Bacteria Are Not What They Eat: That Is Why They Are So Diverse

doi:10.1128/JB.182.2.257-263.2000

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Journal of Bacteriology, January 2000, p. 257-263, Vol. 182, No. 2
0021-9193/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

GUEST COMMENTARY
Bacteria Are Not What They Eat: That Is Why They Are So Diverse

Donna Parke, David A. D'Argenio, and L. Nicholas Ornston^*

Department of Molecular, Cellular and Developmental Biology, Yale University, New Haven, Connecticut 06520-8103

	TEXT

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Microorganisms in the environment encounter a varied and not invariably benign diet. The primary suppliers of nutrients formicroorganisms are plants. Consumers such as fungi and bacteriado not act singly and often offer plants a return on their investment.Fixed nitrogen and scavenged minerals are examples of specificcontributions that microorganisms provide plants as a paybackfor nutritional supply. Such relationships require chemical specificitybecause microbial interlopers are prepared to accept the rewardwithout providing the return. Chemicals or mixtures of chemicalscan be produced by organisms as either inducements or deterrents,and microorganisms will vary in their response. So successfuladaptation requires ongoing shifts in chemical communication amongplants and microorganisms. As is true in the rest of biology,the illusion of constancy is achieved at the cost of constantchange. Evolutionary acquisition must be accompanied by the capacityfor rapid revision ofobjectives.

Among the first to appreciate the nutritional versatility of microorganisms was den Dooren de Jong (9) who classified Pseudomonasisolates largely on the basis of the range of chemical substratesthat would support their growth. The capabilities of these organismswere appreciated by biochemists who saw in them a source of enzymesthat challenged the conventions of central metabolism. The swiftadaptations of the organisms were of interest to physiologistswho sought to understand mechanisms governing synthesis of specializedenzymes for catabolic pathways (38, 39). One of these physiologists,Roger Stanier, recognized that scientific enthusiasm for the traitsof Pseudomonas in general had clouded appreciation of the individualorganisms that express these traits. If scientists were to generalizeabout a trait that they had observed, it was necessary to havea sense of what kind of organism expressed the trait. The generalcapabilities of Pseudomonas are great, but one organism, limitedby its size and genetic information, is obliged to be a specialist.Collections of specialists with shared traits form taxa aboutwhich accurate predictions can be made. By returning to taxonomy,the art of prediction of many biological traits by observationof a few, Stanier saw the opportunity to define the individualsubsets that form the collective whole of Pseudomonas and, asit turned out,beyond.

The landmark investigation of Stanier, Palleroni, and Doudoroff (40) built upon the foundations established by den Doorende Jong and demonstrated more or less sharply defined taxa. Inretrospect, it is evident that taxonomy is a snapshot of evolution.Organisms build upon what went before, and shaped by common ancestryand overlapping selective pressures, groups of organisms formedtaxonomic constellations within the genus then known as Pseudomonas.Indeed, some of the groups were sufficiently distinctive to warranttheir subsequent assignment to separate genera such as Burkholderiaand Comomonas.

Among the bacterial strains in the original Stanier collection were some that did not fit the morphological description ofPseudomonas: these bacteria tended to be paired nonmotile cocci,rather than the typical monoflagellate rods. This trait alonewarranted separate generic status, and Baumann was able to classifythe organisms in the genus Moraxella, now known as Acinetobacter(3). The nutritional versatility of Acinetobacter matches butdoes not mirror that of Pseudomonas, and Baumann was able to designprocedures for specific selection of Acinetobacter strains fromthe environment. He showed that the minimum population of theseorganisms in soil or water samples is 10⁵ viable cells/g, a demonstration of the ubiquity of Acinetobacterin nature (2).

Molecular evidence, particularly 16S RNA nucleotide sequences, were in accord with separate generic assignments for many ofthe organisms in the genus formerly known as Pseudomonas and revealeda startling paradox. Remaining members of Pseudomonas, centeredupon members of the fluorescent group, contain 16S RNA quite similarto that of Acinetobacter, and the latter organisms are placedin the Pseudomonas group in the gamma subdivision of proteobacteriain the National Center for Biotechnology Information taxonomyhomepage. Ribosomes aside, Pseudomonas and Acinetobacter are quitedifferent in morphology, motility, the G+C content of their DNA,chromosomal organization, and as described below,ecology.

In order to explore the discontinuities that separate bacterial taxa, we have focused attention upon a single metabolic system,the $beta$ -ketoadipate pathway. The pathway is widespread among terrestrialmicroorganisms because it allows utilization of growth substrates,such as aromatic and hydroaromatic compounds, that are producedabundantly by plants. Central reactions of the protocatechuatebranch of the $beta$ -ketoadipate pathway are shown in Fig. 1. The mostthorough understanding of the pathway in Pseudomonas and Acinetobacterhas been obtained with one representative from each group. Pseudomonasputida PRS1, the type strain for the species, was used by Stanier'sgroup to establish the biochemical outlines of the $beta$ -ketoadipatepathway (29) which subsequently has been the target of numerousphysiological and genetic investigations (21, 32). Acinetobacterstrain ADP1 (BD413) thus far has resisted subclassification withinthis taxonomically turbulent genus. Originally isolated by Juni,it was shown by him to be highly competent for natural transformation(23), and further, he showed that transformation of a trpE mutantof this strain yielded prototrophs when any other member of thegenus served as a donor (22).

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FIG. 1. Central reactions of the protocatechuate branch of the $beta$ -ketoadipate pathway in bacteria. Metabolic steps or sequences are represented by designations for the associated genes. Plant products such as quinate and phenylpropenoid compounds (ferulate, caffeate, and coumarate) are metabolized to protocatechuate (in the box with the thin black border). Enzymes encoded by the pca genes convert protocatechuate to common metabolites. The intermediate carboxymuconate (in the box with the thick black border) is very toxic, and cells lacking a functional pcaB fail to grow when protocatechuate or metabolic precursors of this compound are added to growth media. Secondary mutations preventing formation of carboxymuconate from aromatic compounds can be selected, which has facilitated genetic analysis of vanAB, pobA, and pcaHG. Exposure of cells to high concentrations of protocatechuate also impedes growth, and characterization of strains resisting this toxicity led to discovery of functions associated with the transporters VanK and PcaK in Acinetobacter. The $beta$ -ketoadipate transporter encoded by pcaT is found in fluorescent Pseudomonas species and has no known counterpart in Acinetobacter.

The genetic system developed by Juni has been of great assistance in analysis of the $beta$ -ketoadipate pathway, and further conveniencehas been provided by the evident toxicity of carboxymuconate,the product of protocatechuate oxygenase (Fig. 1). Mutations knockingout PcaB, the enzyme that acts upon carboxymuconate, prevent thegrowth of cells with succinate if either protocatechuate or p-hydroxybenzoate(Fig. 1) is added to the growth medium (17). Secondary mutationsblocking metabolism of these compounds allow growth with anothercarbon source in their presence. Thus, strains lacking PcaB haveopened opportunities for analysis of mutants defective in catabolismof protocatechuate (8, 14), p-hydroxybenzoate (10, 13),and their metabolic precursors (37; M. A. Smith, G. Huang, D.M. Young, and L. N. Ornston, Abstr. 98th Gen. Meet. Am. Soc. Microbiol.abstr. K-148, p. 350,1998).

It is clear that Acinetobacter and Pseudomonas called upon the same pool for genes for the $beta$ -ketoadipate pathway. Isofunctionalproteins from the two genera usually share amino acid sequenceidentities of about 50% despite the fact that the genes for theseenzymes usually have diverged by more than 12% in the G+C contentof their DNA. It is also clear that the chromosomal organizationof the respective sets of genes is entirely different. Comparisonof the pca gene order (Fig. 2) shows that only three pairs ofgenes (pcaIJ, pcaBD, and pcaHG) retain the same configuration,and two of the pairs (pcaIJ and pcaHG) encode separate subunitsof a single enzyme. Shuffling of the genes has been nearly maximized,although their overall clustering is largely preserved. The selectivebenefit of the shuffling is unknown but would minimize opportunitiesfor recombination between homologous sets of genes (16). Itis possible that shuffling is favored at a point in evolutionarydivergence where the benefits of recombination are outweighedby the detriments (24).

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FIG. 2. Organization of genes for protocatechuate catabolism in P. putida and Acinetobacter. The structures of inducing metabolites are shown. Arrows indicate the transcriptional activator genes pcaR and pcaU. They encode proteins that are similar in sequence and bind to similar operators, but the proteins respond to different inducers.

Acinetobacter and P. putida are also distinguished by the metabolites they use to govern expression of the pca genes (5).In Acinetobacter, all of the pca structural genes are in a singleoperon that is expressed in response to protocatechuate (Fig.2). Insofar as is known, the only P. putida genes expressed inresponse to protocatechuate are pcaHG, the structural genes forprotocatechuate oxygenase. In contrast to Acinetobacter, P. putidaemploys $beta$ -ketoadipate as a regulatory metabolite that inducesall of the enzymes in the protocatechuate pathway except theoxygenase.

Among the P. putida genes is pcaT which has no known counterpart in Acinetobacter. The function of pcaT is subtle, and discoveryof its activity emerged from a false premise about the organizationof the pca genes. The regulatory functions of $beta$ -ketoadipate wereknown, and it seemed likely that all of the pca genes save pcaHGformed a regulon that might be expressed collectively in a constitutivemutant. $beta$ -Ketoadipate was available, so it was possible to selectfor strains that grew with the compound without an induction lagafter transfer from growth medium containing succinate. Demandfor growth with $beta$ -ketoadipate was unusual because Stanier (38,39) had demonstrated that it did not readily permeate the cellmembrane. Slow growth with $beta$ -ketoadipate occurred, so it was possibleto select strains with the desired phenotype (33).

The presumed targets of the selection were pcaIJ, genes for the coenzyme A transferase that acts upon $beta$ -ketoadipate, and thepresumption was that shared regulation would cause constitutiveexpression of pcaB, pcaC, and pcaD. Indeed these three genes wereexpressed constitutively in the selected strains, but mysteriously,pcaIJ were not. What was the target of the selection for rapidadaptation to $beta$ -ketoadipate as a growth substrate? After somebrooding, we entertained the possibility that we had selectedfor constitutive expression of a $beta$ -ketoadipate transport system,now known to be the product of pcaT, and that this gene sharedbiosynthetic regulation with pcaB, pcaC, and pcaD. This hypothesisrequired suspension of disbelief because of the known permeabilitybarriers to $beta$ -ketoadipate but was easily tested because adipate,available in radiochemical form, is not utilized effectively bywild-type P. putida (33).

Quite remarkably, the constitutive mutant strains, unlike wild-type cells, rapidly and effectively concentrated radioactiveadipate. $beta$ -Ketoadipate was a strong competitive inhibitor of theprocess, an observation compatible with the interpretation thatit was the natural substrate of the transport system now knownas PcaT. This conclusion has subsequently been confirmed by sequenceevidence that pcaT is clustered with other genes associated withthe $beta$ -ketoadipate pathway in the pcaTBDC operon of P. putida (21;G. W. Buck, Z. Guo, and J. E. Houghton, Abstr. 98th Gen. Meet.Am. Soc. Microbiol., abstr. K-158, p. 352). These genes are separatedfrom pcaIJ in the chromosome (Fig. 2).

A selective benefit from the $beta$ -ketoadipate transport system is indicated by its broad distribution within the genus Pseudomonas(27), and we are left with the question of its function. Permeabilitybarriers preclude utilization of $beta$ -ketoadipate as a robust growthsubstrate, so what is the contribution of a transport system thatconcentrates the compound? Clues emerge from the regulation ofPcaT. Constitutive synthesis of the transport system is stronglyrepressed by readily utilized growth substrates such as succinateand acetate, and exposure of cells to these compounds also inhibitsthe activity of PcaT (28). Expression of PcaT in constitutivestrains rises as cells go into stationary phase and remains elevatedfor weeks in starved cells. A deleterious consequence is thatexposure of such cells to the nonmetabolizable analog adipatekills them, presumably as a result of the demand for energy tosupport gratuitous transport activity (20).

The observed regulation of the activity of PcaT is consistent with its function as a scavenging system used by starved cellsto assimilate $beta$ -ketoadipate from the environment. Since P. putidais motile, the compound also may serve as a chemoattractant forthe bacteria. The implication that $beta$ -ketoadipate is a nutrientfor some bacteria in the environment was fortified by observationthat wild-type Bradyrhizobium spp. constitutively express a highlevel chemoattraction system for $beta$ -ketoadipate (35). These slow-growingbacteria also constitutively express pcaIJ, genes for the enzymethat acts upon $beta$ -ketoadipate, at a level comparable to that foundin fully induced cultures of the rapidly growing P. putida (33).In contrast, the possibility that $beta$ -ketoadipate may serve as thesole nutrient for Acinetobacter in the environment appears tobe precluded by the fact that growth of these bacteria with thecompound as the sole carbon source requires a mutation leadingto constitutive expression of genes with pcaIJ activity (6).

At first glance, the toxic metabolite carboxymuconate might seem to be an unlikely nutrient in the environment, but as withPcaT, analysis of mutant P. putida strains revealed an inducibletransporter for the compound (26). The notion that carboxymuconatesupports the growth of microorganisms in the environment is fortifiedby the observation that members of the genus Comomonas grow withcarboxymuconate which is not formed by these bacteria during growthwith protocatechuate (30).

The motility of P. putida yielded the first evidence for a biological function associated with a member of what has grownto be a large family of transport proteins associated with the $beta$ -ketoadipate pathway. Mutations blocking attraction of P. putidato p-hydroxybenzoate were demonstrated to be in pcaK, a gene withsequence matching that of known transport proteins. The mutationsalso reduced transport of p-hydroxybenzoate into the cells, althoughit was necessary to elevate the pH in order to demonstrate thiseffect in the laboratory. At lower pH, the transport system mayfacilitate growth with low levels of p-hydroxybenzoate (19).

The sequence of P. putida pcaK closely matches that of an Acinetobacter gene also designated pcaK, and each gene is linkedto other genes associated with protocatechuate catabolism (Fig.2). The Acinetobacter gene was blocked fortuitously by the $Delta$ pcaBDK1deletion designed to cause intracellular accumulation of carboxymuconatefrom protocatechuate (17, 18). As indicated in Fig. 1, themutation prevents growth of Acinetobacter in the presence of p-hydroxybenzoateor protocatechuate and has been useful in analysis of genes requiredfor the first steps in catabolism of these compounds. A differentpattern emerged when the mutant cells were exposed to quinate(Fig. 1) and succinate. Numerous small colonies emerged on thismedium, but contrary to expectation, none of the mutations inthese colonies mapped in the region containing genes known tobe required for quinate catabolism (11). Upon further investigation,it became evident that the mutations were in a chromosomally distantregion containing van genes associated with demethylation of vanillateto protocatechuate (37).

The van genes are unstable. This conclusion emerged from characterization of Acinetobacter $Delta$ pcaBDK1 secondary mutants whichgrew with succinate in the presence of protocatechuate. As expected,such cells usually were blocked in pcaHG, the structural genesfor protocatechuate oxygenase (14). Unexpectedly, about 20%of these cells contained additional mutations preventing conversionof vanillate to protocatechuate (37). This fostered the interpretationsthat protocatechuate is somewhat toxic in its own right and thatinactivation of van genes helped to protect cells against protocatechuatethat had been provided in the growth medium. The premise thatthe van genes are genetically unstable was fortified by characterizationof the genes from strains that had acquired spontaneous defectsin vanAB, the structural genes for vanillate demethylase. Thegenes proved to be susceptible to deletions and rearrangementsto which two recently characterized mobile elements, IS1236 andTn5613, contribute. Any Acinetobacter population of significantsize contains strains blocked in vanillate demethylation. Suchcells are bioreactors that convert the common environmental chemicalferulate to vanillate (37).

Near vanAB in the Acinetobacter chromosome are two genes that, on the basis of sequence comparisons, appear to be associatedwith transfer of exogenous compounds into the cell. One of thesequenced genes matches known porins. The other, directly upstreamfrom the putative porin, is vanK, which is closely related topcaK, mucK, and benK, other genes for transporters known to beassociated with the $beta$ -ketoadipate pathway. Mutants blocked inthe transporters encoded by vanK and pcaK are severely impededin their ability to grow with quinate, and such cells accumulateprotocatechuate in the medium when exposed to quinate. Restorationof wild-type vanK or pcaK to such cells restores their abilityto grow with quinate (7).

These findings are consistent with the interpretation that the first three steps of quinate metabolism, conversion of quinateto protocatechuate, take place on the outer surface of the innercell membrane (Fig. 3). This allows compartmentation of catabolicenzymes that act upon shikimate and dehydroshikimate so that thesebiosynthetic intermediates do not trigger their catabolism inthe absence of an exogeneous supply. The cells' response to protocatechuatealso depends upon how it is supplied. Low concentrations of thecompound can support vigorous growth, and the organism forms twotransport systems (PcaK and VanK) which can move the moleculeinto the cell under these circumstances. Transcriptional regulationof pcaK and pcaHG is unified (Fig. 2), so the transport activityof PcaK is balanced with the activity of the enzyme that removesprotocatechuate as it enters the cell.

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FIG. 3. Compartmentation of quinate catabolism in Acinetobacter. Mutations blocking both pcaK and vanK impede growth with quinate, and cells containing these mutations accumulate protocatechuate in the growth medium. Thus, in accord with earlier suggestions, the initial steps in quinate utilization appear to take place on the outer surface of the inner cell membrane. Not shown in the figure is shikimate which is catabolized directly to dehydroshikimate by QuiA. Compartmentation keeps catabolic enzymes that act upon shikimate and dehydroshikimate physically separate from enzymes that must supply these compounds as biosynthetic intermediates under all growth conditions.

A different kind of balance is achieved with vanK (7). Most spontaneous mutations inactivating this gene abbreviate a homopolymericG tract within vanK by one residue (Fig. 4). Reversion of suchmutants occurs frequently, and any Acinetobacter population containsa mixture of cells. Some contain an active VanK and are preparedto pump protocatechuate into cells when this growth substrateis available at low concentrations. Other cells lack a functionalVanK and therefore can resist the potentially toxic effect ofthe compound when it is provided in high concentrations. Comparisonof the vanK nucleotide sequence with those of related transportsystems (Fig. 4) shows that the homopolymeric G tract, the basisof genetic instability, was acquired by vanK during its evolutionarydivergence from the other transport genes. It is difficult toescape the conclusion that the G tract has selective benefit.Intriguingly, the genetic oscillation of vanK may contribute tothe evolutionary stability of Acinetobacter cell lines that eitheruse VanK or fail to use VanK depending upon the supply of protocatechuate.

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FIG. 4. Frequent mutations causing loss or gain of vanK function in Acinetobacter. The gene acquired a homopolymeric G tract during its evolutionary divergence from related transporters. Evidently slippage during replication can cause loss of a G residue from the tract. This mutation introduces a stop codon directly downstream from the G tract. The deletion reverts readily, so most populations of the Acinetobacter cell line have a mixture of wild-type cells and cells containing the deletion mutation.

Adaptation of cells to different concentrations of a potentially toxic growth substrate illustrates a core strategy of catabolism:how to obtain compounds that are beneficial without accumulatingcompounds that are detrimental. In this context, it is importantto remember that growth substrates are provided singly only inthe laboratory. Even in these cases, the concentrations of potentialgrowth substrates may exceed the threshold of toxicity and, bypreventing growth, may mask the ability of organisms to utilizethe compounds (34). Additional challenges may be introducedinto the environment by toxic chemicals with structures mimickingthose of established growthsubstrates.

Mixtures of compounds are released by plants, and mixtures of genes are required for microorganisms to respond. This necessitymay help to account for supraoperonic clustering of some genesfor catabolic pathways in bacterial chromosomes. A contributingfactor to such clustering may be horizontal transfer (25), butother selective forces may be at work as well. One such forceis the possibility for coamplification by duplication of genesthat are called into play at the same time (1, 8).

Whatever the selective forces favoring clustering, the Acinetobacter pca genes provide part of a rich example. To one sideof the pca operon are genes associated with catabolism of diversecompounds (11, 12; Smith et al., Abstr. 98th Gen. Meet. Am.Soc. Microbiol.) such as quinate, shikimate, and phenylpropenoids(e.g., ferulate), all of which form protocatechuate during theirmetabolism. To the other side of the pca operon is a cluster ofgenes associated with catabolism of dicarboxylic acids (D. Parke,M. A. Garcia, and L. N. Ornston, Abstr. 99th Gen. Meet. Am. Soc.Microbiol., abstr. K-25a, p. 405). All of these compounds sharethe property of being chemically bifunctional in that they canform a vast array of ether and ester bonds as found, respectively,in the plant products lignin and suberin (4). The importanceof lignin is widely appreciated because there is a lot of it:its ether bonds are difficult to break. However, a material neednot be abundant in order to be metabolically significant, andturnover of the biochemically accessible suberin in the environmentmay well exceed that oflignin.

As characterization of chromosomal clusters of catabolic genes proceeds, attention will be drawn increasingly to genes forfilters and pumps (porins [15] and transporters [31]) thatoften emerge as components of catabolic systems. Additional componentsare genes for efflux pumps with an ancient evolutionary historyand now notable for their contributions to antibiotic resistance(36). Unravelling the contributions of all of these biomoleculeswill be a challenging task because of their overlapping specificitiesin the laboratory. The story may be different in the natural environmentwhere populations of cells must adapt to a shifting dietary blend.The cell surface is where the rubber hits the road in bacterialevolution.

As this case study illustrates, questions about metabolism need not be limited to what it is. We also need to know where itcame from, where it is, and when it is. Someday we may learn whyit is. Some years past, the study of metabolism fell out of fashionbecause its fundamental mechanics appeared to have been understood.The same could have been said of the piano more than two centuriesago, but the diverse ways in which it can be played continuedto be a source of creativity, fascination, and delight. So toowith metabolism, two centurieshence.

	ACKNOWLEDGMENTS

Research in our laboratory has been supported by grants DAAG55-98-0232 from the Army Research Office and MCB-9603980 fromthe National ScienceFoundation.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Molecular, Cellular and Developmental Biology, Yale University, P.O.Box 208103, New Haven, CT 06520-8103. Phone: (203) 432-3498. Fax:(203) 432-3497. E-mail: nicholas.ornston{at}yale.edu.

Publication 22 from the Biological Transformation Center in the Yale BiosphericsInstitute.

Present address: Department of Genetics, University of Washington, Seattle, WA 98195-7360.

The views expressed in this Commentary do not necessarily reflect the views of the journal or of ASM.

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32. Parke, D. 1997. Acquisition, reorganization, and merger of genes $---$ novel management of the $beta$ -ketoadipate pathway in Agrobacterium tumefaciens. FEMS Microbiol. Lett. 146:3-12[CrossRef].

33. Parke, D., and L. N. Ornston. 1976. Constitutive synthesis of enzymes of the protocatechuate pathway and of the $beta$ -ketoadipate uptake system in mutant strains of Pseudomonas putida. J. Bacteriol. 126:272-281[Abstract/Free Full Text].

34. Parke, D., and L. N. Ornston. 1984. Nutritional diversity of Rhizobiaceae revealed by auxanography. J. Gen. Microbiol. 130:1743-1750.

35. Parke, D., M. Rivelli, and L. N. Ornston. 1985. Chemotaxis to aromatic and hydroaromatic acids: comparison of Bradyrhizobium japonicum and Rhizobium trifolii. J. Bacteriol. 163:417-422[Abstract/Free Full Text].

36. Saier, M. H., Jr., I. T. Paulsen, and A. Martin. 1997. A bacterial model system for understanding multi-drug resistance. Microb. Drug Resist. 3:289-295[Medline].

37. Segura, A., P. V. Bunz, D. A. D'Argenio, and L. N. Ornston. 1999. Genetic analysis of a chromosomal region containing vanA and vanB, genes required for conversion of either ferulate or vanillate to protocatechuate in Acinetobacter. J. Bacteriol. 181:3494-3504[Abstract/Free Full Text].

38. Stanier, R. Y. 1950. Problems of bacterial oxidative metabolism. Bacteriol. Rev. 14:179-191[Free Full Text].

39. Stanier, R. Y. 1950. Simultaneous adaptation: a new technique for the study of metabolic pathways. J. Bacteriol. 54:339-348.

40. Stanier, R. Y., N. J. Palleroni, and M. Doudoroff. 1966. The aerobic pseudomonads: a taxonomic study. J. Gen. Microbiol. 43:159-271[Medline].

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31.	Pao, S. S., I. T. Paulsen, and M. H. Saier, Jr. 1998. Major facilitator superfamily. Microbiol. Mol. Biol. Rev. 62:1-34[Abstract/Free Full Text].
32.	Parke, D. 1997. Acquisition, reorganization, and merger of genes $---$ novel management of the $beta$ -ketoadipate pathway in Agrobacterium tumefaciens. FEMS Microbiol. Lett. 146:3-12[CrossRef].
33.	Parke, D., and L. N. Ornston. 1976. Constitutive synthesis of enzymes of the protocatechuate pathway and of the $beta$ -ketoadipate uptake system in mutant strains of Pseudomonas putida. J. Bacteriol. 126:272-281[Abstract/Free Full Text].
34.	Parke, D., and L. N. Ornston. 1984. Nutritional diversity of Rhizobiaceae revealed by auxanography. J. Gen. Microbiol. 130:1743-1750.
35.	Parke, D., M. Rivelli, and L. N. Ornston. 1985. Chemotaxis to aromatic and hydroaromatic acids: comparison of Bradyrhizobium japonicum and Rhizobium trifolii. J. Bacteriol. 163:417-422[Abstract/Free Full Text].
36.	Saier, M. H., Jr., I. T. Paulsen, and A. Martin. 1997. A bacterial model system for understanding multi-drug resistance. Microb. Drug Resist. 3:289-295[Medline].
37.	Segura, A., P. V. Bunz, D. A. D'Argenio, and L. N. Ornston. 1999. Genetic analysis of a chromosomal region containing vanA and vanB, genes required for conversion of either ferulate or vanillate to protocatechuate in Acinetobacter. J. Bacteriol. 181:3494-3504[Abstract/Free Full Text].
38.	Stanier, R. Y. 1950. Problems of bacterial oxidative metabolism. Bacteriol. Rev. 14:179-191[Free Full Text].
39.	Stanier, R. Y. 1950. Simultaneous adaptation: a new technique for the study of metabolic pathways. J. Bacteriol. 54:339-348.
40.	Stanier, R. Y., N. J. Palleroni, and M. Doudoroff. 1966. The aerobic pseudomonads: a taxonomic study. J. Gen. Microbiol. 43:159-271[Medline].

GUEST COMMENTARY Bacteria Are Not What They Eat: That Is Why They Are So Diverse

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Bacteria Are Not What They Eat: That Is Why They Are So Diverse