Dictyostelium AMPKα regulates aggregate size and cell-type patterning

Starved Dictyostelium cells aggregate into groups of nearly 105 cells. AMPK is a highly conserved serine/threonine protein kinase consisting of a catalytic and two regulatory subunits. As multi-cellular development in Dictyostelium is initiated upon starvation, we explored the role of the energy sensor, AMPK, which shows significant similarity to human AMPK and is expressed throughout development. Deletion of the ampkα gene results in the formation of numerous small-sized aggregates that develop asynchronously to form few fruiting bodies with small sori and long stalks. On the other hand, ampkαOE cells form fruiting bodies with small stalks and large sori when compared with wild-type, Ax2. A minimum of 5% ampkα− cells in a chimaera with Ax2 cells was sufficient to reduce the aggregate size. Also, the conditioned media collected from ampkα− cells triggered Ax2 cells to form smaller aggregates. The starved ampkα− cells showed low glucose levels and formed large aggregates when glucose was supplied exogenously. Interestingly, ampkα− cells exhibit abnormal cell-type patterning with increased prestalk region and a concomitant reduction of prespore region. In addition, there was a loss of distinct prestalk/prespore boundary in the slugs.


Background
AMPK (5 0 adenosine monophosphate-activated protein kinase) is a heterotrimeric serine/threonine kinase, comprising a catalytic (a) and two regulatory (b and g) subunits, and is conserved from yeast to humans. It is both a nutrient and an energy sensor that helps maintain energy homeostasis. It plays a role in the regulation of cellular as well as whole-body energy metabolism and also participates in the cell-cycle and membrane excitability regulation. AMPK coordinates control of cell growth and autophagy, acting as a metabolic checkpoint, and inhibits cellular growth via suppression of the mTORC1 (mammalian target of rapamycin complex 1) pathway. It acts as a central regulator of cell growth, cell proliferation and development [1][2][3][4][5]. When activated, AMPK promotes energy-producing catabolic pathways while inhibiting anabolic pathways, such as cell growth and proliferation. Besides its role as an energy sensor, it also plays a role in cell differentiation and development of organisms [6]. In Caenorhabditis elegans, AMPKa promotes cell survival and arrests germline development during nutrient stress [7].
In the case of Dictyostelium discoideum, the size of multi-cellular structures formed is well regulated. Dictyostelium amoeba divides mitotically when food is abundant, but undergoes multi-cellular development upon starvation. Vegetative cells secrete prestarvation factor (PSF) that helps monitor cell density relative to the amount of available nutrients [8]. High PSF induces the expression of genes required for aggregation. When the food supply is depleted, PSF production declines and another cell density sensing factor called conditioned medium factor (CMF) begins to accumulate. Once the starving cells reach high cell density, CMF accumulates and the cells initiate aggregation via cAMP signal relay [9] to aggregate into groups of approximately 10 5 cells. Hohl & Raper [10] had earlier investigated several small-sized aggregate mutants and found them to be defective in either aggregation or cell number or mass sensing. It was observed that mutants defective in aggregation could be rescued by crowding of the cells, so that aggregation becomes unnecessary. The cell number sensor senses the number of cells present in a group, and if they are exceedingly high it breaks them into smaller groups. Earlier, Brock & Gomer [11] observed the smlA mutants that formed small-sized aggregates, due to the oversecretion of Countin A protein. The aggregates then form the migratory slugs where the anterior quarter region is composed of prestalk cells and the remaining posterior region of prespore cells. The ratio of the cell types remains constant regardless of the size of the multi-cellular structures formed. Prestalk cells are further divided into subtypes: pstA cells occupy the anterior 10% of the slug, pstAB cells occupy the core to the tip, pstO cells are found behind the pstA cells and anterior-like cells (ALCs) lie dispersed within the prespore region [12]. A number of genes play a role in cell-type proportioning and spatial patterning [13][14][15][16], thus there is a large selective pressure on the starved cells to form fruiting bodies for proper spore dispersal. Neither too long nor too short fruiting bodies are advantageous for the organism. A fruiting body is composed of two terminally differentiated cell types, namely the stalk (dead vacuolated) cells and the spore (viable) cells [17].
AMPK plays an important role in starvation responses and nutrient deprivation is necessary for the initiation of development in this organism. Earlier, Bokko et al. [18] investigated the role of AMPK in mitochondrial diseases and found overexpression to result in fruiting bodies with short, thick stalks and comparatively large sori, while antisense inhibition developed fewer and smaller fruiting bodies.
This study was undertaken to explore the functions of AMPKa during development of D. discoideum, which was found to be involved in regulating the aggregate size. The ampka 2 cells formed small-sized aggregates, which developed asynchronously and the spores formed displayed reduced viability. The developmental defects shown by ampka 2 cells were cell autonomous as chimaeras formed with only 5% ampka 2 mixed with 95% Ax2 cells caused the aggregation streams to break up. The conditioned medium (CM) collected from ampka 2 cells caused the Ax2 cells to form small-sized aggregates. The ampka 2 cells showed low cytosolic glucose levels during starvation and the small-aggregate phenotype could be corrected to a certain extent when developed in the presence of exogenous glucose. In chimaeras with Ax2 cells, the ampka 2 cells showed a propensity towards the prestalk region and had lower tendency to form spores. Importantly, our results showed AMPKa to play a regulatory role in the spatial cell-type patterning as mutation caused an increase and mis-localization of the prestalk cells and a decrease in the prespore cells, ultimately resulting in fruiting bodies with small sorus and long stalk.

ampka mRNA is expressed in prestalk/stalk cells
To determine the spatio-temporal mRNA expression patterns of ampka, reverse transcriptase PCR (RT-PCR) and in situ hybridization analyses were performed. The ampka transcript was present during growth and development, showing minimum levels in the vegetative cells and increased levels during multi-cellular development (figure 1a,b). It remained more or less constant during later stages of development. The whole mount in situ hybridization analyses showed ampka transcript to be localized in the tip of the mound and at the site of contact with the substratum corresponding to the prestalk cells (figure 1c(A)). As development proceeded towards culmination, the transcript was localized in the pstAB cells, stalk tube and the basal disc region (figure 1c(B-E)). The high expression levels in the basal disc suggest it to be present largely in the pstB cells as they are shed off during culmination. The sense probe did not show any evident staining (figure 1c(A 0 -E 0 )).
In conclusion, ampka transcript shows prestalk localization and is expressed throughout growth and development.

Successful creation of ampka mutants
To investigate the functions of AMPKa, we successfully made both overexpressing and deletion mutants (electronic supplementary material, figures S1 and S2). The constitutive promoter, actin 15, was used to drive the expression of the fusion protein AMPKa-Eyfp and was called AMPKa overexpressor (ampka OE ). Following transformation and blasticidin selection, 500 independent clones were isolated and screened rsob.royalsocietypublishing.org Open Biol. 7: 170055 for positional integration by PCR amplification of the genomic DNA. Four positive clones of ampka null were obtained having similar growth and development patterns. One of these clones, designated as ampka 2 , was used for further studies. Rescue (ampka Res ) was created by expressing the AMPKa fusion protein in ampka 2 cells. The growth and early developmental defects shown by ampka 2 were more or less rescued in ampka Res cells.

AMPKa suppresses cell proliferation and growth
To measure the rate of cell proliferation in liquid culture, Ax2, ampka OE , ampka 2 and ampka Res log phase cells were identically diluted into fresh media at a density of approximately 5Â10 5 cells ml 21 and monitored over several days. Ax2 cells reached stationary phase at 12.8 Â 10 6 cells ml 21 and cell proliferation of ampka OE cells was consistently lower when compared with all other strains and displayed a decline phase after 108 h. ampka OE cells proliferated more slowly, reaching stationary phase tardily and at a much lower density of approximately 9. In the case of D. discoideum, cell proliferation (increase in the number of cells) and cell growth (increase in cell mass or size) are regulated independently. To determine the role of AMPKa in regulating growth, we measured the cell mass of Ax2, ampka OE , ampka 2 and ampka Res cells. The average cell mass of Ax2 cells was 10.3 + 0.2 mg and comparable to that observed previously [19]. The average cell mass of ampka OE , ampka 2 and ampka Res cells were 8.5 + 0.3, 12.3 + 0.3 and 11.1 + 0.2 mg, respectively. Change in the average cell mass of ampka Res was insignificant compared with Ax2 cells (figure 2b). To determine if AMPKa affects cell size, flow cytometry analyses were performed. Figure 2c shows ampka 2 cells to be larger in size, whereas ampka OE cells were smaller when compared with Ax2 cells. ampka Res cells exhibited similar cell size as Ax2 cells. Taken together, the data suggest that AMPKa regulates both cell proliferation and growth of vegetative cells.

Disruption of ampka gene results in small-sized aggregates, asynchronous development and reduced spore viability
To examine the role of AMPKa in multi-cellular development, we plated cells from the various strains at equal densities (5 Â 10 7 cells ml 21 ) on non-nutrient agar plates and allowed them to develop after synchronization. Ax2 cells completed their development by forming aggregation territories (mounds) by 12 h, slugs at 16 h and finally culminate into fruiting bodies at 24 h. ampka 2 cells developed into smaller aggregates and, subsequently, not all aggregates pursued further development, with only few of them proceeding towards slug formation. Following that, not all slugs proceeded to early culminant at the same time, further added more asynchrony. Thus, the development of ampka 2 cells appeared highly asynchronous, showing various developmental intermediates (aborted mound, slugs, early culminant and culminant) when compared with the Ax2 cells by 24 h of development (figure 2d). The fruiting bodies formed by ampka 2 had smaller sori (spore heads) and longer stalks when compared with the Ax2 cells. In fact most of the fruiting bodies formed by ampka 2 cells collapsed, which could be attributed to the longer stalks formed (figure 2d). By contrast, the fruiting   rsob.royalsocietypublishing.org Open Biol. 7: 170055 bodies formed by ampka OE cells showed large sori and short stalks when compared with the Ax2 cells (figure 2e). As only few fruiting bodies were formed by ampka 2 cells, we checked the viability of the spores. The average viability of Ax2 spores was 84 + 1.4% [20,21], of ampka OE spores was 71 + 2.8% and of ampka 2 spores was significantly reduced to 45 + 1.8% (figure 2f ). The reduced spore viability of ampka 2 was rescued in the ampka Res , which displayed average spore viability of 78 + 4.2% (figure 2f ).
The early developmental defects (small-sized aggregates) shown by ampka 2 were rescued by the exogenous expression of AMPKa, but the late developmental defects (asynchronous development) were still apparent. The ampka 2 cells formed smaller (approx. 3.4-fold decrease) and comparatively more (approx. 1.8-fold increase) aggregation territories than Ax2 cells (figure 3a-d).
The above data suggest that an optimum level of AMPKa is necessary for proper development.

ampka 2 cells exhibit changes in secreted factors
To investigate the role of secreted factors in the development of ampka 2 phenotype (small-sized aggregates), we performed cell mixing experiments with the Ax2 cells in varying proportions (5-90%) and allowed them to develop. The Ax2 cells in the chimaeras formed were not able to rescue the phenotypic defects caused by ampka 2 cells, suggesting that the small-sized aggregate phenotype was not due to the lack of secreted factor(s). However, with only 5% addition of ampka 2 cells to 95% Ax2 cells, there was a significant increase in aggregate numbers and decrease in aggregate size when compared with Ax2 cells alone (figure 4a; electronic supplementary material, figure S3a,b). The size of the aggregates in these cell mixtures was indistinguishable from size of those formed by ampka 2 cells alone (figure 4a). The size and number of aggregates formed by Ax2 cells were affected by addition of only 5% mutant cells, thus it is possible that mutant cells secrete some factors that regulate group size. rsob.royalsocietypublishing.org Open Biol. 7: 170055 cell-adhesion proteins expressed during early development of Dictyostelium are Gp24 and Gp80. High expression levels of gp24 were observed in countin 2 cells, whereas gp80 expression levels were not significantly altered during early development [22]. The mRNA expression of cadA (gp24) was significantly decreased from streaming onwards in developing ampka 2 cells resulting in decreased cell-cell adhesion, and subsequently resulting in the formation of small-sized aggregates (figure 5b). Overexpression of the Gp80 celladhesion protein, which causes aggregation streams to break up [23], was significantly increased at the mRNA level from mound onwards in the developing ampka 2 cells, suggesting the possible reason for the break-up of streaming cells to result in small-sized aggregates (figure 5c).

Starving ampka 2 cells show low glucose levels
CF appears to regulate cytosolic glucose levels and these in turn affect cell adhesion, suggesting that glucose levels are a part of the Countin signal transduction pathway [24]. In other words, glucose affects the group size in Dictyostelium and is the downstream target of CF. Adding glucose exogenously negates the effect of high extracellular CF on aggregate size and mimics the effect of depletion of CF. When Ax2 cells were allowed to  rsob.royalsocietypublishing.org Open Biol. 7: 170055 develop on non-nutrient agar plates containing 5 mM glucose [25], it resulted in the formation of large-sized aggregates ( figure 6a, upper panel). In our studies, we too found 5 mM of glucose to be the best concentration (data not shown). Our earlier results showed high countin expression in the ampka 2 cells; thus, it was possible that the CF could repress the internal glucose levels in these cells. When ampka 2 cells were allowed to develop in the presence of 5 mM glucose, we observed large aggregates, but the size was still comparable to Ax2 (figure 6a, lower panel; electronic supplementary material, figure S4a,b). Therefore, we measured the cytosolic glucose levels in both the vegetative and starved cells. Cytosolic glucose levels in the vegetative cells of Ax2 (31.26 + 1.8 nmol mg 21 protein) and ampka 2 (27.59 + 2.8 nmol mg 21 protein) were not significantly altered, but the starved ampka 2 cells showed low glucose levels (6.98 + 0.39 nmol mg 21 protein) when compared with the Ax2 cells (11.2 + 0.18 nmol mg 21 protein) (figure 6b). Taken together, the data show increased countin expression and low glucose levels in the starved ampka 2 cells to be responsible for regulating the aggregate size.

AMPKa regulates spatial cell-type patterning
As aberrant fruiting bodies were made by ampka 2 cells, we were interested in elucidating the role of AMPKa in regulating cell-type differentiation ( figure 7). We monitored mRNA levels of the cell-type-specific marker genes during development of both Ax2 and ampka 2 cells. Expression levels of the prestalk-specific genes, ecmA and ecmB, were significantly increased in the ampka 2 cells (electronic supplementary material, figure S5a,b) while the expression level of the prespore-specific gene, pspA (electronic supplementary material, figure S5c), was reduced when compared with the Ax2 cells.
We attribute these differences to the formation of fruiting bodies with long stalks and small sori by the ampka 2 cells. We substantiated our results by examining the spatial celltype patterning using cell-type-specific promoters fused to the lacZ reporter in both the Ax2 and ampka 2 cells. We found an increase in the staining region and/or mis-localization of prestalk-specific genes during the development of ampka 2 cells ( figure 7a-d), while the prespore-specific gene, pspA, staining region was reduced (figure 7e). The spatial distributions of prestalk-and prespore-specific genes were compared in the Ax2 and ampka 2 developmental structures (figure 7a-e). In the ampka 2 mound, the spatial distribution of ecmA/lacZ was aberrant, as it was dispersed all over the mound (figure 7b(E 0 )) rather than only at the tips as in the case of the Ax2 mound ( figure 7b(E)). The spatial localization of ecmB/lacZ was also strikingly aberrant as it was precociously expressed in the ampka 2 loose aggregates (figure 7d(M 0 )) when compared with Ax2 (figure 7d(M)) and the staining region of pspA/lacZ was decreased in the ampka 2 mound (figure 7e(Q 0 )). The spatial localizations of these genes were also compared in the Ax2 and ampka 2 slugs. In Ax2 slugs, the spatial localization of ecmAO/lacZ was found in the anterior region and also distributed throughout the slugs (the anteriorlike cells (ALCs)) (figure 7a(B)), whereas the ecmAO/lacZ staining was expanded in the anterior region of ampka 2 slugs and also more pronounced at the rear-guard region ( figure 7a(B 0 )). The ecmA/lacZ staining displayed in the anterior region was expanded and aberrant as it was also found in the prespore region of ampka 2 slugs (figure 7b(F 0 )), and the ecmO/lacZ spatial localization was expanded in the tip region of ampka 2 migratory slugs (figure 7c(J 0 )) that normally is occupied by pstA cells in Ax2 (figure 7c(J)) but was absent in the rear-guard region (figure 7c(J 0 )). The ecmB/lacZ expression was found in the anterior region of slugs that was normally occupied by pstA cells and also the staining region was expanded in the rear-guard region ( figure 7d(N 0 )), and the pspA/lacZ staining was reduced in ampka 2 slugs (figure 7e(R 0 )).
In the ampka 2 early culminant, ecmA/lacZ expression was mis-localized as it was also found in the prespore/spore region (figure 7b(G 0 )), ecmO/lacZ was absent in the prespore/spore region and the basal disc (figure 7c(K 0 )), ecmB/ lacZ was absent in the stalk region ( figure 7d(O 0 )) and the staining region displayed by pspA/lacZ was reduced rsob.royalsocietypublishing.org Open Biol. 7: 170055 (figure 7e(S 0 )). In the ampka 2 culminant, ecmA/lacZ was also observed in the stalk (figure 7b(H 0 )), ecmO/lacZ was absent in the stalk region (figure 7c(L 0 )) and the pspA/lacZ staining region was reduced, basically found towards the posterior region of the sorus (figure 7e(T 0 )). In conclusion, we can say that the prestalk/prespore ratio was perturbed and there was a loss of distinct prestalk/prespore boundary in ampka 2 cells. Taken together, our results showed that AMPKa is involved in cell-type patterning and regulates the ratio of prestalk/prespore cells in the multi-cellular structures formed.

Developmental defects displayed by ampka 2 cells are cell autonomous
In the migratory slug, the rear-guard compartment is composed of two prestalk cell types, namely the ALCs and the pstAB-derived cells [26]. The ampka 2 cells in the chimaeras formed with Ax2 cells tend to distribute themselves in the rear-guard region of the slugs formed and in ALCs when mixed in ratios ranging from 5 to 50%, and also show lower tendency to form spores (figure 8). When the percentage of the ampka 2 cells in the chimaeras was increased to 75%, they occupied the prestalk as well as prespore regions but failed to distribute themselves at the boundary of prestalk and prespore regions. This result is consistent with the celltype-specific marker expression studies, which showed a clear loss of boundary between cell types. Furthermore, this trend also appeared in the chimaeric fruiting bodies formed, where ampka 2 cells distributed themselves largely in the posterior stalk, basal disc (derived from rear-guard cells) and the lower cup of the fruiting bodies (derived from pstO/ALCs) formed (figure 8a). Ax2 cells reduced the contribution of ampka 2 cells in chimaeric spore formation (figure 8b). Mixing of 5%, 10%, 25%, 50% and 75% of ampka 2 cells with Ax2 cells resulted in chimaeric spore formation in which ampka 2 cells contributed only to 1.22 + 0.78%, 2.8 + 0.32%, 5.8 + 0.32%, 14 + 4.15% and 44 + 9.5%, respectively (figure 8b). The Ax2 and ampka 2 cells when developed individually could form fruiting bodies on their own. Our data suggest that AMPKa is a critical component responsible for the maintenance of the prestalk/prespore ratio as well as the boundary between prestalk/prespore regions.

Discussion
During the past several years numerous studies have explored the importance of AMPK in various aspects, but still it needs to be investigated to uncover many unsolved issues. AMPK, a central regulator of metabolism, is a nutrient and energy sensor that is regulated reciprocally upon starvation by either energy or glucose [27][28][29][30]. Mammalian AMPK and its homologue present in plants and yeast are known to be activated in response to glucose depletion [31,32] and regulate expression of genes that permit growth on alternative carbon sources [33,34]. Previous findings have shown that AMPK is activated upon decrease in ATP/ADP or ATP/AMP levels [35]. The change in ATP/ADP level could be the consequence of various factors like glucose depletion, hypoxia, reactive oxygen species, etc. [29,36]. In Dictyostelium, multi-cellular development programme is initiated upon nutrient starvation and cells undergo various metabolic changes to survive and further differentiate. The major energy sources for starving cells result from the cellular degradation of RNA and protein, but glycolysis and gluconeogenesis contribute minimally [37]. We have characterized AMPKa from D. discoideum and show its involvement in the regulation of aggregate size and cell-type patterning. Dictyostelium AMPKa, like other AMPK homologues, is activated upon starvation (electronic supplementary material, figure S6), suggesting its role in nutrient sensing. The mRNA is expressed at all stages of development  rsob.royalsocietypublishing.org Open Biol. 7: 170055 and is localized in the dying cell population, suggesting it to be involved in stalk cell differentiation and also to play a role in cell differentiation.

AMPKa regulates aggregate size
One of the most interesting aspects of development is how a large number of cells organize themselves into structures of specific sizes and shapes. In this study with D. discoideum, we have identified AMPKa in regulation of aggregate size. We show the mutant ampka 2 cells to have a defect in aggregate size determination, which causes the formation of a high density of aggregates containing small numbers of cells. We found (data not shown) that when plated at higher density for development, they formed smaller aggregates, showing there is a defect in the size-determination mechanism rather than an inability to form aggregates. In fact, the defect was not limited only to the aggregate size-determination mechanism, as the mutants also showed defects in cell proliferation, development and differentiation of prespore and prestalk cells. It is known that CF (a 450 kDa complex of five proteins), a component of CM, is secreted in moderate amounts by the Ax2 cells, and regulates the number of cells present within the group and ultimately controls the size of the aggregates. Disruption of the countin gene does not allow the aggregation stream to break up, thus resulting in the formation of large aggregates and subsequently larger fruiting bodies, while oversecretion of Countin protein causes the aggregation streams to break up resulting in smaller aggregates and ultimately smaller fruiting bodies [11,38]. The small aggregates are due to an increased amount of secreted factor by the ampka 2 cells, as ampka 2 phenotype could be imitated by developing the Ax2 cells in the presence of the CM collected from the mutant cells, but it also could not be rescued by starving ampka 2 cells in the presence of Ax2 CM. The ability of 5% ampka 2 cells in a population of 95% Ax2 cells to cause the entire population to form small aggregates suggests that the mutant phenotype is not due to the lack of secreted factor. As AMPK is a serine/threonine kinase and regulates the expression of a variety of proteins, it possibly could regulate the group size by regulating countin expression which involves levels of intracellular glucose and also represses the cell-adhesion proteins. The ampka 2 cells exhibit increased countin expression, which reduces the glucose levels and exhibits aberrant cell-adhesion expression to maintain the group size. From our studies, we conclude that in wild-type cells, AMPK represses Countin and subsequently the glucose levels and cell-adhesion proteins to regulate the aggregate size ( figure 9). The ampka 2 cells developed into comparatively larger aggregates in the presence of exogenous glucose, but the size still remained comparable to wild-type. Therefore, we could say that decreased glucose levels were not the only cause of small-sized aggregates, but there may also exist some other factors that directly or indirectly regulate aggregate size. rsob.royalsocietypublishing.org Open Biol. 7: 170055 An enigmatic aspect of AMPKa is that disruption caused increase in cell growth and proliferation; thus, one would think that the absence of it is advantageous to the cell. A vital aspect of Dictyostelium development is formation of the fruiting body for maintaining its generation. The spores thus produced are a measure of one's fitness and germinate upon favourable conditions. The ampka 2 and ampka OE cells both formed aberrant fruiting bodies and the spores displayed reduced viability when compared with Ax2. Therefore, abnormally low or high levels of AMPKa reduce the ability of spores to germinate and an optimum level is necessary for efficient spore formation. The function of the fruiting body is to lift the spore mass as high off the ground as possible, for optimal spore dispersal. If the fruiting body is too large, it would collapse and the spores on the ground will not get dispersed. Therefore, there is a limit on the number of cells in the spore mass as well as in the stalk of a fruiting body. As the mutants do complete their development and form fruiting bodies, we believe that all other components required for development are below the acceptable range.

AMPKa helps maintain prestalk/prespore ratio and spatial cell-type patterning
In the case of Dictyostelium, cell differentiation is initiated when myxamoebae stop growing and dividing. During development, cells terminally differentiate into two main cell types, the stalk and the spore cells, whose precursors are prestalk and prespore, respectively, and are observed at earlier developmental stages and distinguished by marker genes. The ratio of prestalk and prespore cells remains constant regardless of the size of the slug, and any alteration in this would lead to aberrant morphogenesis and differentiation [15,39,40]. Previous reports with Dictyostelium showed cells grown in the presence of glucose (G þ cells) had increased spore-to-stalk as well as prespore-to-prestalk ratio when compared with the cells grown in glucose-depleted conditions [41,42]. The study was also supported by other groups who showed that cells when grown in the absence of glucose (G-) developed fruiting bodies with long stalks and small sori when compared with the cells grown in glucose-rich conditions, attributed to the differences in spore-to-stalk ratio [42,43]. Cell-type-specific marker expression studies in ampka 2 cells display an increase in prestalk-specific gene expression and concomitant reduction in prespore-specific gene expression, and also the spatial localization of these genes was altered. In our study, we found that starved ampka 2 cells had low glucose levels and developed fruiting bodies with long stalks and small sori. Therefore, reduced glucose levels could be one of the causes for this inequitable fruiting body formation. Mixing of cell types in the ampka 2 mutant suggest its role in maintaining the boundary between them. Thus, AMPKa assists in proportioning and patterning of prestalk/prespore cells. Glucose has also been shown to play a role in the cell sorting behaviour of Dictyostelium cells. The differential preferences of cells in development and differentiation have been observed in various organisms using chimaera study. Chimaeras are mixture of cells from two or more genetically different backgrounds. Several chimaeras in Dictyostelium show unequal apportionment of the genetically different cells into spore and stalk cells [21,44]; the one that gets a higher proportion of spores is called cheater and the other is called loser [45]. Khare & Shaulsky [46] have led this concept of multi-cellular bodies using competition to place their best cells into justified functions, so the question arises, do the mutant cells contribute equally in spore formation of chimaeras? ampka 2 cells form few fruiting bodies from a given number of cells when compared with the wild-type cells in pure populations; this result is sufficient to explain the competitive failure of mutant cells in contributing to spore formation in chimaeras. There are various reports that explain the role of glucose in the sorting behaviour of Dictyostelium cells during differentiation. In chimaeras, G þ cells preferentially become prespore cells of the slug and G 2 cells sort out to become prestalk cells [47][48][49]. Our study provides insights about the differential preferences of ampka 2 cells that exhibit low glucose levels in the cell sorting behaviour. The ampka 2 cells participate mainly in prestalk-derived structures and have less proclivity to occupy the prespore/spore region within chimaeras in the presence of Ax2 cells. Previous studies showed deletion of ampka resulted in embryonic lethality and, therefore, its direct impact on cellular differentiation and lineage choice is still unknown [50]. Young et al. [51] showed direct impact of AMPKa in cell fate determination during differentiation. Further studies are still required to understand the direct impact of AMPKa on cell lineage tracing and differentiation in Dictyostelium.

Conclusion
Our results demonstrate that AMPKa regulates aggregate size in Dictyostelium. The fruiting bodies formed by ampka 2 cells result from the differences in prestalk/prespore ratio. The results also suggest a role in cell-type differentiation and spatial patterning.

Growth and development of Dictyostelium discoideum
The Dictyostelium cells were grown and developed as described [52]. The logarithmic phase cultures (2.5-5 Â 10 6 cells ml 21 ) were identically diluted into fresh media at a density of CF AMPK cell growth cell proliferation cell size maintain prestalk/prespore ratio and spatial distribution G-6-P G -6 -P a s e c o m p l e x glucose aggregation territory cell-cell adhesion Figure 9. Model illustrates the role of AMPKa in growth and development. AMPKa inhibits cell growth, proliferation and size. It inhibits CF that represses the conversion of glucose from glucose-6-phosphate to control cellular events such as cell -cell adhesion, aggregation territory size, prestalk/ prespore ratio and spatial cell-type distribution. AMPKa also helps in maintaining the prestalk/prespore ratio and spatial distribution. In the above model, solid lines indicate known information, while dotted lines display proposed hypothesis from this study. rsob.royalsocietypublishing.org Open Biol. 7: 170055 approximately 5 Â 10 5 cells ml 21 and monitored over 6 days for measuring cell proliferation.
For development, exponentially growing cells were harvested, washed in 1ÂKK 2 buffer and spotted at a density of 5 Â 10 7 cells ml 21 on non-nutrient agar plates. The plated cells were incubated at 48C for 4-6 h for synchronization of the development, followed by incubation at 228C. Analyses of mound size were performed using NIS ELEMENTS AR v. 4.0.

RNA detection by RT-PCR and in situ hybridization analyses
RNA was isolated as described [52] from growing amoebae and at various developmental stages. RT-PCR reactions were performed using gene-specific primer pairs (electronic supplementary material, table S1). rnlA (ig7) was used as an internal control.
The in situ hybridization studies were performed as described [52]. The probe was obtained by cloning a 744 bp PCR amplified region using the gene-specific primer pairs into XhoI/XbaI site of commercially available pBluescriptII phagemid (pBSIISKþ) vector (electronic supplementary material, figure S7). It was followed by in vitro transcription into RNA, sense probe with T7 polymerase (template obtained after construct digestion with XbaI) and antisense probe with T3 RNA polymerase (template obtained after construct digestion with XhoI) were obtained. The probe was labelled with a DIG RNA labelling kit (Roche Diagnostics) and in situ hybridization was performed. A sense probe was used as a control.
The list of primer pairs for other genes used in this study is given in the electronic supplementary material, table S1.

ampka overexpressing strain
A full-length ampka gene was PCR amplified (electronic supplementary material, figure S1) from genomic DNA using the gene-specific primer pairs (electronic supplementary material, table S1) and cloned into act15/Acg-Eyfp vector (electronic supplementary material, figure S1) that contains the actin 15 promoter, enhanced yellow fluorescent protein (Eyfp) at the C-terminus, a G418 resistance marker for selection in Dictyostelium and an ampicillin resistance marker for selection in bacteria.

ampka 2 strain
The 5 0 and 3 0 targeting regions were PCR amplified (electronic supplementary material, figure S2) by using the gene-specific primer pairs (electronic supplementary material, table S1) and introduced into the flanking side of the Blasticidin (Bsr) cassette. After restriction digestion, linearized knockout construct was introduced into Ax2 cells by electroporation and the transformed cells were selected at 10 mg ml 21 Blasticidin-S (Invitrogen). Genomic DNA was extracted as described [53] and targeted gene disruptions were identified by several PCR reactions (electronic supplementary material, figure S2e) using primers (electronic supplementary material, table S2), and the absence of protein was further confirmed by western hybridization (electronic supplementary material, figure S2f ).

ampka rescue strain
The rescue strain was made by expressing an AMPKa-Eyfp fusion construct into ampka 2 cells.

Cell dry weight
Nearly 5 Â 10 7 log phase cells were washed and vacuum dried at 558C. After 1 h, the weight of dry pellets was scored.

Flow cytometry
To determine cell size, a BD FACS Calibur flow cytometer with CELL QUEST software was used. About 1 Â 10 7 log phase cells were harvested, washed in 1ÂKK 2 buffer and re-suspended in 1.5 ml buffer (0.9% NaCl, 2% sucrose, 5 mM EDTA in KK 2 buffer). Cells were fixed by adding 75% chilled ethanol dropwise and incubated for 30 min at 228C and stored at 48C. Immediately before analysis, 1 Â 10 6 cells were washed, resuspended in KK 2 buffer, and incubated at 378C for 30 min in 10 mg ml 21 RNase A (Sigma-Aldrich, USA) followed by incubation at room temperature in 50 mg ml 21 propidium iodide (Sigma-Aldrich).

Conditioned medium experiments
CM was prepared as described previously [54]. Briefly, log phase cells of Ax2 and ampka 2 were starved and re-suspended at a density of 1 Â 10 7 cells ml 21 and kept under shaken conditions for 20 h, at 228C. Cells were pelleted down and the supernatant was further clarified by centrifugation. The clarified supernatant thus prepared or CM was used immediately.
To check the effect of CM on aggregate size, Ax2 and ampka 2 cells were starved on dialysis membranes, which were placed on Whatman filters (two to three layers) soaked in Ax2 CM or ampka 2 CM. Cells starved on Whatman filters (two to three layers) soaked in 1ÂKK 2 buffer were used as a control.

Spore viability assays
Spore viability assay was followed as described [21]. Spores from mature fruiting bodies were harvested in spore buffer (40 mM KH 2 PO 4 , 20 mM KCl, 2.5 mM MgCl 2 ), washed twice by centrifugation at room temperature and counted in a haemocytometer. Aliquots of 100 spores were mixed with a suspension of bacteria (Klebsiella aerogenes) and grown for 5 days. The per cent viability of spores was measured by counting the number of clear plaques formed on the bacterial lawns divided by total spores plated followed by multiplication with 100. Three independent experiments in triplicate were performed.

Glucose assay
Glucose assay was performed as described [25] with minor modifications. Log phase cells were harvested and re-suspended at a density of 8 Â 10 6 cells ml 21 and kept under shaken conditions for 6 h at 228C. Cells were harvested and lysed by the freeze-thaw method. Glucose assay was performed as per instructions given by the manufacturer (GAHK20; Sigma-Aldrich). Protein levels were measured using Bradford reagent (BIO-RAD).
rsob.royalsocietypublishing.org Open Biol. 7: 170055 5.9. Development of chimaeric mixtures Ax2 and ampka 2 cells were transfected with pTX-RFP and pTX-GFP, respectively, and selected at 40 mg ml 21 of G418. GFP-and RFP-marked cells were mixed in varying percentages (5-75%) and developed on non-nutrient agar plates. Both DIC and fluorescent images were captured on a Nikon SMZ-1500 microscope. Individual spore heads were picked on a glass-slide and photographed, both under brightfield and under fluorescence using a Nikon eclipse 80i fluorescence microscope. Red and green fluorescent spores were counted from the photographs. A minimum of 10-15 fruiting bodies developed from each mixture per individual experiment was counted.

b-Galactosidase staining
b-Galactosidase staining was performed as described [52]. Images were captured using a Nikon AZ100 microscope.

Statistical analysis
The statistical analyses were performed (mean standard deviation and standard error) and values were plotted in graph using Microsoft EXCEL-2013 and GraphPad PRISM. p-Values of less than 0.05 were considered as significant.
Data accessibility. The datasets supporting this article have been uploaded as part of the electronic supplementary material.