Abstract
Background
Mutations that cause feeding defects in the nematode C. elegans are known to increase life span. Here we show that feeding defective mutants also have a second general trait in common, namely that they are small.
Results
Our measurements of the body lengths of a variety of feeding defective mutants, or of a variety of double mutants affecting other pathways that regulate body length in C. elegans, i.e. the DBL-1/TGFβ, TAX-6/calcineurin and the SMA-1/βH-spectrin pathways, indicate that food uptake acts as a separate pathway regulating body length. In early stages, before eating begins, feeding defective worms have no defect in body length or, in some cases, have only slightly smaller body length compared to wild-type. A significant difference in body length is first noticeable at later larval stages, a difference that probably correlates with increasing starvation. We also show that autophagy is induced and that the quantity of fat is decreased in starved worms.
Conclusion
Our results indicate that the long-term starvation seen in feeding-defective C. elegans mutants activates autophagy, and leads to depletion of fat deposits, small cell size and small body size.
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Background
It is obvious that body size in the nematode C. elegans is genetically regulated: many mutations in C. elegans result in abnormal body sizes. Examples include mutations that affect cuticle collagen and cause Dumpy (Dpy) phenotypes [1]. There is a number of genes that seem to regulate body size in a more indirect manner resulting in Small (Sma) or Long (Lon) worms. According to the literature, there appears to be at least three different genetic pathways that determine C. elegans body length (see Fig. 1 and Table 1). These are: 1) A TGF-β pathway, involving the dbl-1, sma-2, sma-3, sma-4, kin-29, lon-1 and additional genes [2–5]; 2) A spectrin pathway involving the sma-1 [6], spc-1 [7] and unc-70 [8] genes and 3) A calcineurin pathway involving the calcineurin homologs tax-6 [9] and cnb-1, both expressed in many sensory neurons and most muscle cells [10], where expression of tax-6 specifically in neurons rescues the small body phenotype in the tax-6 mutant [9]. Some mutations that cause small worms have not yet been firmly assigned to these pathways. For example, rnt-1, which encodes a homolog to the mammalian RUNX transcription factors, has been assigned to the TGF-β pathway but this conclusion rests on genetic interaction experiments still compatible with other interpretations [11, 12]. Also, the sma-5 mutant exhibits a small, thin and slow growth phenotype, and was recently found to encode a homolog to the MAP kinase BMK1/ERK5. This gene is expressed in the intestine, hypodermis, excretory cell and the pharynx, and the body length defects are additive to the DBL-1/TGF-β pathway [13]. It will therefore be interesting in the future to find out if sma-5 is part of another yet undiscovered pathway regulating body size besides the ones described here (Fig 1).
While the genetic basis of body size in C. elegans is beginning to be well understood, it is perhaps less well appreciated that the life experience of this organism can also influence body size. It is well known that caloric restriction can increase life span in C. elegans or induce formation of the growth arrested dauer larva [14, 15]. Lakowski et al [14] showed that mutations in many of the eat mutant genes lengthens the life span: eat-1(ad427) lives 33% longer, eat-2 (ad465) 29%, eat-3 (ad426) 11% and eat-10 (ad606) 8% longer. They also showed that there is a correlation between longer life span and the severity of the feeding defect: the eat-1 allele with the slowest pumping rates (ad427) lives 33% longer while the weakest allele (e2343) lives 11% longer.
However, very few reports have emphasized the fact that reduced food uptake also correlates with reduced body length. In one report, a feeding defective mutant (eat-2) was shown to have a smaller body volume than wild-type worms, but no actual length measurements were reported [16]. In another study, a deletion in the intestinal peptide transporter gene pep-2, which effectively reduces the delivery of amino acids for growth and development from the gut lumen into the intestinal cells, was found to have a reduced body length, [17]. Given the great interest in correlating the effect of food deprivation on longevity [14, 18, 19], as well as the strong inverse relationship between height and longevity in humans [20], we decided to determine whether body size is also inversely correlated with food uptake in the organism C. elegans, a popular model to study longevity.
Here we show that feeding defective mutants are short, independently of the nature of the genetic defect that impairs the feeding behavior. This suggests that food uptake acts as a separate pathway regulating body length. We also show that fat stores are depleted but that autophagy is upregulated in feeding defective mutants. Autophagy is a catabolic process through which proteins and organelles are degraded and the amino acids are reused by the cells. Constituents to be degraded are engulfed by double-membrane cytoplasmic vesicles forming an autophagosome that further fuses with lysosomes for degradation (for review see [21, 22]). In the fruit fly Drosophila Melanogaster it has been reported that starvation induces autophagy in the larval fat body [23]). In C. elegans, autophagy was previously known to occur before entry into the dauer larval stage and the process is thought to be involved in the remodelling of various tissues of the dauer larva [24].
Results
Feeding defective mutants are short and thin
We measured the length of photographed age-matched C. elegans adults of a variety of genotypes and found that all the feeding defective mutants that we studied were significantly shorter than wild-type animals (Fig. 2, 3 and Table 2). In particular, we found that mutants with abnormal pharyngeal anatomies (pha-2, pha-3), or normal pharynxes with reduced pumping rates (eat-1, eat-2, eat-3) or with inefficient pharyngeal pumping (e.g. slippery pharynx that inefficiently traps bacteria; eat-10) were all short.
As control for our general methodology we evaluated the length of wild-type N2 worms and found it to be the same as published values. Also, we scored a variety of other small mutants that fall within the TGF-β pathway (dbl-1, egl-4, sma-2, sma-3 and kin-29), the spectrin pathway (sma-1) or the calcineurin pathway (tax-6), as well as the mutant rnt-1: as expected, all of these mutants were short (Table 2). Finally, the lon-1 (e185) null allele caused worms to be slightly longer than wild-type, as expected (Table 2).
We also measured the body width of the feeding-defective mutant and of other single mutants with a small phenotype (dbl-1, egl-4, kin-29, rnt-1, sma-1, sma-2, sma-3 and tax-6) and one double mutant (dbl-1;pha-2) (Fig. 3 and Table 2). All feeding defective mutants were significantly thinner than wild-type, as were sma-2, sma-3 and tax-6. dbl-1 worms were only slightly thinner and sma-1 and rnt-1 worms exhibited wild-type widths. The thinnest worms were the dbl-1;pha-2 double mutants, which indicates an additive effect between these two mutations.
Food uptake efficiency acts as a separate pathway regulating body length
If two separate mutations cause reduced body length via separate pathways, one would expect that an individual worm homozygous for both mutations should be much smaller than either single mutant alone: the two mutations would show an additive effect. It is even possible that the additive effects of two such mutations might result in lethality, if their combined effect is too severe. We generated several double mutants and found that the results generally agree with the hypothesis that food uptake efficiency is a separate pathway regulating body length that shows an additive effect with the other established pathways. In particular, mutations in the DBL-1/TGF-β pathway showed an additive effect on body length (or even caused larval lethality) when combined with the pharyngeal abnormal mutation pha-2 (e.g. dbl-1;pha-2, kin-29;pha-2, pha-2;sma-2, pha-2;sma-3) and the pharyngeal pumping mutants eat-1 (e.g. eat-1;dbl-1) and eat-3 (e.g. eat-3;sma-2, eat-3;sma-3) (Table 2). Similarly, combining pha-2 or eat-3 with the βH spectrin sma-1 mutation or the rnt-1 mutation resulted in shorter worms or larval lethality (Table 2). Also consistent with the additive effects of combining mutations from distinct length-regulating pathways were the consequences of creating dbl-1;sma-1 and sma-1;tax-6 double mutants, which were both smaller than the single mutants involved (Table 2). Finally, we found that combining two separate mutations that impair food uptake via different mechanisms, and thus potentially completely prevent feeding, can cause larval lethality, as with the eat-3;pha-2 double mutant.
If one mutation causes an increase in body length by interfering with one pathway while a second mutation causes a reduced body length by interfering with a separate pathway, one would expect the double mutant to show an additive effect and thus to be of intermediate length. Morita et al previously reported that double mutants of lon-1(e185) and dbl-1(nk3) had intermediate body length, as if these genes belonged to separate pathways [24]. In contrast, the weaker lon-1(wk50) allele behaves as if lon-1 and dbl-1 were in the same pathway: the double mutant lon-1(wk50) dbl-1(nk3) results in worms longer than wild-type, indicating that lon-1 is epistatic to dbl-1 [25]. Given these premises, we used both lon-1(e185) and lon-1(wk50) to test whether feeding acts separately from the DBL-1/TGFβ pathway in regulating body length. This was indeed the case: the eat-3;lon-1 (wk50), lon-1(e185);pha-2 and lon-1 (wk50);pha-2 double mutants had intermediate lengths compared to their constituent single mutants (Table 2). (Note that in our study, the dbl-1;lon-1(wk50) double mutant showed an additive effect of the mutations, suggesting that lon-1 is not completely epistatic to dbl-1.)
Three of the double mutants tested behaved in unexpected ways: the dbl-1;eat-3, eat-3;kin-29 and pha-2;tax-6 double mutants showed no additive effect between the individual two mutations involved (Table 2). This may possibly reflect overlaps in branching pathways between these mutants.
The difference in body length is most prominent at later larval stages
Some of the mutants studied were dramatically smaller than wild-type worms, especially double mutants such as dbl-1;pha-2 that are only 30% of wild-type in length (Fig. 3). We studied the eggs of small mutants to determine if they are also reduced in size. Specifically, we measured the circumference of eggs containing embryos of the same developmental stage for the mutants dbl-1, dbl-1;pha-2, eat-1, eat-3, eat-10, pha-2, pha-3, sma-1 and tax-6 (Fig. 4 and Table 3). Only dbl-1;pha-2 and sma-1 showed a minor decrease in size.
To investigate at which stage of postembryonic development the difference in body length between wild-type and the feeding defective mutants are first prominent we measured the body length at two larval stages, L1 and L4. In this study we also included some of the mutants from the other pathways (dbl-1, sma-1 and tax-6) and one double mutant (dbl-1;pha-2) (Fig. 4 and Table 3).
L1 larvae from all the feeding mutants, except eat-1 and sma-1, were only slightly smaller than wild-type larvae, and so were the dbl-1 and tax-6 mutants. In a previous report sma-1(ru18) was shown to exhibit a small phenotype already at the embryo stage due to elongation defects [6], an observation that we here confirmed: sma-1 worms are significantly smaller already at the L1 stage. The double mutant dbl-1;pha-2 is also shorter than wild-type but only a small additive effect is seen at this stage compared to the single mutants.
At the L4 stage all the feeding-defective and other small mutants are much smaller than wild-type, a difference that persists in adults (Fig. 4, Table 2 and 3). In conclusion, most of the short body length phenotype of the feeding-defective mutants develops once feeding has begun.
Autophagy is induced in feeding defective mutants
Growth of cells and tissues during development is influenced not only by anabolic processes such as protein synthesis, but also by the rate and extent of catabolic, degradative processes. The turnover of most long-lived cellular proteins occurs through a process known as autophagy (reviewed in [26]). In this process, cytoplasm and organelles are non-selectively engulfed by a double membrane-bound vesicle, the autophagosome, which fuses with the lysosomal and/or endosomal compartment. The resulting degradation products can be a source of cellular nutrients, and indeed autophagy is strongly induced in response to nutrient deprivation in many cell types. Autophagy is also activated in C. elegans lavae that are entering the long-lived dauer state in response to adverse conditions [24].
We wished to test if the small body size among the feeding defective mutants is associated with autophagy. To visualize autophagy we used the extrachromosomal reporter lgg-1::gfp which was introduced into the mutants eat-3, pha-2 and pha-3. lgg-1 is homologous to the S. cerevisiae gene Apg8/Aut7p [27] and mammalian MAP-LC3 [28] and is useful as a marker for autophagy. The gene is expressed in many cells, including neurons, pharyngeal muscle cells, intestinal cells, gonad, vulva and hypodermal seam cells [24]. During conditions where autophagy is absent the expression of lgg-1::gfp is diffuse; when autophagy occurs preautophagosomal and autophagosomal structures are seen as GFP-positive punctate areas (Fig. 5 and [24]). We studied the hypodermal seam cells in L3 larvae, a stage before the most noticeable difference in body length is seen between wild-type and the feeding defective mutants. We found that feeding mutants have many more GFP-positive punctate areas than wild-type control worms, indicating increased autophagy activity in the mutants. (Fig. 5A–B).
We also used the lgg-1::gfp reporter as a tool to estimate the size of the seam cells and found that, in three studied mutants, the reduction in body length (Table 2 and Fig. 4) correlates well with the reduced size of the seam cells (Fig. 5C).
Feeding defective mutants exhibit decreased levels of fat deposits
We then wished to investigate if the increased autophagy correlates with depletion of fat stores in the feeding defective mutants. Fat deposits can be labelled by uptake of the vital dye Nile Red, which can conveniently be included in the culture plates. Wild type, dbl-1, eat-3, pha-2, pha-3, sma-1 and tax-6 worms at different stages were grown 24 hrs on plates containing the dye. No difference in the level of Nile Red staining could be detected between wild type and dbl-1, sma-1 or tax-6 at any stages of life. In contrast, 1-day old adults of the three feeding-defective mutants tested (eat-3, pha-2 and pha-3) showed a clear reduction in Nile Red staining compared to age-matched controls (Fig. 6). Nile Red staining in these same mutants was indistinguishable from controls during the larval stages (data not shown). These results indicate that fat stores present during the larval stages are depleted as post-embryonic development proceeds in feeding-defective mutants.
Discussion
We show here that a variety of unrelated mutations in genes that cause a wide range of feeding defects in C. elegans also cause a reduction in body length, and that the effects of these mutations are generally additive with body-shortening mutations that act via other pathways, namely the DBL-1/TGF-β pathway, the SMA-1/Spectrin pathway or the TAX-6/calcineurin pathway.
Reduced body length is therefore a second general property of the feeding defective mutants. The first reported general property is their increased longevity, which was attributed to the presumed benefits of caloric restriction on lifespan [14, 18]. The nematode C. elegans is thus an organism where caloric restriction causes both a decrease in body size, and an increase in longevity. It has been known for decades that caloric restriction produces smaller mice and rats that also have increased lifespan, and the same correlations hold true within human populations [20]. Our study indicates that this is true also for nematodes.
All the feeding defective mutants in our study are significantly shorter than wild-type at the L4 and adult stages. The reduced body length also correlated well with the reduced size of seam cells in the studied mutants. However just after hatching and before feeding starts, the difference in length is only minor and for one of the shortest mutants, eat-1, that exhibits 53% of wild-type length as an adult, there is no difference at all in length at the L1 stage. These results indicate that the decrease in body length is mostly a post-development consequence of food deprivation.
Entry into the dauer state is environmentally triggered by a combination of starvation and high pheromone concentration, a measure of crowdedness [29, 30]. It was recently shown that autophagy is enhanced in C. elegans during dauer formation where it might play a role in the remodelling of the animal as it becomes a dauer larva [24]. Our results show that autophagy is also induced at the L3 stage in feeding defective mutants, even the presence of abundant food and low worm density. This is an interesting observation because of the proposed role of autophagy in the increased longevity of insulin receptor mutants or of animals subjected to caloric restriction [31].
The insulin pathway, acting via the phosphatidylinositol kinase PI3K/TOR, plays an evolutionarily conserved role as an integrator of growth factor signalling and nutrient availability to regulate metabolism and body/organ/cell size [32, 33], and longevity [34]. In C. elegans, the daf-2 pathway (daf-2 encodes a homolog of the insulin receptor) regulates entry into the long-lived dauer state, which involves a dramatic change from a sugar to a fat-based metabolism, as well as developmental arrest, activation of the autophagy process and other changes [24, 35]. daf-2 acts via daf-16 (a FOXO forkhead transcription factor homolog) to regulate let-363 (the C. elegans PI3K/TOR homolog) which in turn activates autophagy, fat storage and other effector genes [36, 37]. Published literature on the effects of feeding defects on body length, and the results that we present here show that these same processes (body size, longevity, autophagy) are coupled to nutrient availability in C. elegans even when these worms do not actually enter the dauer state: feeding-defective mutants have short body/cell size, increased autophagy and, known from previous publications [14], increased longevity.
It is the varied nature of the feeding-defective mutations that together support the idea that it is the feeding defect itself that causes reduced body length: the only phenotypic aspect these mutations have in common is their impact on feeding. For example, eat-2 encodes a nicotinic acetylcholine receptor subunit that regulates the rate of pharyngeal pumping. The gene is only expressed in the junction between the pharyngeal muscle cells pm4 and pm5 and the allele studied here (ad465) is considered as a null allele [38]. The eat-2 mutants exhibit 66% of wild-type body length and, given the function and expression profile of the encoded protein, it seems evident that the feeding defect is the cause of the decrease in body length in that mutant.
pha-2 mutants on the other hand, exhibit a severe pharyngeal morphological defect in which the isthmus that is normally a narrow passage for food, is shortened and thickened. In pha-2 worms, bacteria are trapped within the isthmus and are poorly transferred further to the intestine. The pha-2 gene encodes a homeodomain transcription factor and is expressed in pharyngeal cells (pm4, pm5, I4, epithelial cells) but also in many cells outside the pharynx (extrapharyngeal neurons, intestinal cells, rectal cells; [39]). The functions of the extrapharyngeal expression of pha-2 are at present unknown. We have recently showed that in the only existing pha-2 allele, ad472, the mutation is located upstream of the start codon and impairs the expression of pha-2 specifically in the pharynx [40]. Thus, here again, it is clearly the pharyngeal defect of the pha-2 (ad472) mutant that is responsible for the shorter length. The molecular identity of eat-10 and pha-3 is not yet known and eat-1 and eat-3 have only proposed identities so far (Table 1).
In summary, we have shown that food uptake efficiency acts as a pathway regulating body length, and that this pathway is likely separate from the DBL-1/TGFβ pathway. Given that a reduced rate of food uptake also causes increased longevity [14], we are tempted to propose that the effects of mutations that impair food uptake in some way result in a partial activation of the dauer program via a non-TGF-β pathway such that growth is slowed or arrested, even as development into a long-lived fertile adult stage proceeds.
Conclusion
1. C. elegans feeding-defective mutants have previously been reported to have an extended lifespan. We show here that they are also smaller than wild-type.
2. Feeding defective mutations generally behave as a separate pathway regulating body length in C. elegans: their effects on body size are generally additive with mutations in other pathways that regulate body length.
3. C. elegans feeding-defective mutants have increased autophagy activity and decreased fat deposits.
Methods
Nematode strains and culturing
Maintenance and handling of worms were as described [41]. Wild-type parent strain used was the C. elegans Bristol variety strain, N2, [42]. All strains were cultured at 20°C. In addition to wild-type the following mutations were studied:
LG I: rnt-1(ok351).
LG II: eat-2(ad465), eat-3(ad426).
LG III: lon-1(e185), lon-1(wk50), sma-2(e502), sma-3(e491).
LG IV: eat-1(ad427), egl-4(ad450), eat-10(ad606), pha-3(ad607), tax-6(p675).
LG V: dbl-1(nk3), sma-1(ru18).
LG X: kin-29(oy38), pha-2(ad472).
Generations of double mutants
Double mutants were generated by crossing males to hermaphrodites using standard techniques [41] and scoring progeny for the expected phenotypes. An exception was the rnt-1(ok351) mutation for which double mutants were confirmed by PCR using the following primers:
5'-rnt-1: 5'-CATCGTCGGCTCATAATAAAACTGC-3'
3'-rnt-1: 5'-CGAGGAGAAGATGGTCGTTTTAAC-3'
The PCR reaction produces a 2162 bp fragment for amplification of the wild-type allele and a 662 bp fragment for the deletion allele.
Length measurements of eggs, L1, L4 larvae and adults
To measure the lengths and widths of adults, L4 larvae were picked to fresh plates and incubated at 20°C for 48 hrs. For study of L4 larvae worms with an obvious white crescent surrounding the visible prospective vulva were chosen. All L1 larvae were picked, mounted and photographed within 1 hour after hatching. Only eggs containing 3-fold stage embryos were studied. Eggs and worms were mounted on 2% agarose pads (in M9 buffer) and paralyzed with a drop of 100 mM levamisole and examined and photographed with a Zeiss axioplan compound microscope, using Nomarski optics and an attached AxioCam digital camera. All length measurements were performed with the free Java image processing program ImageJ [43]. Larvae and adults were measured from the nose to the tail tip (Fig 2). Eggs were measured by tracing their circumferences. The body widths were measured at the position of the vulva, from side to side.
Autophagy study
Wild-type worms carrying the extrachromosomal array lgg-1::gfp [24] were kindly provided by Beth Levine. The array was introduced into eat-3, pha-2 and pha-3 mutants by crossing. Worms were studied at 1000 × magnification using a Zeiss axioplan compound microscope equipped with fluorescent optics. GFP positive punctate regions were counted from photographs of lateral hypodermal seam cells of worms at the L3 stage.
Nile red staining
Worms were cultured 24 hrs on NGM plates containing 1 ng/ml Nile Red (5H-benzo [α] phenoxazine-5-one, 9-diethylamino) seeded with OP50. Fat content was monitored by fluorescence microscopy (rhodamine channel). All worms were photographed at a fixed exposure time.
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Acknowledgements
We thank Richard W Padgett and Tina Gumienny for the lon-1 (wk50) strain, Beth Levine for the lgg-1::gfp construct, and the C. elegans Genetics Center (funded by the NIH National Center for Resources), and particularly Theresa Stiernagle, for providing many of the strains used in this study. This work was supported by the Swedish funding agencies Vetenskaprådet, Cancerfonden and Carl Trygger Stiftelse.
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CM maintained the worm strains, generated the double mutants, and measured them. CM also performed the autophagy and Nile Red experiments, and helped in writing a draft of the manuscript. MP participated in the design of the study and in its coordination and helped to write the manuscript. All authors read and approved the final manuscript.
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Mörck, C., Pilon, M. C. elegansfeeding defective mutants have shorter body lengths and increased autophagy. BMC Dev Biol 6, 39 (2006). https://doi.org/10.1186/1471-213X-6-39
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DOI: https://doi.org/10.1186/1471-213X-6-39