FabF Is Required for Piezoregulation of cis-Vaccenic Acid Levels and Piezophilic Growth of the Deep-Sea Bacterium Photobacterium profundum Strain SS9

doi:10.1128/JB.182.5.1264-1271.2000

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Journal of Bacteriology, March 2000, p. 1264-1271, Vol. 182, No. 5
0021-9193/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

FabF Is Required for Piezoregulation of cis-Vaccenic Acid Levels and Piezophilic Growth of the Deep-Sea Bacterium Photobacterium profundum Strain SS9

Eric E. Allen and Douglas H. Bartlett^*

Center for Marine Biotechnology and Biomedicine, Marine Biology Research Division, Scripps Institution of Oceanography, University of California, San Diego, La Jolla, California 92093-0202

Received 28 September 1999/Accepted 1 December 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

To more fully explore the role of unsaturated fatty acids in high-pressure, low-temperature growth, the fabF gene from thepsychrotolerant, piezophilic deep-sea bacterium Photobacteriumprofundum strain SS9 was characterized and its role and regulationwere examined. An SS9 strain harboring a disruption in the fabFgene (strain EA40) displayed growth impairment at elevated hydrostaticpressure concomitant with diminished cis-vaccenic acid (18:1)production. However, growth ability at elevated pressure couldbe restored to wild-type levels by the addition of exogenous 18:1to the growth medium. Transcript analysis did not indicate thatthe SS9 fabF gene is transcriptionally regulated, suggesting thatthe elevated 18:1 levels produced in response to pressure increaseresult from posttranscriptional changes. Unlike many pressure-adaptedbacterial species such as SS9, the mesophile Escherichia colidid not regulate its fatty acid composition in an adaptive mannerin response to changes in hydrostatic pressure. Moreover, an E.coli fabF strain was as susceptible to elevated pressure as wild-typecells. It is proposed that the SS9 fabF product, $beta$ -ketoacyl-acylcarrier protein synthase II has evolved novel pressure-responsivecharacteristics which facilitate SS9 growth at highpressure.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Increased hydrostatic pressure and reduced temperature elicit similar physical effects on the phase and fluidity propertiesof membrane lipids. As growth temperature is lowered or growthpressure is elevated, biological membranes undergo a reversiblechange from a fluid disordered state to a nonfluid ordered state(22, 29). Such changes would seem particularly problematicfor life in deep ocean environments. Many poikilothermic organismsrespond to decreased temperature and/or increased hydrostaticpressure by altering their membrane lipid composition, apparentlyto tailor the membrane with physical properties suited to prevailingenvironmental conditions. Such changes may include increases infatty acyl chain unsaturation, decreases in mean chain length,increased methyl branching, cis/trans isomerization of unsaturatedfatty acid double bonds, increases in the ratio of anteiso branchingrelative to iso branching, acyl chain shuffling between the phospholipidsn-1 and sn-2 positions, or phospholipid headgroup compositionchanges (22, 25, 36, 39). Among these changes, the mostcommon change observed among deep-sea bacteria involves the incorporationinto membrane phospholipids of increased proportions of unsaturatedfatty acids (UFAs) (1, 11, 12, 47). UFAs adopt a moreexpanded conformation, pack less compactly, and possess lowermelting temperatures than their saturated counterparts, allowingfor their less orderly alignment within membrane phospholipids(22). This response presumably functions to offset the membranegelling effects of increased pressure or decreased temperature,thereby maintaining biological membranes in a fluidity or phaseoptimized for growth. In addition to producing increased amountsof monounsaturated fatty acids (MUFAs) such as palmitoleic acid(16:1n-9) and cis-vaccenic acid (18:1n-11), many deep-sea bacteriaalso produce substantial quantities of omega-3 polyunsaturatedfatty acids (PUFAs) at high pressure (1, 12, 47, 48).

The way in which a bacterial species modulates its membrane fatty acid unsaturation depends on its method of UFA synthesisand involves either an aerobic or anaerobic mechanism. In gram-positivebacteria and cyanobacteria, a double bond is introduced into apreexisting fatty acid chain by means of an oxygen-dependent desaturasesystem (13, 44). In contrast, gram-negative bacteria employan anaerobic pathway, whereby at a discrete point in the elongationcycle of fatty acid biosynthesis a cis double bond is introduced(38). Some bacteria utilize both the anaerobic and aerobic desaturationpathways (34).

In Escherichia coli, where the mechanisms of anaerobic UFA synthesis have been well characterized, the response to temperaturedownshift entails the restructuring of membrane fatty acid compositionby increasing the amount of 18:1 and decreasing the amount ofpalmitic acid (16:0) incorporated into membrane phospholipids(33). This regulation is an intrinsic property of the fattyacid biosynthetic enzyme $beta$ -ketoacyl-ACP (acyl carrier protein)synthase II (KAS II), product of the fabF gene (10, 14, 17).E. coli KAS II is one of three isozymes that catalyze the elongationof fatty acyl chains. Specifically, KAS II catalyzes the elongationof palmitoleoyl-ACP (16:1) to cis-vaccenoyl-ACP (18:1) in UFAsynthesis. Neither mRNA nor protein synthesis is required forincreased 18:1 production at reduced temperature, indicating thatthermal modulation of fatty acid production is controlled at thelevel of KAS II activity (17). Indeed, the elongation activityof KAS II is temperature dependent, exhibiting decreased K_m forpalmitoleoyl-ACP and increased relative V_max at reduced temperatures(16, 18). E. coli fabF mutants possess a deficiency in 18:1synthesis as well as a loss of 18:1 thermal regulation (19).

Because of the critical role of fabF (KAS II) in thermal modulation of UFA production in E. coli, we predicted that a similarrole exists for KAS II in the deep-sea bacterium Photobacteriumprofundum strain SS9 and furthermore that SS9 KAS II is requiredfor 18:1 piezoregulation and piezoadaptation. Such propertiescould distinguish the SS9 KAS II enzyme from its homologue inbacteria which have not evolved adaptations for substantiallyelevated pressures. Consistent with this hypothesis, recent studiesin our lab using the fatty acid biosynthesis inhibitor ceruleninand mutants altered in the abundance of various UFAs indicatedthat MUFAs but not PUFAs are required for high-pressure and low-temperatureadaptation in P. profundum strain SS9 (1). Here we report thecloning of the SS9 fabF gene, the engineering of an SS9 mutantharboring a disruption in fabF, and the growth characteristicsand fatty acid analysis of this mutant. In addition, an E. colifabF mutant and parental strain were compared with respect tofatty acid composition and growth ability as a function of pressureand temperature. Our results indicate that SS9 fabF has evolvednovel characteristics critical to pressure sensing and high-pressureadaptation.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Strains and growth conditions. All bacterial strains and plasmids used in this study are listed in Table 1. P. profundum strains were routinely culturedat 15°C, 1 atm (=0.101 MPa) in 2216 marine medium (28 g/liter;Difco Laboratories, Detroit, Mich.). All temperature experiments(15 and 4°C) were conducted aerobically in 2216 marine mediumfor P. profundum strains unless otherwise indicated. E. coli strainsSJ16 and MR86 were graciously provided by John E. Cronan, Jr.E. coli strains were routinely cultured in Luria-Bertani (LB)media (30). For solid media, agar (Difco Laboratories) was addedat 17 g/liter. The antibiotics kanamycin (50 µg/ml for E. coli;200 µg/ml for P. profundum strains), streptomycin (50 µg/ml forE. coli; 150 µg/ml for P. profundum strains), rifampin (100 µg/ml),and tetracycline (12 µg/ml) were added to the media when required.All antibiotics were obtained from Sigma Chemical Co. (St. Louis,Mo.). Exogenous supplementation of marine media with fatty acids(i.e., Na⁺ salts) is not possible due to insolubility problems resultingfrom the presence of a high concentration of divalent cations.Tween compounds, however, are highly soluble in marine media andhave been used for exogenous supplementations (1). Oleic acid(18:1) in the form of Tween 80 (polyoxyethylenesorbitan monooleate;Sigma) was added at a final concentration of 0.025% (vol/vol).

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TABLE 1. Strains and plasmids used in this study

High-pressure growth studies. High-pressure cultivation of P. profundum strains for growth studies or fatty acid analysis were conducted as previously described(1). Cultivation of E. coli strains at elevated pressures wassimilarly performed. Each E. coli culture was grown to stationaryphase in LB medium at 1 atm. Stationary-phase cultures were diluted1/400 into LB medium buffered with HEPES (100 mM, pH 7.5; Sigma)containing 22 mM glucose (Sigma). The diluted culture was usedto fill 4.5- or 15-ml polyethylene transfer pipettes (Samco, SanFernando, Calif.). Pipettes were filled completely and then heatsealed with a hand-held heat sealing clamp (Harwil, Oxnard, Calif.).Cells were incubated at 0.1 or 30 MPa (1 or 300 atm, respectively)of hydrostatic pressure at 37°C (unless otherwise stated) in stainlesssteel pressure vessels equipped with quick-connect fittings forrapid decompression and recompression as described by Yayanosand Van Boxtel (50).

DNA sequencing and analysis. Double-stranded DNA sequencing reactions were performed using a Taq DyeDeoxy terminator cycle sequencing kit (Applied BiosystemsInc., Foster City, Calif.) and run on an Applied Biosystems 373ADNA sequencer. Global similarity searches were performed usingthe BLAST network service (2). Multiple alignments were performedusing ClustalW (23) in conjunction with GeneDoc software (35).

fabF insertional inactivation mutagenesis. An internal fragment of the SS9 fabF gene was initially PCR amplified from P. profundum strain DB110 genomic DNA, using primersfabF1 5'-GTGTCCAAGCGTCGTGTAGTTGT-3' and fabF4 5'-GCGTGTTCGTACTCTTCAAG-3'.These primers were created by analysis of conserved regions fromalignment of the E. coli and Vibrio harveyi fabF gene sequencesin GenBank. The resultant 740-bp PCR product was cloned into pCR2.1(Invitrogen, Carlsbad, Calif.), generating pEA39, and sequencedusing M13R and T7 primers to confirm the identity of the product.The PCR product was then subcloned into the mobilizable suicideplasmid pMUT100 (Kan^r) (7) as an EcoRI fragment yielding pEA40. Bacterial conjugationswere used to transfer plasmid pEA40 from E. coli into P. profundumstrain DB110 as described by Chi and Bartlett (8). Kan^r exconjugants arose from integration of plasmid pMUT100 into thechromosome of P. profundum strain DB110 in a single crossoverevent giving rise to two deleted copies of the gene, one copywith a 5' deletion and the other with a 3' deletion. These experimentsyielded P. profundum strain EA40 containing a disruption in thefabF gene and was confirmed by Southern blot analysis (40).Genomic DNA from P. profundum strains EA40 and DB110 was digestedwith restriction enzymes BglII, HindII, HpaI, or PstI and probedusing the fabF internal fragment harbored on pEA39 labeled with[ $alpha$ -³²P]dCTP by random priming (Life Technologies, Gaithersburg, Md.).

Isolation of the SS9 fabF gene. A P. profundum SS9 genomic library (6) was screened using an internal fragment of SS9 fabF in order to identify recombinantlibrary clones harboring the SS9 fabF gene. Colony hybridizationswere performed according to standard protocols (40). PlasmidDNA was isolated from positively hybridizing clones and subsequentlysequenced. The SS9 fabF gene was PCR amplified from strain DB110genomic DNA, using primers fabF-F(5'-CTAGTAATGGCTCTTGAAGAAG-3')and fabF-R(5'-AATTCTTCACGGCAAAATTA-3'). The PCR product was clonedinto pCR2.1 and subsequently subcloned into pKT231 (3) as aHindIII-XhoI fragment, yieldingpEA44.

Fatty acid analyses. Extraction and analysis of fatty acid methyl ester preparations via combined gas chromatography-mass spectrometry were performedas previously described (1). Compounds were identified by comparisonof retention times with those of known standards (Sigma) as wellas sample mass spectra data compared to the Hewlett-Packard G1034CMS ChemStation software NBS75K library containing mass spectradata of 75,000 known compounds. Fatty acids are denoted as numberof carbon atoms:number of double bonds. Inner and outer membraneseparation and fatty acid analysis on P. profundum strain EA40grown in the presence of 0.025% Tween 80 at 28 MPa (9°C) wereperformed in order to show that the 18:1 from Tween 80 was incorporatedinto membrane phospholipids as previously described (1).

RNA isolation and Northern analyses. Total RNA was extracted from P. profundum strains grown at various temperatures and pressures using the RNAzol B method (Tel-Test,Inc., Friendswood, Tex.). Equivalent amounts of RNA (10 µg) wereelectrophoresed through 1.2% formaldehyde agarose, blotted ontoa Magnacharge nylon transfer membrane (MSI, Westboro, Mass.),and subjected to Northern analysis using the PCR product containedwithin pEA39 as the hybridization probe labeled with [ $alpha$ -³²P]dCTP by random priming (Life Technologies). Hybridizations wereconducted using QuikHyb hybridization solution (Stratagene, LaJolla, Calif.) at a temperature of 64°C.

Nucleotide sequence accession number. The sequence of P. profundum strain SS9 fabF, along with the partial sequences of acpP and pabC, is deposited in the GenBankdatabase under accession no. AF188707.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Isolation and analysis of the P. profundum strain SS9 fabF gene. Using PCR primers designed from conserved portions of known fabF sequences (E. coli and V. harveyi), a 740-bp product wasamplified from P. profundum strain DB110 genomic DNA and subclonedinto pCR2.1 (Invitrogen) to generate pEA39, and its nucleotidesequence was determined. Global similarity searches using gapped-BLAST(2) indicated that the insert DNA present on pEA39 containedan open reading frame with a high degree of similarity to FabFproteins from V. harveyi (E value of 5E-107) and from E. coli(E value of 2E-101). The entire SS9 fabF gene was then isolatedfollowing colony blot hybridization of a SS9 genomic library (6),using the insert on pEA39 as a hybridization probe. From all ofthe three positively hybridizing clones obtained in this way,sequence analysis indicated the presence of fabF DNA. One of thethree plasmids chosen for further study, pEA401, contained a 7.5-kbinsert. Sequence analysis of pEA401 revealed a gene organizationflanking fabF identical to that present in E. coli, V. harveyi,and Pseudomonas aeruginosa (27, 31, 41); in particular itcontained the 3' end of acpP, followed by fabF and pabC. Furthersequence downstream of SS9 pabC contained on pEA401 was notobtained.

The SS9 fabF gene was found to display a high degree of similarity and identity to both the E. coli and V. harveyi fabF genesat both nucleotide and deduced amino acid sequence levels. Atthe DNA level, the SS9 fabF sequence was 73 and 69% identicalto fabF sequences of V. harveyi and E. coli, respectively. Inaddition, possible Rho-independent terminator sequences are presentwithin the SS9 acpP-fabF intergenic region (ending 70 bp upstreamof the fabF GTG start) and the fabF-pabC intergenic region (ending67 bp upstream of the pabC ATG start). These structures are similarin location to putative terminators identified upstream of fabFin V. harveyi, P. aeruginosa, and E. coli and downstream of fabFin V. harveyi and P. aeruginosa. The predicted amino acid sequenceof SS9 KAS II (FabF) was 79 (90) and 76% (88%) identical (similar)to KAS II sequences of V. harveyi and E. coli, respectively. Nodramatic differences in pI value or amino acid composition wereobserved between the KAS II enzymesanalyzed.

fabF transcript analysis. To identify and determine the sizes of SS9 fabF transcripts, Northern blotting was performed (Fig. 1). Northern blot analysisof strain DB110 revealed two fabF probe-specific transcripts,one major transcript at approximately 1.9 kb and one minor transcriptof approximately 1.5 kb. Zhang and Cronan (52) examined theexpression of the E. coli fabF gene and identified two transcriptsidentical in size to those produced by SS9. Their analysis revealedthat the 1.5-kb transcript was a fabF-specific mRNA, whereas the1.9-kb transcript was most likely the product of cotranscriptionof fabF and the upstream acpP gene. In SS9, neither of these transcriptsexhibited differential abundance at decreased temperature or elevatedpressure.

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FIG. 1. Northern analysis of fabF expression in P. profundum strains EA40 (fabF) and DB110 (wild type). Cells were grown to late exponential phase for total RNA isolation and probed using internal fragment of SS9 fabF as described in Materials and Methods. Lanes: 1, EA40 at 4°C; 2, EA40 at 15°C; 3, DB110 at 4°C; 4, DB110 at 15°C; 5, DB110 at 28 MPa (9°C); 6, DB110 at 0.1 MPa (9°C).

Isolation of an SS9 fabF mutant. To explore the in vivo regulation and function of KAS II in SS9, a fabF mutant was constructed. The isolation of an SS9 fabFmutant followed the introduction of an internal fragment of theSS9 fabF gene, harbored on pEA40, into strain DB110 by conjugaltransfer. The ColE1 replicon on this plasmid is mobilizable butreplication impaired in SS9 and thus serves as a suicide plasmidallowing selection of plasmid integrants into targeted regionsof the chromosome, i.e., those cloned on the plasmid. Kan^r exconjugants were screened initially by examining their fattyacid profiles at 4°C compared to 15°C. One exconjugant displayinggreatly reduced levels of 18:1 at 4°C was designated EA40 andsaved for further study. The creation of a fabF insertion mutationin EA40 was verified by both Southern and Northern blotting. Southernanalysis revealed the replacement of specific restriction endonucleasefragments in strain DB110 by DNA approximately 6.3 kb larger inthe case of strain EA40 (data not shown). In addition, no fabF-specifictranscripts were detected in total RNA extracted from mutant EA40grown under various temperature conditions (Fig. 1), providingadditional verification of the insertional inactivation of fabFin thisstrain.

Characterization of the fabF mutant as a function of temperature. The percentages and types of fatty acids produced by strains DB110 and EA40 under different growth conditions are listed inTable 2. When examined at a temperature of 15°C, mutant EA40exhibited greatly diminished 18:1 levels relative to the parentalstrain DB110 (4 versus 9.9%, respectively). Moreover, when examinedat the reduced temperature of 4°C, mutant EA40 displayed furtherreductions in 18:1 content, contrary to that observed in strainDB110. At 4°C strain, DB110 produced approximately 10.3% 18:1,whereas the fabF mutant produced only 0.7% 18:1.

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TABLE 2. Fatty acid composition of P. profundum strains as a function of varying temperature and pressure^a

In concert with the reduction of 18:1, the fabF mutant exhibited elevated levels of the saturated fatty acid 14:0 and theMUFA 14:1 and also upregulated the abundance of the omega-3 PUFAall-cis-5,8,11,14,17-eicosapentaenoic acid (EPA; 20:5). Specificallyat 4°C, mutant EA40 also displayed dramatically reduced 16:0 and16:1 levels relative to parental strain DB110. We have previouslynoted that chemical mutants of SS9 or drug treatments which reducethe amount of MUFAs produced by SS9 result in increased 14:0 andEPA levels (1). We do not yet understand how it is that a fabFmutation induces such pleiotropic effects on fatty acid composition.As previously reported for P. profundum strain SS9, differencesin iso-16:0 content reflect differences in phase of growth attime of harvesting (1). Overall, the ratios of unsaturatedto saturated fatty acids (UFA/SFA) of mutant EA40 were comparableto those for strain DB110 under various temperature conditions(Table 2).

The growth characteristics of the fabF mutant at two temperatures are shown in Fig. 2A. At both 15 and 4°C, mutant EA40 displayedgrowth rates and yields essentially identical to those for parentalstrain DB110. These results are consistent with findings in E.coli, where no growth defect at reduced temperatures have beenascribed to fabF strains (43).

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FIG. 2. Growth characteristics of fabF disruption mutant P. profundum strain EA40 and strain DB110 as a function of temperature (A) and pressure (B). (A)

, DB110 at 15°C; $open circle$ , EA40 at 15°C;

, DB110 at 4°C;

, EA40 at 4°C. (B)

, DB110 at 28 MPa; $open circle$ , EA40 at 28 MPa;

, DB110 at 0.1 MPa;

, EA40 at 0.1 MPa.

Characterization of the fabF mutant as a function of pressure. Table 2 displays the fatty acid profiles of mutant EA40 and strain DB110 at 0.1 MPa (9°C) and 28 MPa (9°C). At 0.1 MPa (9°C),mutant EA40 exhibited markedly reduced 18:1 and 16:1 levels andsubstantially increased 14:0, 14:1, and EPA levels compared tostrain DB110. Similarly, at elevated pressure the most dramaticalterations in fatty acid content of mutant EA40 relative to strainDB110 included severe reduction in 18:1 content (1.1 versus 16.2%,respectively) and elevated 14:0 content. These high-pressure EA40values are similar to those of the mutant grown at 4°C (0.1 MPa).However, at the elevated pressure of 28 MPa (9°C), mutant EA40did not upregulate EPA production as it did at 4°C. EPA contentactually decreased upon a shift in growth pressure from 0.1 MPa(9°C) to 28 MPa (9°C) in mutant EA40 (15.1 versus 11.4%, respectively).This is in contrast to strain DB110, wherein EPA content increasedfrom 2.7 to 11% upon pressurization to 28 MPa. Moreover, the UFA/SFAratios of mutant EA40 at 28 and 0.1 MPa (1.77 and 1.20, respectively)were substantially lower than those for strain DB110 (3.57 and2.53,respectively).

The growth characteristics of mutant EA40 at two pressures are shown in Fig. 2B. The effect of fabF disruption on cell growthwas detrimental at elevated pressure. At 0.1 MPa (9°C), the mutantand parental strains exhibited essentially identical growth abilities.However, at an elevated pressure of 28 MPa (9°C), mutant EA40displayed an extended lag phase, decreased growth rate, and reducedoverall yield in comparison to strain DB110. These results representthe first identification of a growth phenotype associated withsole disruption or mutation of the fabFgene.

It is conceivable that the difference between temperature and pressure growth and fatty acid regulation observed in strainEA40 is the result of an anaerobic effect (which pressure cultivationnecessitates). In other words, high-pressure cultivation conditionsalone may be responsible for the observed high-pressure growthphenotype in strain EA40. To address this possibility, strainsEA40 and DB110 were grown at 4 and 15°C (0.1 MPa) under conditionsidentical to those used with pressure cultivation (in heat-sealablebulbs with glucose and HEPES added). These experiments showedno apparent cold sensitivity in strain EA40, suggesting that thehigh-pressure-sensitive phenotype of EA40 is the result of pressureeffects and not the result of cultivation conditions (data notshown).

Nutritional complementation of strain EA40. If the basis of the high-pressure growth defect in EA40 stems from its reduced abundance of 18:1, it should be possible tonutritionally complement this defect by providing an exogenoussupply of this fatty acid in the growth medium. This approachwas previously used with partial success in overcoming the pressure-sensitiveand cold-sensitive growth characteristics of a chemical mutagen-derivedmutant of SS9 deficient in the production of both 16:1 and 18:1fatty acids (1). The growth characteristics of mutant EA40at 28 MPa (9°C) in the presence or absence of exogenous 18:1 inthe form of 0.025% Tween 80 are shown in Fig. 3. In the presenceof exogenous 18:1, mutant EA40 exhibited completely restored growthcharacteristics at elevated pressure. Fatty acid analysis of innerand outer membrane and total phospholipid fractions of strainEA40 grown in the presence of Tween 80 at 28 MPa (9°C) revealedincorporation of 18:1 into the membrane phospholipids, suggestingthat the exogenous 18:1 supplied is actively utilized for membranerestructuring (data not shown). These results provide furtherevidence of the need for 18:1 fatty acid for growth at high pressure.

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FIG. 3. Nutritional complementation of P. profundum fabF mutant EA40 at elevated pressure (28 MPa, 9°C).

, plus 18:1 supplementation; $open circle$ , minus 18:1.

E. coli does not regulate fatty acid composition in an adaptive manner in response to pressure changes. Although the effects of pressure on fatty acid composition in numerous piezophilic and piezotolerant bacteria have been welldocumented (1, 11, 12, 47), the effect of a pressureincrease on the fatty acid composition of a non-pressure-adaptedbacterial species has not yet been described. To determine whetherthe observed effect of elevated pressure on deep-sea bacterialfatty acids is reflective of an adaptive feature specific to microorganismswhich have evolved in high-pressure, pressure-variable environments,or if the response simply reflects a similar physical effect ofhigh pressure and low temperature on some aspect of cell structureor physiology (i.e., membrane fluidity), experiments were conductedusing E. coli as a representative of a mesophilic bacterialspecies.

Table 3 shows the fatty acid profiles of E. coli strains MR86 (fabF::Km^r) and its parental strain SJ16 at 30 MPa (37°C) and 0.1 MPa (37°C)in pressurizable bulb cultures. As described in Materials andMethods, high-pressure cultivation necessitated growth under microaerobicconditions with glucose and HEPES added to the media. In contrastto the fatty acid changes observed in wild-type E. coli strainsin response to temperature downshift, wherein increased productionof UFAs 18:1 and 16:1 are observed at the expense of 16:0 (33),no changes in fatty acid profile were evident when either strain(SJ16 or MR86) was grown at high pressure (Table 2). The UFA/SFAratios of strain SJ16 at the two pressures were essentially identical,0.41 at 30 MPa and 0.38 at 0.1 MPa. Similar results were obtainedfor fabF strain MR86 at various pressures. At 30 MPa (37°C), strainMR86 experiences a slight reduction in UFA production and an increasein SFA content relative to 0.1 MPa (37°C) cultivation. Specifically,high-pressure incubation resulted in an overall increase in 16:0in combination with a reduction in 16:1 content. Consequently,substantially reduced UFA/SFA ratios are observed at elevatedpressure in this strain (0.16 at 30 MPa, compared to 0.38 at 0.1MPa). Unlike pressure increase, temperature decrease (from 37°Cto 15°C) elicited approximately a twofold increase in UFA/SFAratios in both strains (approximately 0.6 to 1.2; our unpublishedresults).

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TABLE 3. Fatty acid composition of E. coli strains as a function of varying pressure^a

Results comparable to those obtained with SJ16 and MR86 were obtained with other E. coli strains, specifically MG1655 (21)and 1100 (15), which also displayed lower UFA/SFA ratios at30- than at 0.1-MPa cultivation. Moreover, fatty acid analysiswas conducted on all four of the E. coli strains studied at 30and 0.1 MPa at a temperature of 30°C in addition to 37°C. No dramaticfatty acid content differences were observed in any of the E.coli strains at 30 MPa (30°C) compared to 0.1 MPa (30°C) cultivation(data not shown). The conclusion from these studies is that E.coli does not modulate fatty acid production in an adaptive mannerin response to a pressure increase, and therefore the responseof many piezophilic bacteria to increase UFA levels with pressureis likely to be an acclimatory feature specific to microorganismsinhabiting high-pressureenvironments.

Similar to arguments made with P. profundum strain EA40, it is possible that the lack of fatty acid regulation at elevatedpressure in E. coli strains is the result of anaerobic ratherthan pressure effects. When grown at 15 and 37°C (0.1 MPa) inpressurizable bulbs, all E. coli strains (MR86, SJ16, MG1655,and 1100) exhibited approximately twofold increases in UFA/SFAratios and no apparent decreased temperature sensitivities (datanot shown). These results suggest that the lack of an adaptivefatty acid regulatory response of E. coli with exposure to elevatedpressure is not a factor of the conditions used for pressurecultivation.

E. coli fabF mutants do not display increased pressure sensitivity. Another contrasting feature between SS9 and E. coli concerns the role of KAS II in growth at elevated pressure. The growthcharacteristics of E. coli strain SJ16 and its fabF mutant derivativeMR86 at various pressures are shown in Fig. 4. Previous reportshave indicated that E. coli fabF mutants are not cold sensitive(20). Likewise, at both 0.1 and 30 MPa (37°C), the growth ofstrain MR86 was identical to that of parental strain SJ16. Finally,no differences in the growth characteristics of the two strainswere observed even when pressure cultivation was performed atreduced temperatures (30 and 15°C, 30 MPa; data not shown). Thus,even the combined effects of elevated pressure and reduced temperaturedid not result in differential growth susceptibility in fabF strainMR86 relative to strain SJ16.

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FIG. 4. Growth characteristics of E. coli fabF disruption mutant MR86 and parental strain SJ16 as a function of pressure. See Materials and Methods for cultivation conditions. Pressure experiments were conducted at a temperature of 37°C.

, SJ16 at 30 MPa; $open circle$ , MR86 at 30 MPa;

, SJ16 at 0.1 MPa;

, MR86 at 0.1 MPa.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The state of the physical environment (i.e., pressure and temperature) influences the physical properties of biological membranes(22). Decreases in temperature or increases in hydrostatic pressureincrease the molecular order of the fatty acyl chains and promotestighter packing of the phospholipids. The biological responseto such environmental conditions often entails the retailoringof membrane composition, most notably increases in fatty acidunsaturation (39, 49). This modification is believed to optimizemembrane structure and function by offsetting the direct effectsimposed by temperature andpressure.

Previous studies employing the deep-sea bacterium P. profundum strain SS9 have revealed direct correlations between UFA productionand growth ability at low temperature or elevated pressure (1,4). In the present study, we have targeted a key enzyme involvedin UFA production, the KAS II product of the fabF gene. Resultspresented here indicate that SS9 KAS II is required for (i) thepiezoregulation of cis-vaccenic acid (18:1) and (ii) piezophilicgrowth. In addition, our data indicate that pressure modulationof fatty acid levels is likely to be an adaptive feature uniqueto high-pressure-adaptedmicroorganisms.

Since the fabF gene plays an essential role in thermal regulation of fatty acid composition in E. coli, we hypothesized thatthe SS9 fabF gene may play a similar role in the increased productionof 18:1 observed in response to pressure increase. P. profundumstrain EA40 containing an insertionally inactivated fabF genewas engineered using a reverse genetics methodology employingthe suicide plasmid pMUT100 (7). Based on the fatty acid profileof strain EA40, a dual role for SS9 KAS II has been revealed.In addition to temperature regulation, the lack of 18:1 modulationin response to pressure increase in strain EA40 suggests thatSS9 KAS II is responsible for the substantial increase in 18:1levels observed in response to pressure increase in fabF⁺ strains (Table 2).

Studies in E. coli have shown that thermal modulation of 18:1 production does not involve de novo enzyme synthesis (17).Such regulation resides at the level of enzyme activity, whereKAS II exhibits increased catalytic efficiency at reduced temperature(16, 18). Northern analyses were performed using P. profundumstrain DB110 cultivated under different pressure and temperatureconditions in order to determine if the SS9 fabF gene exhibitsdifferential expression. Identical transcripts (sizes and amounts)were detected under all pressure and temperature conditions examined,suggesting that the SS9 fabF gene is not transcriptionally regulatedin response to various cultivation parameters (Fig. 1). In lightof these results, we hypothesize that SS9 KAS II displays increasedcatalytic activity at elevated pressure just as E. coli KAS IIdoes at reduced temperature. Given the high level of identitybetween KAS II of SS9 and that of non-pressure-adapted organisms(E. coli KAS II is 76/88% identical/similar to SS9 KAS II), itwill be of interest to analyze the structure and function of SS9KAS II in comparison to the E. coli enzyme. Of course, the factthat SS9 fabF is not transcriptionally regulated does not precludethe possibility that some posttranscriptional processing eventoccurs which influences KAS II abundance at elevated pressure,thereby influencing 18:1synthesis.

In strain DB110, a pressure increase from 0.1 MPa to 28 MPa results in greater than a fourfold increase in 18:1 levels, risingup to 16% of total fatty acids (Table 2). However, under identicalconditions, 18:1 comprised only 1.1% of the total fatty acidsin mutant EA40. The inability to regulate 18:1 levels at elevatedpressure resulted in pronounced high-pressure sensitivity in thisstrain (Fig. 2). The fact that supplementation of this mutantwith exogenous 18:1 resulted in restoration of wild-type-likegrowth rates and yields at elevated pressure (Fig. 3) suggeststhat the 18:1 defect is responsible for its high-pressure-sensitivegrowth phenotype. These results represent the first reported growthalteration observed in any bacterial strain in which fabF is theonly lesion in lipid synthesis. It should be noted, however, thatE. coli strains harboring a mutation in fabF as well as an additionaltemperature-sensitive mutation in fabB (KAS I) are incapable ofproducing any long-chain fatty acids at the nonpermissive temperature(19).

In contrast to high-pressure conditions, strain EA40 exhibited no apparent growth sensitivity at reduced temperature despiteproducing only trace levels of 18:1 at 4°C. Contrary to pressureincrease, temperature decrease did not elicit substantially elevated18:1 production in wild-type SS9 strains (Table 2). Hence, someaspect of high-pressure growth ability appears reliant upon 18:1production which is not apparent at low temperature. The factthat EPA levels increase significantly in response to temperaturedownshift in mutant EA40 but not with pressure increase is puzzling.It would appear SS9 is capable of compensating for decreased 18:1levels at 4°C by increased EPA production but not at increasedpressure. It could be either the change in global membrane fluidity(or membrane phase state) or that within the local environmentof a key membrane protein that accounts for the pressure sensitivityof 18:1-deficient strains. Membrane proteins which are known orimplicated as important for piezophilic growth include CydD (requiredfor the assembly of the cytochrome bd respiratory complex [26]),RseC (an inner membrane protein of unknown function [5, 9]),and the ToxR transcription factor (which regulates the differentialexpression of outer membrane protein encoding genes as a functionof pressure [45]). It is possible that membrane perturbationresulting from altered 18:1 synthesis contributes to the decreasedactivity of some key membrane component and consequently pressuresensitivity.

Attempts to complement mutant EA40 by the introduction of the wild-type SS9 fabF gene into this strain were unsuccessful.Despite the creation of numerous SS9 fabF constructs, expressionproblems prevented complementation of either the 18:1 defect orthe high-pressure-sensitive phenotype of mutant EA40 by fabF containingplasmids (our unpublished results). One possibility is that allof our plasmid constructs lacked a fabF promoter. It could bethat the two fabF transcripts observed in SS9 by Northern blottingresult from a single promoter upstream of acpP and that the fabF-specificmessage arises from a posttranscriptional processing event. However,even SS9 fabF containing plasmids which placed fabF transcriptionunder the control of the Kan^r promoter on pKT231 (3) still failed to transcribe fabF, evenwhen a potential Rho-independent terminator sequence was removedfrom fabF upstream DNA. These results suggest that some mechanismfor tight control of fabF transcription may exist in SS9. CoordinatingfabF expression with that of other fab cluster genes is criticalto viability in E. coli. Excess fabF transcription leads to thecessation of fatty acid synthesis as a result of blockage of fattyacyl chain elongation (42). Because of these FabF toxicity effects,E. coli fabF mutants have yet to be geneticallycomplemented.

Fatty acid compositional adjustment is a near-ubiquitous response to temperature change among bacteria (39). However, unliketemperature, pressure variation is a seldom encountered environmentalparameter outside of the deep sea or deep subsurface. Previousstudies which have documented pressure regulation of fatty acidsin deep-sea bacteria have inferred that such changes reflect acclimationto pressure change (1, 11, 12, 47). However, anotherpossibility is that because high pressure exerts a physical changeon membrane structure similar to that of a drop in temperature(30), most microbes would perceive high pressure as low temperatureand respond accordingly to restore membrane fluidity or phase.Our results with E. coli indicate that at least for this organism,the latter possibility is not the case even though this mesophileis quite piezotolerant, capable of growing at pressures up to50 MPa (54).

Fatty acid profiling of E. coli was performed at various pressures to determine whether fatty acid composition in this mesophileis responsive to pressure change as it is to temperature change.Because various E. coli strains were discovered to exhibit similarfatty acid compositions at low and high pressures, the resultsindicated that the capacity for thermal regulation of UFAs inbacteria does not necessarily predispose microorganisms to respondin a similar fashion to pressure changes, despite the fact thatboth parameters can be manipulated to produce similar effectson membrane structure. These results are in accordance with observationsmade using cultures of the mesophilic protozoan Tetrahymena pyriformisNT-1 (28). As with E. coli, exposure of T. pyriformis to 26MPa did not result in changes in fatty acid composition or fluidityof microsomal membranes. Of course, the possibility exists thatnot all surface-living bacteria would respond as E. coli doesto elevated pressure. For example, bacteria which possess membrane-localizeddesaturases may increase UFA production at elevated pressure dueto activation of such enzymes in response to membrane fluiditychanges.

While investigating pressure effects on the fatty acids produced by E. coli, we also examined the effect of loss of KAS IIon E. coli growth at elevated pressure (Fig. 4). Previous reportshave described the growth characteristics of E. coli at elevatedhydrostatic pressure (6, 53, 54). Upon pressurization,E. coli experiences retardation in growth and reproduction owingin part to inhibition in macromolecular synthesis and cell division(51, 55). The response of E. coli to elevated hydrostaticpressure results in a unique stress response which results ininduction of numerous heat shock and cold shock proteins as wellas many proteins which appear solely in response to high pressure(46). Despite numerous studies having investigated high-pressureeffects on specific functions in E. coli, it is still unclearas to the key pressure point(s) which limits its growth abilityat elevated pressure (32, 37). Due to the physical effectselevated pressure is known to exert on biological membranes (22),it was hypothesized that the state of the membrane could representsuch a pressure point. Since an E. coli fabF mutant did not exhibitincreased pressure sensitivity, something other than membranephospholipid structure most likely limits E. coli growth at highpressure. Possible limiting factors include aspects of chromosomepartitioning (6), macromolecular synthesis (51), cytochromefunction (26), or proton translocation and ATP production (32).

	ACKNOWLEDGMENT

This work was supported by grant MCB96-30546 from the National Science Foundation to D.H.B.

	FOOTNOTES

^* Corresponding author. Mailing address: Center for Marine Biotechnology and Biomedicine, Marine Biology Research Division,Scripps Institution of Oceanography, University of California,San Diego, La Jolla, CA 92093-0202. Phone: (858) 534-5233. Fax:(858) 534-7313. E-mail: dbartlett{at}ucsd.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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2. Altschul, S. F., T. L. Madden, A. A. Schaffer, J. Zhang, Z. Zhang, W. Miller, and D. J. Lipman. 1997. Gapped BLAST and PSI-BLAST: a new generation of protein database search programs. Nucleic Acids Res. 25:3389-3402[Abstract/Free Full Text].

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1.	Allen, E. E., D. Facciotti, and D. H. Bartlett. 1999. Monounsaturated but not polyunsaturated fatty acids are required for growth of the deep-sea bacterium Photobacterium profundum strain SS9 at low temperature and high pressure. Appl. Environ. Microbiol. 65:1710-1720[Abstract/Free Full Text].
2.	Altschul, S. F., T. L. Madden, A. A. Schaffer, J. Zhang, Z. Zhang, W. Miller, and D. J. Lipman. 1997. Gapped BLAST and PSI-BLAST: a new generation of protein database search programs. Nucleic Acids Res. 25:3389-3402[Abstract/Free Full Text].
3.	Bagdasarian, M., R. Lurz, B. Ruckert, F. C. Franklin, M. M. Bagdasarian, J. Frey, and K. N. Timmis. 1981. Specific-purpose plasmid cloning vectors. II. Broad host range, high copy number, RSF1010-derived vectors, and a host-vector system for gene cloning in Pseudomonas. Gene 16:237-247[CrossRef][Medline].
4.	Bartlett, D. H., and E. E. Allen. 1998. Role of unsaturated fatty acids in growth at high pressure and low temperature in the deep-sea bacterium Photobacterium species strain SS9, p. 32-37. In P. B. Bennett, I. Demchenko, and R. E. Marquis (ed.), High pressure biology and medicine. University of Rochester Press, Rochester, N.Y.
5.	Bartlett, D. H., E. Chi, and T. J. Welch. 1996. High pressure sensing and adaptation in the deep-sea bacterium Photobacterium species strain SS9, p. 29-36. In R. Hayashi, and C. Balny (ed.), High pressure bioscience and biotechnology. Elsevier Science B.V., Amsterdam, The Netherlands.
6.	Bidle, K. A., and D. H. Bartlett. 1999. RecD function is required for high-pressure growth in a deep-sea bacterium. J. Bacteriol. 181:2330-2337[Abstract/Free Full Text].
7.	Brahamsha, B. 1996. A genetic manipulation system for oceanic cyanobacteria of the genus Synechococcus. Appl. Environ. Microbiol. 62:1747-1751[Abstract].
8.	Chi, E., and D. H. Bartlett. 1993. Use of a reporter gene to follow high-pressure signal transduction in the deep-sea bacterium Photobacterium sp. strain SS9. J. Bacteriol. 175:7533-7540[Abstract/Free Full Text].
9.	Chi, E., and D. H. Bartlett. 1995. An rpoE-like locus controls outer membrane protein synthesis and growth at cold temperatures and high pressures in the deep-sea bacterium Photobacterium sp. strain SS9. Mol. Microbiol. 17:713-726[CrossRef][Medline].
10.	Cronan, J. E., Jr., and C. O. Rock. 1996. Biosynthesis of membrane lipids, p. 612-636. In F. C. Neidhardt, R. Curtiss III, J. L. Ingraham, E. C. C. Lin, K. B. Low, B. Magasanik, W. S. Reznikoff, M. Riley, M. Schaechter, and H. E. Umbarger (ed.), Escherichia coli and Salmonella typhimurium: cellular and molecular biology, 2nd ed. American Society for Microbiology, Washington, D.C.
11.	DeLong, E. F., and A. A. Yayanos. 1985. Adaptation of the membrane lipids of a deep-sea bacterium to changes in hydrostatic pressure. Science 228:1101-1103[Abstract/Free Full Text].
12.	DeLong, E. F., and A. A. Yayanos. 1986. Biochemical function and ecological significance of novel bacterial lipids in deep-sea procaryotes. Appl. Environ. Microbiol. 51:730-737[Abstract/Free Full Text].
13.	de Mendoza, D., and R. N. Farias. 1988. Effect of fatty acid supplementation on membrane fluidity in microorganisms, p. 119-149. In R. C. Aloia, C. C. Curtain, and L. M. Gordon (ed.), Physiological regulation of membrane fluidity. Alan R. Liss, Inc., New York, N.Y.
14.	de Mendoza, D., A. K. Ulrich, and J. E. Cronan, Jr. 1983. Thermal regulation of membrane fluidity in Escherichia coli: effects of overproduction of $beta$ -ketoacyl-acyl carrier protein synthase I. J. Biol. Chem. 258:2098-2101[Abstract/Free Full Text].
15.	Durwald, H., and H. Hoffmann-Berling. 1968. Endonuclease I-deficient and ribonuclease I-deficient Escherichia coli mutants. J. Mol. Biol. 34:331-346[CrossRef][Medline].
16.	Edwards, P., J. S. Nelson, J. G. Metz, and K. Dehesh. 1997. Cloning of the fabF gene in an expression vector and in vitro characterization of recombinant fabF and fabB encoded enzymes from Escherichia coli. FEBS Lett. 402:62-66[CrossRef][Medline].
17.	Garwin, J. L., and J. E. Cronan, Jr. 1980. Thermal modulation of fatty acid synthesis in Escherichia coli does not involve de novo enzyme synthesis. J. Bacteriol. 141:1457-1459[Abstract/Free Full Text].
18.	Garwin, J. L., A. L. Klages, and J. J. E. Cronan. 1980. Structural, enzymatic, and genetic studies of $beta$ -ketoacyl-acyl carrier protein synthases I and II of Escherichia coli. J. Biol. Chem. 255:11949-11956[Abstract/Free Full Text].
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