Bacterial Evolution Through the Selective Loss of Beneficial Genes: Trade-Offs in Expression Involving Two Loci

Bacterial Evolution Through the Selective Loss of Beneficial Genes: Trade-Offs in Expression Involving Two Loci

Erik R. Zinser^1,a, Dominique Schneider^b, Michel Blot^2,b, and Roberto Kolter^a
^a Department of Microbiology and Molecular Genetics, Harvard Medical School, Boston, Massachusetts 02115
^b Laboratoire Plasticité et Expression de Génomes Microbiens CNRS FRE2383, Université Joseph Fourier, 38041 Grenoble Cedex 9, France

Corresponding author: Roberto Kolter, Harvard Medical School, 200 Longwood Ave., Boston, MA 02115., rkolter{at}hms.harvard.edu (E-mail)

Communicating editor: J. B. WALSH

ABSTRACT

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ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

The loss of preexisting genes or gene activities during evolutionis a major mechanism of ecological specialization. Evolutionaryprocesses that can account for gene loss or inactivation haveso far been restricted to one of two mechanisms: direct selectionfor the loss of gene activities that are disadvantageous underthe conditions of selection (i.e., antagonistic pleiotropy)and selection-independent genetic drift of neutral (or nearlyneutral) mutations (i.e., mutation accumulation). In this studywe demonstrate with an evolved strain of Escherichia coli thata third, distinct mechanism exists by which gene activitiescan be lost. This selection-dependent mechanism involves theexpropriation of one gene's upstream regulatory element by asecond gene via a homologous recombination event. Resultingfrom this genetic exchange is the activation of the second geneand a concomitant inactivation of the first gene. This gene-for-geneexpression tradeoff provides a net fitness gain, even if theforfeited activity of the first gene can play a positive rolein fitness under the conditions of selection.

MICROBIAL genomes are in a constant state of flux, whereby newgenes are acquired by horizontal transfer and preexisting genesare lost by mutation (LAWRENCE 1999 ; LAWRENCE and ROTH 1999). It is these changes in the repertoire of genes that are thoughtto be the primary mechanisms of prokaryotic adaptation thatlead to speciation. Extensive evidence for the continual expansionand retraction of genomes has been discovered among the specieswhose whole genomes have been sequenced (ANDERSSON et al. 1998; ALM et al. 1999 ; COLE et al. 2001 ; PERNA et al. 2001). Horizontally acquired genetic units range from regions withina single gene to entire gene "islands," often of coordinatedfunction (LAWRENCE and ROTH 1999 ). Loss of genetic materialover the course of the natural history of microbes is also readilyapparent. Both large-scale losses via deletion and gene inactivationsby revertable point mutations (MORISHITA et al. 1981 ; ANDERSSONet al. 1998 ; MAURELLI et al. 1998 ; COLE et al. 2001 ) havebeen observed in modern microbes.

Genes and gene activities are generally thought to be lost frompopulations over the course of evolution by one of two mechanisms:(i) selection against deleterious genes and (ii) selection-independentgenetic drift of neutral or nearly neutral genes (LAWRENCE andROTH 1999 ; COOPER and LENSKI 2000 ). Adaptive losses of geneactivities have been observed in recent studies on the virulenceof Shigella. Whereas nonpathogenic Escherichia coli has bothompT and cadA, Shigella has lost both of these genes, whosepresence attenuates the virulence of the bacterium (NAKATA etal. 1993 ; MAURELLI et al. 1998 ). Adaptive mutation in oneenvironment can often result in lower fitness values for otherenvironmental conditions. This is known as antagonistic pleiotropyand has been observed in a number of experimentally studiedprocesses, including senescence in fruit flies and catabolicdecay in serially transferred glucose-grown E. coli (ROSE andCHARLESWORTH 1980 ; COOPER and LENSKI 2000 ).

Independent of adaptive mutations, genes can also be lost froma population by the fixation of neutral or nearly neutral mutationsvia selection-independent genetic drift. This mechanism, termedmutation accumulation (HUGHES and CHARLESWORTH 1994 ; COOPERand LENSKI 2000 ), is thought to account for much of the lossof genes in prokaryotes: it is impossible to protect every geneagainst mutation and loss by genetic drift if their disappearancedoes not result in a severe loss in fitness (LAWRENCE and ROTH1999 ).

We have investigated the processes of microbial evolution underconditions of prolonged starvation. While the majority of thepopulation quickly dies out during starvation, in bacteria suchas E. coli a significant minority remain viable for months andeven years of prolonged starvation (FINKEL et al. 1997 ; FINKELand KOLTER 1999 ). Prolonged starvation in these cultures ismarked by rapid, continuous evolution among the surviving minority(ZAMBRANO et al. 1993 ; FINKEL and KOLTER 1999 ). One adaptedmutant of E. coli isolated from a starved culture was foundto have acquired four growth advantage in stationary phase (GASP)mutations (ZAMBRANO and KOLTER 1993 ; ZAMBRANO et al. 1993; ZINSER and KOLTER 1999 ). These GASP mutations confer theability of a minority population to grow and invade a wild-typemajority population during the course of culture starvation.Two of these GASP mutations were identified as mutant allelesof the global gene regulators, rpoS and lrp (ZAMBRANO et al.1993 ; ZINSER and KOLTER 2000 ).

In this report we identify a third adaptive GASP mutation (sgaA)in this mutant as a genomic rearrangement, which concomitantlyactivates one locus while inactivating another. Through an insertionof an IS5 element followed by an inversion between it and apreexisting IS5 element, the initially inactive locus effectivelyexpropriated the regulatory element of the initially activelocus. This gene-for-gene expression trade-off is particularlyinteresting because the inactivated locus plays a positive rolein fitness under the conditions in which it was inactivated.The concept of such an expropriation event as a novel evolutionarymechanism of gene loss is then discussed.

MATERIALS AND METHODS

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ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

Fitness assays:
All experiments were performed at 37°. Stationary-phasecompetitions were performed as described (ZINSER and KOLTER1999 ). Briefly, competing strains were marked with either oftwo selectively neutral chromosomal markers: growth on salicinas a sole carbon source (Bgl⁺) or valine-resistant growth onglucose (Val^r). To rule out marker effects on fitness, the Bgl⁺and Val^r markers were switched between competing strains inhalf of the pairwise competitions. Strains were subcultured1:100 into fresh Luria broth (LB) and incubated for 24 hr priorto mixing to facilitate entry into stationary phase. Cultureswere mixed 1:1000 (v:v), and the two populations in the mixedculture were monitored by serial dilution in M63 medium andplating on minimal salicin (0.2%) and minimal glucose (0.2%)plus valine (0.02%) plates. The invasion index, as a measureof relative fitness, was defined as the change in the minorityto total population ratio between days 1 and 3 of the stationary-phasecompetition.

Genetic techniques:
Insertional mutageneses with the mini-Tn10 Cm^r and TnphoA'-1(lacZ) transposons were performed as described (KLECKNER etal. 1991 ; WILMES-RIESENBERG and WANNER 1992 ). Phage P1virtransduction was performed as described elsewhere (MILLER 1992). The TnphoA'-1 insertion alleles were moved into the insertion-/inversion-lessparental background by P1 transduction, selecting for kanamycinresistance and then confirming the absence of the insertion/inversionin the strain by PCR.

Restriction fragment length polymorphism analysis of the GASP mutants:
Restriction fragment length polymorphism (RFLP) analyses (PAPADOPOULOSet al. 1999 ) using eight known E. coli K-12 insertion sequence(IS) elements as probes were performed with EcoRV-digested DNAfrom ZK819 (wild type) and ZK1141 (sgaA; ZAMBRANO and KOLTER1993 ). Among several IS-associated mutations detected in ZK1141,the loss of one IS5-containing fragment (a 3.9-kb fragment,called A) and the gain of two other IS5-containing fragments(3- and 6-kb fragments, called B and C, respectively) were shownto involve a genomic region (14' on the chromosome) known toinclude the sgaA GASP mutation (ZINSER and KOLTER 1999 ). Sequencesadjacent to IS5 fragments in A (using genomic DNA from ZK819),B, and C (using genomic DNA from ZK1141) were cloned after inversePCR (SCHNEIDER et al. 2000 ). Sequence comparisons of the IS5junctions with the E. coli genome sequences suggested a complexrearrangement—a transposition event with an associatedinversion. A new IS5 copy inserted upstream of the cstA geneat 13.6', between its promoter and a CRP-binding site. A recombinationevent between this new IS5 copy and IS5D (located at 14.8' betweenybeJ and cute; BLATTNER et al. 1997 ) led to the inversionof the intervening sequence. This inversion was confirmed byhybridization experiments, using all adjacent sequences of IS5in fragments A, B, and C as probes (data not shown). This rearrangementexplains the loss of fragment A and the gain of fragments Band C in ZK1141.

Construction of the cstA::lacZ fusions:
We analyzed transcriptional activities of plasmid-borne cstA::lacZconstructs, as similar qualitative results with plasmid andchromosomal cstA transcriptional fusions have been reported(SCHULTZ and MATIN 1991 ). We constructed plasmid fusions bycloning the promoter regions of the wild-type parent and theinversion mutant onto the pRS550 plasmid (SIMONS et al. 1987). The promoter of cstA in ZK819 together with the CRP-bindingsite (prior to the inversion) was cloned into pRS550 by PCR,leading to plasmid pGBE153. The promoter of cstA in ZK1141 (afterthe inversion) was cloned into pRS550 by PCR. The resultingplasmid, pGBE155, carries the cstA promoter as well as the upstreamIS5 element. The sequence of the primers was designed to introducesuitable BamHI and EcoRI restriction sites, allowing the easycloning of the PCR products into pRS550. The two plasmid constructswere introduced into ZK126 by standard techniques.

Construction of the ${Delta}$ cstA mutants:
A cstA deletion was constructed in the ZK819 background. ThecstA gene was cloned by PCR using the PCR-Script Cam cloningkit (Stratagene, La Jolla, CA). A deletion within cstA was createdby cutting the resulting plasmid with MluI, which cuts twicewithin cstA, and religating the large fragment. The new plasmidcontains an in-frame 1275-bp deletion within cstA. The insertwas isolated as a SacI-SalI fragment and cloned into the suicide-plasmidpCVD442 cut with SacI-SalI (DONNENBERG and KAPER 1991 ). Thein-frame deletion mutant allele of cstA was introduced, as described(DONNENBERG and KAPER 1991 ), in the chromosome of ZK819, generatingthe ${Delta}$ cstA derivative, GBE111. The presence of the deletion wasconfirmed by PCR and hybridization experiments (data not shown).The ${Delta}$ cstA derivatives of the ZK2552 and ZK2553 strains were constructedby P1 transduction. First, the lipA150::Tn1000d allele was transducedwith P1 phage from KER176 into ZK2552 or ZK2553 (ZINSER andKOLTER 1999 ), selecting for kanamycin resistance. Then the ${Delta}$ cstA allele was transduced from GBE111 into the lipA150::Tn1000dtransductants, selecting for lipoic acid prototrophs. Transductantscarrying the ${Delta}$ cstA allele were identified by PCR using the primersthat flanked the deleted region.

RESULTS

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ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

The sgaA GASP mutation is a genomic rearrangement involving insertion sequence elements:
Previous work identified two of the four adaptive mutationsof a survivor of an aged culture of E. coli as loss-of-functionalleles of the global regulators, rpoS and lrp (ZAMBRANO etal. 1993 ; ZINSER and KOLTER 2000 ). All four of the GASP mutationsin this mutant confer growth phenotypes in addition to GASP.One of the two unidentified GASP mutations, sgaA, confers fastergrowth on glutamate, asparagine, and proline as carbon sourcesand confers the new ability to grow on aspartate as a sole carbonsource (ZINSER and KOLTER 1999 ). It was hypothesized that thesegrowth phenotypes allow the sgaA mutant to outcompete the wild-typeparent for amino acids as nutrients released by the dying majoritypopulation during prolonged starvation (ZINSER and KOLTER 1999). To identify the sgaA GASP locus, an insertional mutagenesisstrategy was employed. Mutants of the sgaA strain with randommini-Tn10 insertions were screened initially for a loss of growthon aspartate, followed by a secondary screen for loss of theGASP phenotype relative to its sgaA⁺ parent. An insertion inthe gltJ locus eliminated both the aspartate growth and GASPphenotypes of the sgaA strain (data not shown).

The gltJ gene is a member of a putative five-gene operon (Fig 1A;BLATTNER et al. 1997 ), the first four members of whichare thought to encode the components of the known aspartate/glutamatebinding protein-dependent ABC-type transporter of E. coli (WILLISand FURLONG 1975 ; D. LUM and B. J. WALLACE, unpublished data).The predicted YbeJ product is most similar to known periplasmicbinding protein components, the GltJ and GltK products are mostsimilar to known integral membrane protein components, and theGltL product is most similar to known ATPases. The predictedproduct of ybeK, the final gene of the putative operon, sharesclosest homology to known nucleoside hydrolases (alignmentsnot shown).

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Figure 1. The sgaA GASP mutation is a two-step genomic rearrangement involving two IS5 elements. Asterisks denote the sites of these genomic rearrangements. (A) In the wild-type parent, the putative ybeJ-gltJKL-ybeK operon is $~$ 60 kb away from the cstA locus. The two loci are transcribed in opposite orientation. (B) The first rearrangement was an insertion of a new IS5 between the transcriptional promoter and the upstream CRP box of cstA. (C) The second rearrangement was an inversion between this new IS5 and the IS5 (IS5D) upstream of the putative ybeJ-gltJKL-ybeK operon. The exact point of crossover between the IS5 elements is unknown. Arrows above the IS5 elements indicate the direction of the ins5A transcript.

RFLP and sequence analyses identified the sgaA GASP mutationas a complex two-step recombination event involving an IS5 element(designated IS5D in the published E. coli genome; BLATTNERet al. 1997 ) present in the wild-type parent 103 bp upstreamof the start of the ybeJ open reading frame (Fig 1A). The firstevent was an insertion of a new IS5 element at a position 60kb away from IS5D, between the transcriptional promoter andthe upstream CRP-binding site (CRP box) of the cstA gene, whichis thought to encode an oligopeptide permease (SCHULTZ and MATIN1991 ; Fig 1B). The second event was a homologous recombinationevent between the new IS5 and IS5D, resulting in a chromosomalinversion (Fig 1C). This rearrangement effectively placed theupstream region, including the CRP box, of cstA upstream ofthe ybeJ-gltJKL-ybeK operon. This two-step recombination event,termed IN(cstA::IS5-IS5D), was the only mutation detected betweenybeJ and the CRP box in the sgaA mutant (data not shown).

The sgaA insertion/inversion event activates one locus while inactivating another:
Given that the ybeJ-gltJKL-ybeK operon encodes a putative aminoacid transporter, it was hypothesized that the sgaA genomicrearrangement enhanced the growth rate on amino acids by increasingexpression of this operon, thereby increasing the transportcapacity of the cell. Analysis of chromosomal lacZ transcriptionalfusions within the ybeJ-gltJKL-ybeK operon, constructed by transposonmutagenesis (WILMES-RIESENBERG and WANNER 1992 ), confirmedthis prediction. Expression of the ybeJ::lacZ fusion was significantlyhigher at all cell densities in the sgaA strain compared tothe sgaA⁺ parent (Fig 2A). Fusions to gltJ and gltK behavedsimilarly to the ybeJ fusion (data not shown), suggesting thatall three genes are members of an operon.

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Figure 2. Transcriptional activities of genes on either side of the sgaA insertion/inversion. (A and B) ß-Galactosidase activities (MILLER 1992

) of mutants with chromosomal lacZ insertions in the ybeJ (A) or IS5 (B) loci. The genetic backgrounds were sgaA⁺ ( ${blacksquare}$ ), sgaA (•), sgaA⁺ ${Delta}$ crp-45 ( ${square}$ ), and sgaA ${Delta}$ crp-45 ( ${circ}$ ). Each point is the average of duplicate assays performed on an LB-grown culture, inoculated 1/100 from a stationary-phase culture. (C) ß-Galactosidase activities of the ZK126 (wild-type) strain with plasmid-borne lacZ fusions to the upstream regulatory elements of the cstA allele of the sgaA⁺ (pGBE153, open bars) or sgaA (pGBE155, hatched bars) strains. Cultures were assayed during midexponential growth and stationary phase in LB broth. The values are means ±95% confidence intervals of three independent experiments.

Significantly, the expression pattern of ybeJ in the sgaA strainwas essentially the same as cstA in the wild type (SCHULTZ andMATIN 1991 ). Expression greatly increased when the cultureentered stationary phase (Fig 2A). Expression of ybeJ was alsofound to be CRP dependent, as it was eliminated when the ${Delta}$ crp-45allele was introduced (Fig 2A). The loss of ybeJ expressionin the ${Delta}$ crp-45 strains was due only to the absence of CRP protein,as normal induction was observed after introduction of a wild-typecrp allele in a pBR322 plasmid (data not shown). These resultsindicate that the regulatory components of the region upstreamof cstA were effectively transferred and are indeed functionalupstream of the ybeJ-gltJKL-ybeK operon in the sgaA mutant.

Interestingly, a transposon insertion within the IS5 elementupstream of the ybeJ-gltJKL-ybeK operon inactivated the operon,as seen by a concomitant loss of the GASP phenotype and theamino acid growth phenotypes in the sgaA background. Expressionfrom the IS5::lacZ fusion, oriented in the same direction asthe ybeJ-gltJKL-ybeK operon, demonstrated that expression ofthe ins5A transposase gene within the element (KROGER and HOBOM1982 ) is also dependent on the insertion/inversion mutation,growth phase, and CRP (Fig 2B). CRP therefore appears to activatethe ins5A promoter, p_5l (KROGER and HOBOM 1982 ), by bindingat the CRP box, located 73.5 bp upstream, which is near theoptimal distance of 61.5 bp for CRP activation (BUSBY and EBRIGHT1999 ).

Concomitant to the activation of the ybeJ-gltJKL-ybeK operonby the expropriation of the regulatory region of cstA was theinactivation of the cstA locus. We analyzed transcriptionalactivities of plasmid-borne cstA::lacZ constructs. Expressionfrom the cstA promoter of the sgaA mutant was significantlylower than that of the wild-type parent, in both exponentialand stationary-phase cultures (Fig 2C), indicating a severedecrease in cstA activity for the sgaA strain. The overall consequenceof the insertion/inversion event was therefore to activate theybeJ-gltJKL-ybeK operon while simultaneously inactivating thecstA locus.

The cstA locus plays a beneficial role during stationary phase:
The cstA gene encodes a starvation-inducible oligopeptide permease(SCHULTZ and MATIN 1991 ) and may therefore play a role in stationary-phasefitness by allowing the surviving cells to scavenge from thedying majority oligopeptides as nutrient resources (ZINSER andKOLTER 1999 ). If so, the decrease in cstA activity of the sgaAmutant suggested that the insertion/inversion mutation may havecompromised its ability to compete for oligopeptides duringstationary phase. We therefore examined the role cstA playsin establishing stationary-phase fitness and the consequencesof the loss of this gene's activity on the fitness of the sgaAmutant.

Competition experiments with a constructed in-frame ${Delta}$ cstA mutantstrain confirmed a positive role for cstA activity in establishingstationary-phase fitness. We defined relative fitness as theability of one population, when inoculated as a thousandfoldminority, to invade a differentially marked majority populationover the course of the stationary-phase incubation, a periodin which the total population decreases only gradually (ZAMBRANOet al. 1993 ). A wild-type minority population that expressedthe cstA gene (WT) invaded a majority that could not ( ${Delta}$ cstA; Fig 3A). However, this same minority could not invade a majoritythat could express cstA (Fig 3A). Hence, there is a clear competitiveadvantage for the ability to express cstA during stationaryphase.

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Figure 3. Relative fitness of strains with different cstA and sgaA alleles. Differentially marked (Bgl⁺ and Val^r) LB-grown stationary-phase cultures (24 hr) were mixed 1:1000 and assayed for viable counts on selection plates. Invasion index represents the mean change in the minority-to-total population ratio between days 1 and 3 of the stationary-phase competition (±SD, n $>=$ 6). For each pairwise competition, two to four replicate experiments were performed for each neutral marker configuration. To rule out marker effects on fitness, the Bgl⁺ and Val^r markers were switched between competing strains in half of the pairwise competitions. (A) The wild type (WT) showed a positive invasion index when competed as a minority vs. the cstA null mutant ( ${Delta}$ cstA), but did not when competed vs. a differentially marked wild type. (B) The wild type and the sgaA mutant each showed a positive invasion index when competed as a minority vs. each other. The cstA null mutant showed a lower invasion index compared to the wild type when competed as a minority vs. sgaA. Data for the sgaA minority vs. the wild-type majority competition are from ZINSER and KOLTER 1999

The sgaA mutant has lost the fitness benefit of the cstA locus:
sgaA was identified as a GASP mutation, and sgaA mutants caninvade an sgaA⁺ (WT) majority population (ZINSER and KOLTER1999 ; Fig 3B). However, because the sgaA mutant has lost transcriptionalactivity of the cstA locus, it should have also lost the fitnessbenefit of cstA. Indeed, the wild type was clearly able to invadethe sgaA majority population when placed as a minority (Fig 3B).This advantage was due primarily to the cstA products,as the ${Delta}$ cstA strain could not invade nearly to the same levelas the wild type (Fig 3B). Hence, both the sgaA mutant and thewild type demonstrate a fitness advantage when competed vs.the other strain as a minority population. Such dependence ofrelative fitness on relative cell density indicates that thetwo strains compete for different nutrient resources and occupydifferent niches in stationary-phase cultures.

DISCUSSION

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ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

We have characterized a two-step genomic rearrangement thatoccurred during prolonged starvation and have demonstrated thatthis mutation provides a fitness gain in stationary phase. TheIN(cstA::IS5-IS5D) mutation activated the ybeJ-gltJKL-ybeK operonby placing a CRP-binding element upstream of the operon. Concomitantwith the activation of the ybeJ-gltJKL-ybeK operon was the inactivationof the cstA locus. Expression of either locus provided a clearability to invade a majority that was incapable of expressingthat locus, indicating that both loci contribute toward fitnessin the same selection environment. From these data we proposethat the insertion/inversion mutation sgaA resulted in an obligateresource trade-off, in which the initial ability to exploitone resource at equal fitness with the parent (oligopeptides),is forfeited for the new ability to outcompete the parent foranother resource (monomeric amino acids). Even with the lossin fitness for the first resource, the insertion/inversion mutationresulted in a net fitness gain, likely because it acted to createa new niche for the mutant during starvation conditions.

We have shown that transposable elements were responsible forthe activation of the ybeJ-gltJKL-ybeK operon (and inactivationof the cstA gene). Transposable elements have been found toactivate transcription of adjacent genes by introducing completeor partial promoters located within the element itself or bydisrupting or displacing a negative element that normally shutsdown transcription (SYVANEN 1984 ). The mechanism of gene activationby the IN(cstA::IS5-IS5D) mutation is distinct from the onesdescribed above. In this case, a transcription-activating DNAfragment is brought into proximity of the adjacent gene, butit is not carried by the transposable element (otherwise, expressionof the ybeJ-gltJKL-ybeK operon would not have been dependentupon the inversion event).

Recombination-mediated regulatory element expropriation as amechanism of gene activation/inactivation has been well establishedas a type of phase variation in bacteria (HENDERSON et al. 1999) and as a causative agent in the human cancer, Burkitt lymphoma(DALLA-FAVERA et al. 1982 ; SHEN-ONG et al. 1982 ; TAUB etal. 1982 ). Directed evolution studies in Salmonella entericahave also demonstrated occurrence of expropriation events inthe restoration of inactive genes under intense selection pressures(SCHMID and ROTH 1983 ).

Here we describe regulatory element expropriation as a selection-dependentmechanism for the loss of genes or gene activities during evolution.Gene inactivation is a byproduct of the regulatory element expropriationevent and, as long as the net fitness change is positive, selectionwill favor the loss of the gene's activity. These expropriationevents can effectively select against gene activities that aredeleterious, neutral, or beneficial to the organism under theconditions of selection. We note a distinction between the expropriationand the classical mutation accumulation mechanisms of gene activityloss. In expropriation, the loss of gene activity is selectiondependent, because it is a necessary consequence of the overallfitness gain. By contrast, under mutation accumulation, lossof gene activity is a neutral or nearly neutral event and resultsfrom selection-independent genetic drift (ROSE and CHARLESWORTH1980 ; HUGHES and CHARLESWORTH 1994 ; COOPER and LENSKI 2000). Expropriation may also differ from antagonistic pleiotropy,in which there is a direct selection against a deleterious geneactivity (ROSE and CHARLESWORTH 1980 ; HUGHES and CHARLESWORTH1994 ; COOPER and LENSKI 2000 ). Expropriation may thereforerepresent a third mechanism that can account for the loss ofgene activity.

Regulatory element expropriation may play a significant rolein the process of ecological specialization and evolution inmicrobes. Growing evidence suggests that the predominant mechanismof microbial evolution is lateral gene transfer (GUTTMAN andDYKHUIZEN 1994 ; LAWRENCE and ROTH 1996 ; LAWRENCE and OCHMAN1998 ; NELSON et al. 1999 ). For lateral gene transfer to modifythe functional activities of the recipient and therefore alterfitness, not only must genetic material be transferred to therecipient, but also the expression of the transferred genesmust be properly regulated (LAWRENCE and ROTH 1996 ). Expropriationmay be an important method to provide immediate selective valueto introduced genes, for it would avoid incompatibilities ofthe donor's promoters and regulatory elements with the recipient'stranscriptional machinery and regulators (LAWRENCE and ROTH1996 ). IS element-mediated gene transfer events can insertforeign genes into positions where they become regulated byendogenous promoters (KASAK et al. 1993 ). Subsequent excisionor decay of the IS element can remove all traces of its involvementin the transfer event. Such expropriation events may thereforebe common in the evolutionary history of microbes, because theyprovide an overall fitness gain to the organism, notwithstandingfitness losses due to inactivation of the preexisting gene.

Initial loss of function by regulatory element expropriationleaves the structural gene intact. If the lost activity is beneficialunder the selection conditions there will be considerable pressureto restore the activity, which can be accomplished by reversion(in this case, by "back" inversion). Such revertants would beat an advantage among a majority of nonrevertants (as seen in Fig 3B), and frequency-dependent selection could establisha form of phase variation (HENDERSON et al. 1999 ), keepingthe gene activity within the population in a metastable state.However, if prior to a reversion event secondary mutations arisewithin the structural component of the inactivated gene (whichwould be neutral events), then genetic drift could lead to permanentloss of the gene.

FOOTNOTES

¹ Present address: Department of Civil and Environmental Engineering,Massachusetts Institute of Technology, Cambridge, MA 02139.
² Deceased September 2002.

ACKNOWLEDGMENTS

We thank S. Dove for strains and valuable discussions. We alsothank S. Finkel for valuable discussions and for critical readingof the manuscript. Research was supported by the National Institutesof Health and National Science Foundation (R.K.) and CentreNational de la Recherche Scientifique and Commissariat àla Énergie Atomique (M.B.).

Manuscript received December 14, 2002; Accepted for publication March 26, 2003.

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