Abstract
Microbial populations often assemble in dense populations in which proliferating individuals exert mechanical forces on the nearby cells. Here, we use yeast strains whose doubling times depend differently on temperature to show that physical interactions among cells affect the competition between different genotypes in growing yeast colonies. Our experiments demonstrate that these physical interactions have two related effects: they cause the prolonged survival of slower-growing strains at the actively-growing frontier of the colony and cause faster-growing strains to increase their frequency more slowly than expected in the absence of physical interactions. These effects also promote the survival of slower-growing strains and the maintenance of genetic diversity in colonies grown in time-varying environments. A continuum model inspired by overdamped hydrodynamics reproduces the experiments and predicts that the strength of natural selection depends on the width of the actively-growing layer at the colony frontier. We verify these predictions experimentally. The reduced power of natural selection observed here may favor the maintenance of drug-resistant cells in microbial populations and could explain the apparent neutrality of inter-clone competition within tumors.
Significance Statement Microbes often live in dense populations such as colonies and biofilms. We show that the success and extinction of yeast strains within a growing colony are determined by a combination of their relative fitness and the forces exerted by proliferating cells on their neighbors. These physical interactions prolong the survival of less-fit strains at the growing frontier of the colony and slow down the colony’s takeover by fitter strains. This reduction in the power of natural selection favors the maintenance of genetic diversity in environments in which the strains’ relative growth rates vary with time. Growth-induced physical interactions may thus favor the maintenance of drug-resistant cells, which are typically less-fit than non-resistant cells, within dense microbial populations.
Author contributions
A.G., D.R.N., A.W.M. designed the research and wrote the paper, A.G. performed the research and analyzed the data.
Introduction
Life in the microbial world often occurs in crowded environments, such as colonies, biofilms, and tissues. Within such dense populations, cells compete for nutrients and space to survive, proliferate, and propagate their genotype to future generations. Classical results of population genetics theory on the competition between different genotypes in well-mixed populations (1) do not apply directly to these microbial aggregates, due to their growing size and spatial structure (2-9). Microbial range expansion experiments are a valuable tool for investigating ecological and evolutionary dynamics in spatial contexts (4, 5, 10-15) and extend our understanding of spatial population genetics (16). Early studies of microbial range expansions have shown that the growth of microbial colonies causes the spatial separation of genotypes (2), which makes theoretical models derived for well-mixed populations inapplicable. Biological interactions between genotypes can either reduce this segregation or increase it, depending on the nature of the interactions. For instance, Müller et al. (10) showed that mutualistic yeast strains cannot de-mix if they are obligate mutualists and thus depend on each other for growth. In contrast, McNally et al. (17) showed that antagonistic interactions among bacterial strains cause a phase separation that further increases the spatial separation of different strains. Although additional deviations from classical theory could be produced by the mechanical interaction between cells in dense populations, the effects of such interactions on microbial competition is still relatively unexplored. Among the few exceptions, Farrell et al. (18) showed that the physical properties of a cell can affect the dynamics of beneficial mutations in growing microbial colonies. They showed that the probability that a mutant spreads in the population can be related to summary statistics characterizing cell alignment and the roughness of the expanding front. In parallel to our investigation, Kayser et al. (19) showed that the mechanical interaction between a faster-growing and a slower-growing strain can cause the prolonged survival of the slower-growing one at the colony frontier, a process that we have investigated in a different geometry and from a different modeling perspective.
In this work, we study the effect of mechanical interactions among cells on the competition of strains in growing colonies of the budding yeast, Saccharomyces cerevisiae. We focus on the competition for space and for nutrients of two yeast strains with different fitnesses and study the dynamics of selective sweeps (the fitter strain’s increase in relative frequency at the frontier of the expanding colony) and the local extinction dynamics of the less-fit strain. In S. cerevisiae colonies, growth occurs mostly in close proximity to the outer boundary, and so we consider a strain to be extinct if it lags behind during the expansion and thus exits the growth zone. We find that mechanical interactions reduce the strength of natural selection by slowing down the extinction of slower-growing strains and by reducing the rate at which faster-growing ones increase their frequency within a population. We show that a continuum model inspired by overdamped hydrodynamics can reproduce the experimental data and make new predictions that we verify experimentally. Specifically, the model predicts that the speed at which selective sweeps spread in a growing colony is inversely related to the width of the actively growing layer at the colony frontier. We tested the model by co-culturing two yeast strains with different temperature-dependent growth profiles. We show that the prolonged survival of the less-fit strain, which occurs via the formation of thin, persistent filaments (Fig. 1A-A2), promotes the maintenance of genetic diversity in the population when two strains compete in an environment in which their relative growth rates vary with time. This reduction in the efficiency of natural selection may be beneficial for microbial populations by delaying the extinction of slower-growing genotypes which carry traits that can later be beneficial for the population, such as resistance to antimicrobial drugs.
Results
When two yeast strains are mixed and inoculated as a drop on a solid nutrient medium, they form a mixed-strain colony that expands radially with time. A well-known feature of such colony expansion is the spatial de-mixing of strains due to genetic drift (2), which forms single-strain sectors. When one strain expands faster than the other, the size of its sectors increases with time (5) (Fig. 1A). We performed colony-growth experiments using two S. cerevisiae strains with different doubling times. As expected, single-strain colonies of the strain (yAG2) with the larger growth rate (, median±SD) expanded faster than single-strain colonies of the strain (yAG1) with the smaller growth rate (, median±SD). We found that single-strain sectors within mixed colonies interact mechanically in ways that affect the competition between the two strains. These mechanical interactions are visible in Fig. 1A. At each side of sweeping sectors of the faster-growing (yellow) strain, the slower-growing (blue) strain was displaced and pulled towards the exterior of the colony (Fig. 1A-A1). Occasionally, the slower-growing strain was trapped between two sectors of the faster-growing one in the early phases of the expansion and traveled longer distances (blue filaments in Fig. 1A-A2) than in other regions of the colony, where the slower-growing strain was farther from the faster-growing strain. The enhanced expansion of the slower-growing strain occurs as a thin, persistent filament (composed of several thousand cells, not to be confused with bacterial filamentous cells) that originates via a combination of cell division and the physical interactions with the faster-growing strain, the most prominent of which is the pressure exerted by proliferating cells on their neighbors.
We wanted to rule out the possibility that persistent filaments were due to the ability of the faster-growing strain to speed up (for example, via chemical secretions) the proliferation of cells of the slower-growing strain that were nearby. We therefore produced mixed colonies from two strains: a wild-type strain that proliferated at temperatures from 20 to 37°C (yAG19, cyan in Fig. 1B-C) and a strain carrying a temperature-sensitive mutation that could only proliferate at temperatures below 30°C (yAG20, magenta in Fig. 1B-C). To ask if the formation of persistent filaments required the proliferation of the less-fit strain, we imposed the extreme condition of preventing the proliferation of the less fit strain. The heat-sensitive strain used here is a cdc26Δ mutant that arrests in mitosis and therefore cannot complete the cell division cycle at temperatures above 30°C (20). We grew single-strain and mixed-strain colonies of these two strains at 28°C for two days and subsequently imaged them with a stereoscope incubated at 37°C for 23 h. We observed that single-strain, heat-sensitive colonies stopped expanding after 9 h from the start of the measurement (Figs. 1B and S1). In the following hours, single-strain sectors of the non-heat-sensitive strain emerged from the mixed colony, displacing the heat-sensitive strain and producing patterns (Fig. 1C-C1) that are visually similar to those shown in Fig. 1A. Specifically, the non-dividing heat-sensitive strain was nevertheless displaced on each side of sweeping sectors of the non-heat-sensitive one and sectors of the heat-sensitive strain trapped between two sectors of the other strain (Figs. 1C1, S2 and Movie S1) were squeezed and formed filaments that resemble those shown in Fig. 1A-A2. Because the heat-sensitive single-strain colonies were not expanding when non-heat-sensitive sectors emerged from the mixed-strain colony (Fig. S1D), the displacement of the heat-sensitive strain was caused by the physical interaction between the two strains and the formation of thin filaments did not require the proliferation of the less fit strain.
The experiments described above show that mechanical interactions cause the prolonged survival of the slower-growing strain in mixed-strain colonies, via thin, persistent filaments trapped between sweeping sectors of the faster-growing strain. To highlight the effect of this persistence on the competitive dynamics of strains in growing colonies, we designed a colony-growth experiment in which we could use environmental switches to alternate which strains grew faster and slower. The strain yAG2 is cold-sensitive due to the trp1-1 mutation, which requires it to import tryptophan from the medium, a process whose efficiency is reduced at lower temperatures (21), so that yAG1 grows faster than yAG2 at low temperatures and more slowly at high temperatures. At 12°C, single-strain colonies of yAG1 expanded faster (0.288±0.004 mm/d) than those of yAG2 (0.226±0.010 mm/d), whereas at 30°C single-strain colonies of yAG2 expanded faster (1.15±0.02 mm/d) than those of yAG1 (0.96±0.03 mm/d). Thus, by changing the temperature during a mixed-strain colony growth experiment, we could control which strain was proliferating faster. We performed mixed-strain colony growth experiments starting from a 50%-50% mixture of yAG1 and yAG2 and incubated these colonies at 30°C at the start of the experiment, then moved the colonies to 12°C after a few days, and moved them again to 30°C towards the end of the experiment (Methods). The duration of each temperature phase varied between different replicates. Fig. 2 and Figs. S3-S5 show that strains can survive as persistent, thin filaments at the temperature where they grow slower and then expand in the next phase, at a temperature where they grow faster than their competitor.
We made a hydrodynamic model to describe the observed interactions between strains at the macroscopic scale (i.e., at scales much larger than the typical cell diameter). Our model for the dynamics of the competition between two strains in growing colonies used a two-dimensional continuum description based on overdamped hydrodynamics. This approach is valid on time scales that are long compared to a cell division time and length scales that are large compared to a cell diameter and to the colony height near the frontier. We first describe the model for a single-strain colony and then generalize it to the case of multiple strains. Let ρ(x,y,t) be the two-dimensional density (with dimensions of cells/length2) of a single-strain colony at time t, where x and y are cartesian coordinates on the agar plane. If h is the height of the colony, we have ρ = hρ3d, where we assume that the three-dimensional density ρ3d (with dimensions of cells/length3) is constant within the colony. Colony expansion in the vertical direction is much slower than the expansion in the horizontal plane of the agar and thus experimental colonies are approximately flat in the direction parallel to the agar surface. We therefore assume that h (and thus ρ) is also constant within the colony, and equal to zero outside. Let g(x,y,t) be the local growth rate (with dimensions of 1/time) of yeast cells in position (x,y) at time t. Experimental observations reveal that the two-dimensional spatial distribution of strains in mixed-strain colonies is approximately time-invariant at distances larger than 500 μm (about 100 cell diameters) behind the colony frontier (SI section 9), indicating that cell divisions that affect the visible surface of the colony take place mostly within this distance from the frontier. This observation led us to define a distance δ from the frontier of the colony such that , with constant , for every point (x,y) inside the colony within a distance δ from the frontier at time t, and g(x,y,t) = 0 for every other point. From a hydrodynamic perspective, cell growth is seen as a source of fluid with space and time-dependent rate g. With these assumptions, the radial expansion speed of a circular single-strain colony is equal to (SI Methods), where the last approximation is justified because typically δ ≪ r in colony-growth experiments. The considerations made above translate into the following equation for the two-dimensional velocity field which displaces cells within the colony: ,where is the divergence of . Eq. 1 enforces mass conservation within the colony along a streamline, ensuring that the two-dimensional density ρ is constant inside the colony. Within the colony, the two-dimensional pressure field p(x,y,t) satisfies the equation: which states that the velocity is proportional to the pressure gradient and inversely proportional to γ, the frictional drag applied to the colony by the substrate. Eqs. 1 and 2 have been used previously to model biofilm growth (22). We show in the SI section 3 that they can be derived from the three-dimensional continuity and Navier-Stokes equations by adopting the lubrication approximation (23), which gives the value of the friction coefficient γ = 2μ/h2 in terms of the colony dynamic viscosity μ and the colony height h. The approximation is appropriate when , that is, when the height of the colony is small compared with the growth layer width, as found experimentally (, depending on the experimental setup). Upon taking the divergence of Eq. 2 and using Eq. 1, one finds: ,that is, the pressure field within the colony satisfies a Poisson equation, with the boundary condition p = p0 at the outer edge of the colony, where p0 is a constant reference pressure (because the value of p0 does not affect the dynamics, we set p0 = 0). This simple model can be generalized to mixed-strain colonies by considering two different two-dimensional densities ρ1 (x y t) and ρ (x y t), giving the density of each strain. Given the sharp boundaries between the two strains observed in colony growth experiments (see, e.g., Fig. 1A), we assume that the two strains cannot simultaneously occupy the same position in space at the same time t, so that for each point (x y) within the colony either ρ1 or ρ2 must be equal to zero, and the colony density is equal to ρ = ρ1 + ρ2. In the same way, the local growth rate is equal to g = g1 + g2 within the colony, where either g1 or g2 must be equal to zero, according to which strain occupies the position (x y) at time t. With this definition of g, the velocity field and pressure in the mixed-strain model are still given by Eqs. 2 and 3. Note that, because pressure is proportional to γ (Eq. 3) and the velocity field is given by (Eq. 2), the frictional coefficient γ drops out and its value does not affect the displacement of strains within the colony and thus its spatio-temporal dynamics. Even though growth is localized within a layer of width δ at the colony frontier, the velocity field given by Eq. 2 will in general be non-zero in the interior of the colony. However, the velocity modulus decreases sharply with the distance from the frontier and is negligible outside the growth layer (Fig. 3D), so that flow in the colony occurs mostly within the growth layer.
We find that simulations based on this continuum model can reproduce the experimental observation of the mechanical interaction of single-strain sectors within growing colonies (Fig. 3B), namely the displacement of the slower-growing strain in the proximity of a faster-growing sector and the prolonged survival and enhanced expansion speed of thin filaments of the slower-growing strain trapped between two sectors of the faster-growing one (Fig. 3B). Both these effects become more pronounced as the width, δ, of the growth layer increases. Note that the same observations are not predicted by a constant-speed model (5) inspired by geometrical optics in which each strain advances at a constant speed, perpendicular to the frontier of the colony (Fig. 3A). The constant-speed model is known to fail for the early dynamics of sweeping sectors (e.g., for sectors composed of cells with beneficial mutations), for example when the two walls bounding such sectors are close to each other (5). The temporal dynamics of a sweeping sector can be quantified by its opening angle, which is defined as the angle formed by the two lines connecting the center of the inoculum to the boundary between the two strains at the frontier of the colony (e.g., the angle ϕ in Fig. 1A). In the constant-speed model, the sector boundaries form logarithmic spirals, with their opening angle increasing logarithmically with the radius of the colony (5). In simulations of the continuum model, however, the dynamics of opening angles can be separated into two stages, which are best seen on a log-linear scale (continuous lines in Fig. 4D). Initially, opening angles increase exponentially with the radius r, defined at the point in which the two strains meet at the frontier of the colony (Fig. 4A, inset). At later times (or, equivalently, larger radii r), the rate of increase of sweeping sector opening angles versus r eventually tends to the constant-speed model prediction (Fig. 4D and Fig. S9), that is, opening angles increase logarithmically with r. We find that the continuum model results tend to the constant-speed model ones as the width of the growth layer δ tends to zero, while keeping the constant asymptotic expansion speed of each strain i constant by varying (Fig. S9). This observation makes sense because the constant-speed model, which is inspired by geometrical optics, assumes that each point at the colony frontier (corresponding to an extremely narrow growth layer) is the source of a circular growth wave in the infinitesimal time interval dt, and that the outline of the colony at time t + dt is given by the envelope of such waves (5).
We tested whether our continuum model could reproduce the observed temporal evolution of the opening angles of sweeping sectors. We performed colony growth experiments at 30°C with the slower-growing strain yAG1 and the faster-growing strain yAG2 and measured the opening angles of sweeping yAG2 sectors that remained far from each other throughout the entire experiment (e.g., the four isolated yellow sectors at 2, 8, 9 and 11 o’ clock in Fig. 1A). Opening angles measured at different times and colony radii are shown in Fig. 4A-B and Fig. S10. We grouped the experimentally-measured opening angle trajectories of sweeping yAG2 sectors into two classes (small and large angles), based on the opening angle of each sector at the second measurement point, which was taken as the initial condition for the comparison with the models (see SI section 7 for an explanation). A log-linear plot highlights the initial exponential dependence of opening angles on the distance from the center of the colony to the points at which yAG1 and yAG2 sectors meet at the frontier of the colony (Fig. 4B). The constant-speed model (dashed lines in Fig. 4A-B, based on each strain’s expansion velocity measured in single-strain colony growth experiments), strongly overestimates the initial increase in the opening angles of sweeping yAG2 sectors. We tested if our continuum model could reproduce the experiments by fitting the continuum model to the experimental opening angles of sweeping sectors. The expansion velocities and measured in single-strain colony growth experiments (SI section 8 and Fig. S11) constrained the products and in the continuum model, assuming an identical growth layer width δ for the two strains. Thus, we could vary the width δ of the growth layer in the model ( and were then uniquely determined) and use it as a parameter to fit the sector opening angles. The resulting model fit is shown in Fig. 4A-B (continuous lines). The best-fit estimate is δ=290 μm (68% CI [260, 350] μm). We experimentally measured the characteristic length-scale over which growth affects the visible surface of yeast colonies and found it to be equal to δexp =530±120 μm (mean±SD, see SI section 9 and Fig. S12). The best-fit estimate of δ is smaller than δexp, but this is not surprising given that the colony height goes to zero at the colony frontier, whereas the model assumes constant height everywhere (geometrical considerations suggest that δexp =2δ, see SI section 9).
The continuum model predicts that the opening angles of sweeping sectors increase faster for smaller values of δ. To test this prediction, we reduced the value of the growth layer width δ by reducing the wetness of the agar plates and measured the dynamics of the opening angles of sweeping sectors in this condition (Fig. 4C-D). We experimentally verified that the growth layer width was reduced, compared to wetter plates (SI section 9 and Fig. S12). In the experiment with a narrower growth layer width, even though the ratio of the expansion velocities of the two single strains was slightly smaller than in the experiment with wider growth layer width , the opening angles increased more rapidly, consistent with the smaller growth layer width δ, thus verifying the continuum model’s prediction. Although the constant-speed model fails to predict correctly the early time dynamics of opening angles, it does a better job than for the previous experiment, as expected given the smaller value of δ and our observation that the continuum model tends to the constant-speed model in the limit δ → 0. As in the previous experiment, our continuum model can reproduce the experimental dynamics of sweeping sector opening angles by fitting the growth layer width to the data (Fig. 4C-D, continuous lines). The best-fit parameter for this experiment is δ=110±20 μm. In this case, one can observe the transition from the exponential (for small ϕ and small r) to logarithmic dependence of ϕ on r predicted by our continuum model (Fig. 4C-D). Such a transition is not discernible (or barely so) in the experiment described in the previous paragraph (Fig. 4A-B), due to the larger value of the growth layer width δ for wetter plates. In both experiments, the ratio matches the ratio of experimentally-measured growth rates (, mean±SE), as expected based on the model prediction for the asymptotic expansion speed .
Discussion
Our experiments show that physical (pressure-induced) interactions between yeast strains within growing colonies reduce the efficiency of natural selection both by allowing less fit strains to persist and by slowing down the expansion of fitter strains. Slower-growing strains expand faster in parts of the colony that are close to faster-growing strains. When a slower-growing strain is trapped in a thin gap between two sectors of the faster-growing one, it expands at almost the same speed as the latter and forms a persistent, thin filament that can survive for very long times. A geometrical, toy model which neglects the contribution of curvature to the front propagation velocity (SI section 10) suggests that the thickness of these filaments decreases exponentially over a typical length scale , which increases with increasing growth layer width δ and the ratio . In the experiments, we found that thin filaments can persist longer than initially-larger sectors of the slower-growing strain, which are usually pinched off by sectors of the faster-growing strain that meet each other at the frontier of the colony subtending a substantial angle (SI section 11 and Fig. S15). The prolonged survival of thin, persistent filaments is favored by the small fluctuations of the filament boundaries relative to the filament thickness (SI section 12 and Fig. S16). Physical interactions also slow the initial dynamics of selective sweeps compared to the expectation of the constant-speed model, which assumes that the strains expand independently of each other except that two strains cannot occupy the same position. The magnitude of these effects increases with the width δ of the actively-growing layer at the frontier of the expanding colony. Our continuum model gives us an intuition for the physical origin of the experimental observations. Thin, persistent filaments are pushed towards the exterior of the colony by the surrounding faster-growing strain and benefit from the pressure field generated by the latter. Conversely, sweeping sectors of the faster-growing strain that have small initial opening angles are too small to generate enough pressure and thus initially expand more slowly than the predictions of the constant-speed model. Even though our continuum model is deterministic and thus cannot reproduce the stochastic extinction of small sectors of the faster-growing strain, which are sometimes observed in the experiments (see, e.g., Fig. 1A), it helps us to understand why such extinctions can occur. Sectors of the faster-growing strain initially expand at approximately the same speed as the surrounding slower-growing strain, making the competition between the two strains almost neutral, somewhat enhancing the importance of stochastic effects. Our experiments in time-varying environments show that the existence of thin, persistent filaments can play an important role in determining the outcome of competition between strains. In environments that fluctuate between two environmental states in which each strain has a selective advantage over the other one, the persistent filaments facilitate survival during detrimental environmental states and allow immediate recovery once the relative advantage of the two strains is reversed.
Because the reduced efficiency of natural selection described here is due to physical forces acting within dense cell populations, we believe such effects are relevant for a broad range of biological systems. We expect that the observed reduction in the effective selective advantage of a fitter strain (when sector widths are small) should be relevant for beneficial mutations that arise in a colony and manage to establish a clonal sector. In the initial phase of their dynamics, such sectors will expand at approximately the same rate as the surrounding wild type cells, and the expansion speed of the beneficial mutation will increase as its sector grows wider. This size-dependent selective advantage of a fitter strain or beneficial mutation is reminiscent of positive frequency-dependent selection (24), in which the fitness of a genotype increases with its frequency in the population. In the context of our work, the frequency dependence is caused by the pressure field induced by cell division. Experimental (25) and theoretical (26) studies have shown that populations undergoing range expansion accumulate deleterious mutations as a result of consecutive founder events and genetic drift being stronger at the frontier in spatial (compared to well-mixed) populations, due to their reduced effective population sizes. Our work suggests that deleterious mutations have higher chances of being maintained in dense, expanding microbial populations than expected based on genetic drift alone, because the effects of differences in fitness are reduced by physical interactions. Our findings are relevant for the fate of drug-resistant mutations that arise in microbial colonies or biofilms. Such mutations are typically associated with fitness deficits. Our work suggests that drug-resistant mutants (e.g., antibiotic-resistant bacteria) emerging in the outer layer of an expanding colony may benefit from the physical interaction with the surrounding wild-type cells and survive for long times in the actively-dividing frontier of the colony in the absence of the drugs that they confer resistance to. The application of a drug would reverse the relative fitness of drug-resistant mutants and wild-type cells and allow the drug-resistant mutant to take over the population, similar to our experiments where temperature varies in time for temperature-sensitive strains. We thus expect that the physical interactions between different genotypes investigated here would favor the maintenance of genetic diversity within dense microbial populations and allow such populations to withstand time-dependent fluctuations of the environment or the application of antimicrobial drugs. Finally, our findings may extend beyond microbial populations and inform us about the dynamics of pre-vascular tumor growth (7, 27). Within tumors, various cell lineages compete for space and form spatially-coherent clusters that are reminiscent of the genetic de-mixing found in colony-growth experiments (28). A recent study (28) has shown that individual tumors can have high levels of genetic diversity and argued that such high-diversity levels can only be explained by non-Darwinian selection, i.e., neutral competition between different clones. The reduced efficiency of natural selection highlighted here, transposed to the three-dimensional environment at the frontier of a spherical cell cluster, is one possible mechanism to explain the apparent neutrality of inter-clone competition within such tumors.
Methods
Strains
The genotypes of all strains used in this study are reported in Table S1. In fluorescent images, yAG1 is portrayed in blue, yAG2 in yellow, yAG19 in cyan and yAG20 in magenta. Strains’ growth rates were measured by imaging time-lapse videos of micro-colonies of each strain on standard YPD agar plates at 30°C using an inverted microscope and counting the number of cells in each micro-colony at successive time points. The ratio of experimentally-measured growth rates (mean±SE) was estimated by randomly sampling micro-colonies of the two strains, computing their growth rate ratio and taking the mean across 106random samples.
Colony-growth experiments
Colony-growth experiments were conducted on 1% agarose plates with YPD (Yeast extract-Peptone-Dextrose) medium at 30°C, unless otherwise stated. Plates were poured two days before inoculation and stored at room temperature. Strains were pre-grown at 30°C overnight in liquid YPD. Before inoculation on agarose plates, 200 μL of each overnight culture were spun down for 1 min at 9400 g and re-suspended in 1 mL of 1% PBS (Phosphate-Buffered saline). The densities of such suspensions were measured with a Coulter Counter and brought to a density of 3·107cells/mL by adding 1% PBS or removing the supernatant in appropriate amounts. If required, suspensions were mixed in the desired ratios. A 0.6 μL droplet was pipetted on each agarose plate.
Sweeping sectors dynamics experiment
We performed two sets of experiments to measure the dynamics of sweeping yAG2 sectors at different growth layer widths at 30°C. For the wide growth layer experiment, we poured 7 mL YPD 1% agarose medium into 35 mm Petri dishes. After one day from pouring, solidified YPD agarose discs were transferred to 100 mm Petri dishes, three discs for each larger dish. One droplet of either a single-strain or a mixed-strain suspension (yAG1 and yAG2 were at a 99%-1% frequency) was inoculated on the surface of each disc. 7 mL of liquid YPD medium were added to the Petri dish and substituted daily to ensure that nutrients did not become depleted. Colonies were imaged twice per day with a Zeiss Lumar stereoscope. For the narrow growth layer, we poured 33 mL YPD 1% agarose medium into 100 mm Petri dishes. One droplet of either a single-strain or a mixed-strain suspension (yAG1 and yAG2 were at a 99%-1% frequency) was inoculated on the surface of each plate. Colonies were imaged once per day with a Zeiss Lumar stereoscope.
Radial expansion velocities
Single-strain colony radii were measured by fitting circles to each single-strain colony bright-field image. Radial expansion velocities were computed by fitting the radius-vs-time data to straight lines, separately for each colony. The mean radial expansion velocity of each strain was computed as the mean slope of the radius-vs-time fits. For the wide growth layer experiment, yAG1 and yAG2 expansion velocities were measured across 10 and 9 single-strain colonies, respectively. The mean radii at different times are shown in Fig. S11A. The measured velocities were (mean±SD) and (mean±SD). For the narrow growth layer experiment, yAG1 and yAG2 expansion velocities were measured across 11 single-strain colonies for each strain. The mean radii at different times are shown in Fig. S11C. The measured velocities were (mean±SD).and (mean±SD).
cdc26Δ mutant experiments
We performed colony-growth experiments with the strains yAG19 and yAG20 to show that filaments and strain displacements can occur without proliferation of the less-fit strain. These experiments were done with 100 mm Petri dishes filled with 33 ml of 1% agarose YPD medium. We grew single-strain and mixed-strain colonies of yAG19 and yAG20 (yAG19 and yAG20 were at a 5%-95% frequency) for two days at 28°C and then moved them to the stage of a stereoscope incubated at 37°C. Colonies were imaged every 10 min for 23 h. The same experiment was performed with yAG2 and yAG20 single-strain and mixed-strain colonies and the results do not differ qualitatively.
Time-varying temperature experiments
We performed time-varying temperature experiments with 100 mm Petri dishes filled with 33 mL of 1% agarose YPD medium. We inoculated 11 plates with a mixed-strain 0.6 μL droplet (yAG1 and yAG2 were at a 50%-50% frequency). Three of these plates were incubated at 30°C for 2 days, then at 12°C for 9 days and then at 30°C for 14 days (Fig. S3). Three plates were incubated at 30°C for 3 days, then at 12°C for 16 days and then at 30°C for 10 days (Fig. 2A-C and Fig. S4). Three plates were incubated at 30°C for 3 days, then at 12°C for 20 days and then at 30°C for 9 days (Fig. S5). One plate was incubated at 30°C for 13 days and then at 12°C for 18 days (Fig. 2D-L). We inoculated 6 plates with a 0.6 μL droplet of yAG1 and other 6 with yAG2. Three of each strain’s plates were stored at room temperature overnight and then moved to a 12°C incubator for the rest of the experiment. The remaining three plates for each strain were placed in a 30°C incubator for the entire experiment. We took frequent fluorescent and bright-field images of all plates. Single-strain colonies were used to measure single-strain radial expansion velocities.
Acknowledgements
AG thanks Sauro Succi for helpful discussions on the numerical integration of the continuum model and the Harvard Center for Biological Imaging and Douglas Richardson for helping with the growth rates measurement on agar plates. We thank the members of the AWM and DRN groups for valuable suggestions. AG was supported by research fellowships from the Swiss National Science Foundation, projects P2ELP2_168498 and P400PB_180823, and work on this project was supported by the Human Frontier Science Program Grant RGP0041/2014 to AWM and DRN. Work by AG and DRN was supported by the National Science Foundation, through grants DMR1608501 and via the Harvard Materials Science Research and Engineering Center via grant DMR1435999.
Author contributions
A.G., D.R.N., A.W.M. designed the research and wrote the paper, A.G. performed the research and analyzed the data.