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From the Cover
BIOLOGICAL SCIENCES / EVOLUTION
Cooperation and conflict in microbial biofilms

Joao B. Xavier, and Kevin R. Foster^*

Center for Systems Biology, Harvard University, Bauer Laboratory, 7 Divinity Avenue, Cambridge, MA 02138

Edited by Richard E. Lenski, Michigan State University, East Lansing, MI, and approved November 13, 2006 (received for review September 1, 2006)

	Abstract

Top Abstract Results and Discussion Conclusions Methods Acknowledgements References

 
Biofilms, in which cells attach to surfaces and secrete slime (polymeric substances), are central to microbial life. Biofilms are often thought to require high levels of cooperation because extracellular polymeric substances are a shared resource produced by one cell that can be used by others. Here we examine this hypothesis by using a detailed individual-based simulation of a biofilm to investigate the outcome of evolutionary competitions between strains that differ in their level of polymer production. Our model includes a biochemical description of the carbon fluxes for growth and polymer production, and it explicitly calculates diffusion–reaction effects and the resulting solute gradients in the biofilm. An emergent property of these simple but realistic mechanistic assumptions is a strong evolutionary advantage to extracellular polymer production. Polymer secretion is altruistic to cells above a focal cell: it pushes later generations in their lineage up and out into better oxygen conditions, but it harms others; polymer production suffocates neighboring nonpolymer producers. This property, analogous to vertical growth in plants, suggests that polymer secretion provides a strong competitive advantage to cell lineages within mixed-genotype biofilms: global cooperation is not required. Our model fundamentally changes how biofilms are expected to respond to changing social conditions; the presence of multiple strains in a biofilm should promote rather than inhibit polymer secretion.

sociobiology | bacteria | individual-based modeling

A defining feature of many biofilms is the matrix or slime that surrounds the cells (1, 2). These extracellular polymeric substances (EPS) are present in many biofilms where they embed bacteria. Despite the ubiquitous nature of polymer production, the exact evolutionary benefits it provides are unknown. However, polymers are typically viewed as a shared resource that provides a benefit to the biofilm by maintaining its structure (15, 16); protecting it from aggressive agents such as dehydration, ultraviolet radiation, and predator grazing (5–10, 17); and facilitating extracellular enzymatic activity and signaling (6). In the first model of its kind, Kreft (5) analyzed the success of strains with different rates of substrate uptake in mixed biofilms. He showed that slow-growth, high-yield strains could be exploited by high-growth, low-yield strains, and he concluded that cooperation and altruism were necessary for optimal biofilm formation. Like slow substrate uptake, polymer production reduces the available energy for growth. What then maintains polymer production in the face of selection for competition and rapid growth?

Perfect cooperation in biofilms is predicted when they contain a single strain (high genetic relatedness) (5–7). Genetically identical cells, as occurs in most multicellular organisms, do not have evolutionary conflicts of interest, and they are predicted to behave simply as is optimal for the group (18–20). We currently know very little of within-species genetic diversity in biofilms. However, given the huge diversity of species that can occur within biofilms (21–23), it seems unlikely that all or indeed most biofilms will have the clonal structure necessary to generate perfect cooperation throughout. We, therefore, investigated whether cooperation was necessary for polymer production in an individual-based simulation.

Our model investigates the outcome of evolutionary competitions between strains that differ in their level of extracellular polymer production [see supporting information (SI) Fig. 6]. Fig. 1 represents the carbon fluxes involved from the uptake of a substrate (e.g., glucose) to the formation of the end-product biomass (X) and EPS. A central parameter is the investment in polymer production, f, or more specifically, the carbon dedicated to polymer production:

where the r terms capture the rate of EPS and biomass production (for a full list of terms, see Table 1). Further assumptions are needed to characterize the system fully. Substrate uptake is assumed to be the rate-limiting step, and it is described by double-saturation kinetics (Table 2)

The concentration of all intermediaries is assumed to be at steady state. The yield of carbon that goes into organic matter production, i.e., X and EPS, is constant, and the remaining carbon is released as CO₂, hence,

where Y is the yield coefficient for use of carbon. The oxygen consumption is related to CO₂ consumption by a second yield coefficient, Y_O,

Having defined the system, mass conservation for carbon produces the following equations for the rate of biomass and EPS,

and

Biofilms consist of densely packed aggregates inside of which fluid flow is reduced and where most of the solute transport to and from the bacteria occurs through diffusion. The dimensions of typical biofilms are large enough that the diffusion of solutes through the matrix is slow compared with the bioconversions occurring, creating well known solute gradients (24). In aerobic biofilms, for example, gradients in oxygen concentration are formed, and consequently cells at the biofilm surface experience more favorable conditions than cells in the interior where conditions are anoxic (25). Importantly, it might be expected that polymer production, which alters the structure and density of the biofilm, will have important effects on the solute gradients and resulting concentrations of resources experienced by cells.

View larger version (12K): [in this window] [in a new window]   Fig. 1. Simplified representation of the pathway for growth on glucose of an EPS-producing strain (EPS+) (a) and a corresponding nonproducer (EPS–) (b). Triple dots represent pathway intermediaries whose concentration is assumed to be stationary. In this pathway, glucose uptake is the rate-limiting step, and it has the same expression for both EPS+ and EPS– strains. EPS– has a higher intrinsic growth rate by directing its carbon flux to biomass, as opposed to dedicating part of the flux to EPS synthesis as in the case of EPS+.

	Results and Discussion

Top Abstract Results and Discussion Conclusions Methods Acknowledgements References

 
Simple Competition of EPS+ and EPS–. Direct-competition simulations were initialized with an equal amount of individuals of each strain placed randomly at the solid substratum. We observed the outcome after 20 days of growth (Fig. 2, SI Movies 1–3, and http://sysbio.harvard.edu/csb/foster/biofilmeps/). Fitness of both EPS+ and EPS– was then computed as the average number of cell divisions occurring during this time:

Fig. 3 shows that the outcome of competition depends on the value of EPS production (f) and the density of EPS (_X/_EPS ratio). For high EPS densities (_X/_EPS = 1) EPS+ producers lose the competition against EPS–, independently of the value of f. However, for low EPS densities (_X/_EPS >1), there is a broad range of values of f for which EPS+ wins, despite the higher intrinsic growth rate of EPS–. This observation is illustrated in Fig. 2, which contrasts the effects of EPS production, with and without solute gradients. The upper simulation (a–d) was carried out by shutting off the diffusion–reaction component of our model to simulate the unrealistic case where no solute gradients exist. In these conditions, the competition is purely driven by growth rate, and EPS– wins. The lower simulation (e–h) was carried out with the diffusion–reaction back on. The resulting gradients now give EPS+ an advantage of rapid progression toward the top of the biofilm.

View larger version (54K): [in this window] [in a new window]   Fig. 2. Direct competition between an EPS+ and EPS– showing the importance of oxygen gradients in the outcome of the competition. (a–d) Simulation (a–c) and competition outcome (d) in the unrealistic case of absence of oxygen gradients. In this case, competition is decided purely by growth rate, and the fast-growing strain (EPS–) wins. (e–h) Simulation (e–g) and competition outcome (h) in the presence of oxygen gradients, showing the advantage to the EPS+ strain. Note, however, that the EPS+ strains only gain an advantage after a few days of growth so that for transiently formed biofilms, the EPS+ strategy will not be favored. (a–c and e–g) Oxygen concentration is shown in the background, where thick isoconcentration lines are shown for 1 mg/liter steps, and thin gray isoconcentration lines represent order of magnitude changes in the concentration (i.e., 0.1 mg/liter, 0.01 mg/liter, 0.001 mg/liter, etc.). These simulations where carried out at f = 0.55 for the EPS+ strain and X/EPS = 6. See also SI Movies 1–3.

View larger version (18K): [in this window] [in a new window]   Fig. 3. Relative growth rate of an EPS+ in a biofilm with an equal starting frequency of an EPS–. Competition outcome depends on both the rate of EPS production of the producing strain and the density of EPS (X/EPS). Importantly, the EPS– often loses despite its higher intrinsic growth rate. Each box and whisker set results from 10 replicate simulations. Lines are a curve fitting using results from the 10 replicates. The dashed line represents the fitness of value 1, i.e., the borderline value above which the competition is won by EPS+.

where, following Eq. 8, w_S1 is the fitness of a rare mutant in competition with the strategy S2, which is the majority in the population. Importantly though, w_S2 is not the fitness of the cells in direct competition with the rare mutant but rather the mean fitness of all S2 individuals in the population. With an assumption of large population sizes, we take this measure to equal the fitness in a biofilm containing only S2 cells, which assumes that cells go through a phase of global competition at the whole-population level (33), i.e., that cells disperse randomly after growth in a biofilm such that the more cells of a strain present in a biofilm, the higher the contribution to subsequent biofilms. Eq. 8 then evaluates whether the rare mutant reproduces more rapidly than an average cell of the majority strategy in the population and therefore its ability to invade. Both the invasiveness of EPS+ over EPS– was computed (EPS+ EPS–) and vice versa (EPS– EPS+).

We investigate invasion for different initial frequencies of the rare mutant, which captures the effect of different numbers of strain randomly settling during biofilm initiation. For example, if many different strains are always present, then the initial frequency of a rare mutant will be low: with 10 strains, a rare mutant will start at a frequency of 0.1 in the biofilm. Of course, when a mutant first arises, its proportion in a biofilm will depend on when exactly the mutation occurred. However, this first biofilm will not determine invasion success, so we consider only the subsequent biofilms, in which its initial frequency is defined precisely by the number of strains at biofilm initiation.

The presence of many strains at biofilm initiation favors invasion of polymer-producing strains (Fig. 4). Invasion is also strongly dependent on the polymer density and most favored at low densities (high _X/_EPS). Interestingly, for some conditions, we find both that EPS+ can invade an EPS– population and the reverse, which is characteristic of negative frequency-dependent selection (34) and predicts the existence of genetic polymorphism under some conditions, in which both EPS+ and EPS– strains coexist stably in the population.

View larger version (13K): [in this window] [in a new window]   Fig. 4. Rare-mutant invasion analysis. (a) Invasion of a rare polymer-producing strain (EPS+) into a population of nonproducers (EPS–). (b) Invasion of a rare EPS– strain into a population of EPS+ strains. The x axis captures the number of strains randomly settling to form biofilms, where increased strains (and reduced within-group relatedness) cause a lower initial frequency of the rare mutant. For example, if 10 strains are present in all biofilms, the initial frequency of a rare mutant will be 0.1. All simulations were carried out at f = 0.5. Each box and whisker set results from 20 replicate simulations.

Why Do Polymer Producers Win? Polymer-producing cells invade most easily when many strains found a biofilm (Fig. 4); that is, polymer producers perform best with low relatedness at biofilm initiation (6, 7, 19). Indeed, fitness is lower in polymer producers than nonproducers in single-strain biofilms (rightmost bar of Fig. 4a), which suggests that polymer production is selected specifically because it provides a selfish competitive advantage to strains in mixed biofilms. To understand better the fitness effects of polymer production, we modeled a single polymer-producing cell in a field of nonproducers (Fig. 5), which was used to calculate the fitness effects of the EPS+ strategy on the lineage of the focal cell and on lineages of EPS– cells at increasing distance from the focal cell.

View larger version (66K): [in this window] [in a new window]   Fig. 5. Polymer production by a founding cell is altruistic to the cells above but spiteful to adjacent cells (38, 39). Simulations were initiated with a single polymer producer (EPS+) surrounded by nonproducers (EPS–) (a) Plot of fitness of founding cells after 20 days of biofilm growth. The lineage of the focal cell (rightmost bar) benefits greatly from polymer production, whereas neighboring cells are suffocated and have reduced fitness. Fitness is calculated as the total number of cells that result from a focal cell in the mixed biofilm, and it is shown here as relative to a cell in a biofilm of pure nonpolymer producers (EPS–; dotted line). (b) Polymer producers are typically very successful in the mixed biofilms. (c) In a minority of cases, the polymer producers are smothered by nonproducers, which explains the high variance in the fitness of the focal polymer-producing cell (a). (d) Polymer production in biofilm has a strong analogy with growth in plants, where competition for light favors vertical growth.

Strong local competition can prevent altruism among relatives (33). However, the upward expansion of the biofilm reduces local vertical and horizontal competition for space within a lineage, and it favors their cooperation. There is strong lateral competition at biofilm initiation, however, which can be seen by the reduced fitness of cells lying horizontal to the polymer-producing lineage (Fig. 5). For these cells, polymer production can be considered spiteful: the focal cell lowers its reproductive rate to produce polymer that reduces the fitness of the lateral neighboring cells (38, 39). The extracellular polymer, therefore, provides a competitive advantage to a lineage by allowing its cells to rise up and over other cells and suffocate them. This suffocation effect also explains the frequency-dependent nature of the advantage, whereby polymer producers invade most easily in biofilms containing many nonproducers (Fig. 4). As the frequency of polymer producers increases in a biofilm, they have less opportunity to overgrow other lineages (increased competition for oxygen and space), which reduces the benefit of polymer production (compare Figs. 2g and 5b).

	Conclusions

Top Abstract Results and Discussion Conclusions Methods Acknowledgements References

 
Cooperative and altruistic adaptations present a significant problem for evolutionary biology because theory predicts that selection for selfishness and cheating should often undermine group behaviors (6, 18, 40, 41). Microbial biofilms are widely viewed as an example of this problem (5–8, 10, 42, 43) because the production of EPS by one cell that can be used by another would seem to be an exploitable resource. By using a simple model of mixed-strain biofilms that incorporates realistic diffusion–reaction effects, here we show that a strong advantage to polymer production arises as an emergent property (44). Secretion of extracellular polymers by a cell allows it altruistically to push descendents into a more oxygen-rich environment. At the same time, it provides a strong competitive advantage at the scale of the cell lineage by suffocating neighboring nonproducers. The effect of polymer production, therefore, has a strong analogy in plants competing for light, where vertical growth and increased foliage area selfishly increase access to light at the expense of competitors (45). The polymer-producing cells that initiate a biofilm are analogous to a tree trunk that allows descendent cells to raise up and outward into the best growth conditions and overgrow the rest (Fig. 5).

Although phrased in terms of oxygen gradients, comparable results can be expected whenever the biofilm forms a barrier to a limiting resource, and an analogous process may also occur in the initiation of biofilms that float on the surface of liquids (14). Our simulations suggest that cells must secrete low-density polymers to gain an advantage. We are unaware of any empirical estimates of extracellular polymer density; but for the values assumed in previous simulations (26, 31, 46, 47), polymer producers would readily invade (_X/_EPS = 6; Fig. 4). Another important point is that the advantage to polymer production increases with biofilm age (Fig. 2h). Our model, therefore, predicts that polymer production is most likely to be favored when biofilms last for several days. Finally, polymer production is not expected to increase indefinitely. Modeling the evolution of polymer production as a continuous trait predicts that it will stabilize at an intermediate equilibrium level (see SI Text and SI Fig. 8).

We do not wish to suggest that extracellular polymer production in biofilms will always be selected through within-biofilm competition. Clearly, under some conditions, the polymers may provide global benefits that help both the lineage that produces it and others in the biofilm, such as protection against antimicrobials or desiccation. Nevertheless, our model shows that one should not uncritically assume that biofilms with their matrix of secreted polymers are purely cooperative. These polymers may often provide competitive benefits to lineages by allowing them to suffocate unrelated cells of their own or other species (26).

Why is it important to know whether polymer production requires global cooperation within biofilms? The fitness effects of a trait define how it responds to changing social conditions over ecological and evolutionary time (6). For example, the predicted effect of mixing strains together is reversed between cooperative and competitive traits (7, 48, 49). The standard assumption that extracellular polymers are purely cooperative predicts that the presence of multiple strains will decrease the matrix and, potentially, antimicrobial resistance (7). Our model predicts the opposite: that mixed-strain biofilms will tend to have increased polymer production. General support for this prediction comes from the recent discovery that mixing genetically different strains of the bacterium Pseudomonas aeruginosa results in more robust biofilms (E. Martinez-Garcia, R. Kolter, and K.R.F., unpublished data). The "cooperative" behavior of biofilm-forming bacteria may not be so cooperative after all.

	Methods

Top Abstract Results and Discussion Conclusions Methods Acknowledgements References

 
The individual-based approach used for simulations is a multiagent description of biofilm dynamics where agents (cells) behave independently according to rules mimicking the behavior of a bacterial cell, including growth, division, and polymer production and excretion (26–28). The beginning of each simulation starts with cells adhered to a surface. These cells then grow in a two-dimensional computational space where movement occurs through shoving of neighboring cells, which do not overlap. The dynamics of the biofilm community is emergent from the interactions at the cell scale. Cell growth and polymer production rates are strain-specific following the equations defined in Table 2. The effects of local nutrient concentrations are included in the simulation, which are computed by solving partial differential equations describing diffusion–reaction at each step of the simulation. For an extended description of the model, see SI Text.

	Acknowledgements

Top Abstract Results and Discussion Conclusions Methods Acknowledgements References

 
We thank Angus Buckling, Ashlee Earl, Esteban Martinez Garcia, Joan Strassmann, Stuart West, and two anonymous referees for thoughtful comments. This work was supported by National Institute of General Medical Sciences Center of Excellence Grant 5P50 GM 068763-01 (to K.R.F.).

	Footnotes

 

Abbreviations: EPS, extracellular polymeric substances; EPS+, EPS-producing strain; EPS–, non-EPS-producing strain.

*To whom correspondence should be addressed. E-mail: kfoster{at}cgr.harvard.edu

Author contributions: J.B.X. and K.R.F. designed research; J.B.X. performed research; J.B.X. analyzed data; and J.B.X. and K.R.F. wrote the paper.

The authors declare no conflict of interest.

This article is a PNAS direct submission.

This article contains supporting information online at www.pnas.org/cgi/content/full/0607651104/DC1.

© 2007 by The National Academy of Sciences of the USA

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Top Abstract Results and Discussion Conclusions Methods Acknowledgements References

 

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