of isogenic phoR20, $Delta$ (cheA-cheZ),and creB creC derivatives of an envZ22 strain, carrying an ompF-lacZoperon fusion, were assayed during growth in LB broth adjustedto different pHs and compared with the activities in the envZ22mutant. ompF expression was found not to be significantly modifiedin the presence of these mutations (data not shown). These resultsindicate that in an EnvZ-deficient strain, in vivo cross-regulationbetween noncognate histidine kinases (PhoR, CheA, and CreC) andOmpR does not play any physiological role in ompF pHo-dependenttranscription.

Role of AcP in ompF and ompC pHo regulation. AcP is synthesized from acetyl coenzyme A and P_i with the release of free coenzyme A by phosphotransacetylase. AcP and ADPare then converted to acetate and ATP by acetate kinase. An ackAmutant is expected to accumulate AcP because its breakdown isblocked. An ackA pta mutant is expected to display a low AcP levelbecause its synthesis no longer occurs and the phosphotransacetylase-acetatekinase pathway cannot be inverted (10). Use of pyruvate as acarbon source was described to lead to a fourfold higher AcP levelthan the use of glucose during the exponential growth phase (12).To determine the role of AcP in OmpR activation, we analyzed theexpression of ompF-lacZ and ompC-lacZ operon fusions with glucoseor pyruvate as the carbon source and in the presence of an ackApta or ackA mutation. $beta$ -Galactosidase activities were assayedduring the growth of isogenic strains (Table 1) in LO minimalmedium adjusted to pH 6 or 7.8 (Fig. 1A and C and 2A andC).

In the presence of EnvZ, with a low AcP level, and in pyruvate or glucose, ompC was not significantly induced at pHo 6, leadingto pHo-independent expression (Fig. 2A and C, ackA pta strain).This result indicates that in the presence of EnvZ, AcP wouldcontribute to OmpR phosphorylation during growth at pHo 6. Withoutthis contribution, OmpR-P levels would be the same at both pHos.Unexpectedly, the 1.7-fold induction of ompF during growth withpyruvate at pHo 7.8 compared to pHo 6 was not significantly modifiedwhen the AcP level was decreased (Fig. 1A, ackA pta strain). WhenAcP was high, whatever the carbon source, ompC expression wasalmost the same at both pHos, meaning that OmpR-P levels werethe same at both pHos (Fig. 2A and C, ackA strain). ompF expressionwas not modified, whatever the pHo, by a high AcP level (Fig.1A and C, compare parent and ackAstrains).

We next tested if OmpR activation requires AcP in the absence of EnvZ. We assayed $beta$ -galactosidase activities of isogenic envZ22,envZ22 ackA pta, and envZ22 ackA derivatives carrying an ompF-lacZor ompC-lacZ operon fusion (Table 1) during growth in LO mediumadjusted to pHo 6 or 7.8 and supplemented with pyruvate or glucoseas the carbon source (Fig. 1B and D and 2B and D). In the absenceof EnvZ and AcP, ompF was no longer expressed in glucose (Fig.1D, ackA pta strain) but was still expressed in pyruvate althoughat a lower level than in the presence of AcP (Fig. 1B, compareackA pta to parent strains). This expression was slightly pHodependent. These results indicate that in the absence of EnvZ,ompF transcription is controlled by an AcP-dependent mechanism.Moreover, ompF residual expression during growth in pyruvate evidencesapparently pyruvate-dependent activation of ompF (Fig. 1B, ackApta strain). This mechanism, independently of EnvZ and AcP, wouldallow OmpR phosphorylation only during growth in pyruvate. Pyruvate-dependentactivation of the phosphate regulon was previously reported byWanner and Wilmes-Riesenberg (22). In the absence of the P_isensor (PhoR) and its homolog CreC, pyruvate led to the activationof alkaline phosphatase synthesis. When the AcP level was high,ompF expression increased up to the parental level and becamepHo independent (Fig. 1B and D, ackA strain). In this strain,lacking EnvZ phosphatase activity, the OmpR-P formed by the AcP-dependentmechanism accumulates to a level corresponding to ompF activation(8).

In the absence of EnvZ and AcP, ompC was not expressed (Fig. 2B and D, ackA pta strain). This result indicates that whateverthe carbon source, AcP is responsible for ompC expression whenEnvZ is absent. We assume that the pyruvate-dependent OmpR phosphorylationevidenced with ompF would yield an OmpR-P level too low to activateompC. With an increased AcP level, ompC expression was increased,with slightly higher expression at pHo 7.8 than at pHo 6 (Fig.2B and D, ackA strain). These results correlate well with theresistance of the envZ22 ackA pta derivative (strain GPH8273)and the sensitivity of the envZ22 ackA derivative (strain GPH8274)to bacteriophage MeI, which uses OmpC as areceptor.

Unexpectedly, growth of an EnvZ-deficient strain with pyruvate and a high level of AcP was associated with high expressionof both the ompF and ompC genes (Fig. 1B and 2B, ackA strains).Such a phenotype was previously described by McCleary and Stock(12) for an envZ⁺ pta strain during growth with sodium acetate and by Russo etal. (17) for a mutant with an OmpR protein unable to repressompF.

In the absence of EnvZ, pHo-dependent expression of ompF and ompC was clearly demonstrated to depend upon the AcP amount,which would be higher at pHo 6 than at pHo 7.8. To obtain directevidence of pHo modulation of the AcP level, we tried to directlymeasure AcP by enzymatic methods during growth at different pHosbut the concentration of this compound in cells proved to be toolow under our conditions to be quantitativelyassayed.

Conclusion. In the absence of EnvZ, our results show that ompF and ompC expression is influenced by pHo and AcP. A higher OmpR-P levelat low pHo than at high pHo might be responsible for this regulation.We propose that with or without EnvZ, the AcP amount is influencedby pHo, leading to modulation of the OmpR-P level and, consequently,pHo-dependent expression of ompF and ompC. According to our resultsobtained with and without EnvZ, both EnvZ activities are not involvedin pHo regulation of the porin regulon. We do not know whetherOmpR is phosphorylated directly by AcP or indirectly through anoncognate kinase, as suggested by Kim et al. (10). AcP wasalso shown to be responsible for ompF and ompC osmoregulationin the absence of EnvZ (11; Kim and Wanner, personal communication).Our study also suggests that the OmpR-P level is higher duringgrowth in pyruvate than during growth in glucose, when EnvZ isabsent. Indeed, under our assay conditions, ompF and ompC expressiondepends on the nature of the carbon source. Similar results weredescribed by Kim et al. (10). The link between the carbon sourceand the expression of ompF and ompC might simply be explainedby the modulation of the AcP level as a function of the carbonsource, this hypothesis cannot account for all of our results.Indeed, ompF residual expression, in the absence of AcP and EnvZ,was still higher in pyruvate than in glucose (compare Fig. 1Bto D, ackA pta strain), so it may be that a specific signal leadsto OmpR phosphorylation in response to pyruvate. This pyruvate-dependentsignal would not depend on EnvZ and AcP. Pyruvate-dependent activationof the phosphate (22) and porin regulons should involve differentmechanisms. Indeed, AcP is required for pyruvate-dependent activationof the phosphate regulon but not for pyruvate-dependent activationof the porin regulon. This regulon constitutes another two-componentregulatory system affected by a control linked to the use of pyruvateas a carbon source. This control might be of more generalinterest.

	ACKNOWLEDGMENTS

We thank S.-K. Kim and B. Wanner for unpublished information; M. Berlyn, S. Garrett, D. E. Koshland, and B. Wanner for generousgift of strains; and B. Dequatre for excellent technicalassistance.

This work was supported by grants from the Centre National de la Recherche Scientifique (UMR5577) and the University ClaudeBernard LyonI.

	FOOTNOTES

^* Corresponding author. Mailing address: Unité de Microbiologie et Génétique, UMR CNRS 5577, Bâtiment 405, Université LyonI, F-69622 Villeurbanne Cedex, France. Phone: 33 472 431 621.Fax: 33 472 432 686. E-mail: plaloi{at}biomserv.univ-lyon1.fr.

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1.	Berlyn, M. K. 1998. Linkage map of Escherichia coli K-12, edition 10: the traditional map. Microbiol. Mol. Biol. Rev. 62:814-984[Abstract/Free Full Text].
2.	Forst, S., and D. Roberts. 1994. Signal transduction by the EnvZ-OmpR phosphotransfer system in bacteria. Res. Microbiol. 145:363-373[Medline].
3.	Forst, S., J. Delgado, A. Rampersaud, and M. Inouye. 1990. In vivo phosphorylation of OmpR, the transcription activator of the ompF and ompC genes in Escherichia coli. J. Bacteriol. 172:3473-3477[Abstract/Free Full Text].
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