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Corresponding author: Jennifer L. Watts, Washington State University, Pullman, WA 99164-6340., jwatts{at}mail.wsu.edu (E-mail)
Communicating editor: B. J. MEYER
 | ABSTRACT |
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 TOP ABSTRACT MATERIALS AND METHODSRESULTS AND DISCUSSIONLITERATURE CITED |
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Arachidonic acid and other long-chain polyunsaturated fatty acids (PUFAs) are important structural components of membranes and are implicated in diverse signaling pathways. The 
6 desaturation of linoleic and linolenic acids is the rate-limiting step in the synthesis of these molecules. C. elegans fat-3 mutants lack 6 desaturase activity and fail to produce C20 PUFAs. We examined these mutants and found that development and behavior were affected as a consequence of C20 PUFA deficiency. While fat-3 mutants are viable, they grow slowly, display considerably less spontaneous movement, have an altered body shape, and produce fewer progeny than do wild type. In addition, the timing of an ultradian rhythm, the defecation cycle, is lengthened compared to wild type. Since all these defects can be ameliorated by supplementing the nematode diet with gamma-linolenic acid or C20 PUFAs of either the n6 or the n3 series, we can establish a causal link between fatty acid deficiency and phenotype. Similar epidermal tissue defects and slow growth are hallmarks of human fatty acid deficiency.
THE 6 fatty acid desaturase catalyzes the rate-limiting step in the conversion of the essential fatty acids, linoleic acid (18:2n6) and linolenic acid (18:3n3), into C20 polyunsaturated fatty acids (PUFAs) such as arachidonic acid (20:4n6) and eicosapentaenoic acid (20:5n3). (Fatty acid nomenclature used here is the following: X:YnZ refers to a fatty acid chain of X carbon atoms and Y methylene-interrupted cis double bonds; Z indicates the position of the terminal double bond relative to the methyl end of the molecule.) PUFAs play critical roles in regulating membrane structure, dynamics, and permeability. In mammals, C20 PUFAs are substrates for oxygenases that produce powerful short-range eicosanoid effector molecules, including prostaglandins, leukotrienes, and thromboxanes (
Caenorhabditis elegans is an attractive animal model in which to investigate the physiological roles of specific fatty acids in growth, development, and the nervous system. Unlike mammals, C. elegans does not require essential fatty acids in its diet, but is capable of synthesizing 20:4n6 and 20:5n3 using only saturated and monounsaturated fatty acids from bacteria as precursors (12 and n3 desaturase) and animals (5 and 6 desaturase) as well as PUFA elongase activities found in animals (
To investigate the roles of various fatty acids in growth, development, and neurological function in an animal system, we recently isolated C. elegans mutants deficient in PUFA synthesis by direct analysis of fatty acid composition (5 unsaturated PUFAs for normal development under laboratory conditions. The n3 and 5 desaturase mutants are deficient in certain classes of C20 PUFAs but accumulate higher levels of precursor C20 PUFAs as a consequence of these deficiencies. In contrast, the fat-3 mutants that lack 6 desaturase activity fail to produce any of the common C20 PUFAs and, as a result, their growth and behavior are compromised. Here we demonstrate that although the fat-3 mutants are viable and fertile, they exhibit neuromuscular defects, cuticle abnormalities, reduced brood size, and altered biological rhythms. These defects can be biochemically complemented by dietary supplementation of various 20-carbon PUFAs.
| MATERIALS AND METHODS |
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| TOPABSTRACTMATERIALS AND METHODSRESULTS AND DISCUSSIONLITERATURE CITED |
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Culture and measurement of nematodes:
Nematodes were cultured and maintained according to standard methods (
Behavioral assays:
The defecation cycles of first-day adult animals were scored by measuring the time from one posterior body contraction to the next. The presence or lack of an enteric muscle contraction at the end of each cycle was noted as well. For each strain a minimum of six animals were scored for 10 cycles each. Unless otherwise noted, defecation cycles and enteric muscle contractions were scored with the petri dishes closed. Movement assays were performed as described (
Construction of the fat-3::GFP reporter gene:
The full-length translational fusion was constructed by fusion PCR of the amplified fat-3 promoter and coding sequences together with the green fluorescent protein (GFP) coding sequence amplified from pPD95.75 (
Fatty acid supplementation and analysis:
Fatty acid sodium salts were obtained from NuChek Prep (Elysian, MN) and stored at -20° in the dark. For each experiment, a fresh 0.1 M stock was prepared by dissolving fatty acids in sterile H2O. NGM agar was prepared with the addition of 0.1% tergitol (NP-40). Agar was cooled to 45°–50° and fatty acid stock was added slowly and stirred for 1 min. Plates were poured immediately and then covered to dry in the dark for 24 hr. Plates were then seeded with Escherichia coli and allowed to dry for 2 days in the dark at room temperature before the addition of embryos. Embryos were prepared by alkaline hypochlorite treatment of adult nematodes to obtain a semisynchronized population of early embryos. After phenotypic analysis of adult worms, nematodes were washed off the plates in H2O and centrifuged gently to pellet the worms. As much water as possible was removed and the worm pellets were frozen for determination of fatty acid composition as described in WATTS and BROWSE (2002).
| RESULTS AND DISCUSSION |
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| TOPABSTRACTMATERIALS AND METHODSRESULTS AND DISCUSSIONLITERATURE CITED |
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Fatty acid composition of 6 desaturase mutants and growth phenotypes:
The 6 desaturase mutants were isolated without selection using gas chromatography analysis of fatty acids derived from mutagenized nematodes (6 desaturase precursors 18:2n6 and 18:3n3 and a deficiency in C20 fatty acids, most notably undetectable levels of dihomogamma-linolenic acid (20:3n6), arachidonic acid (20:4n6), and eicosapentaenoic acid (20:5n3). We found that the phenotypes described in this work were indistinguishable among the three fat-3 alleles (wa22, wa23, and wa25). Worms of all three genotypes display identical fatty acid compositions with undetectable 6 unsaturated PUFAs, implying that all three alleles represent loss of activity of the 6 desaturase. Detailed phenotypic characterization was carried out with fat-3(wa22).
The fat-3 homozygous worms are viable and fertile, indicating that C20 PUFAs are not essential for life in this organism. However, they grow at a slower rate than wild type, requiring one extra day of development at 20° before they become fertile adults (
20% of the fat-3 embryos failed to hatch. These observations indicate that C20 PUFAs are necessary for optimal egg production at a range of temperatures and that at low temperature embryogenesis is compromised by the lack of C20 PUFAs. Mutations that affect the degree of fatty acid unsaturation in plants and cyanobacteria also result in cold-sensitive phenotypes, presumably because proper membrane fluidity and permeability at lower growth temperatures requires high levels of membrane unsaturation (
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Even though development is delayed and brood size is reduced, we did not notice any apparent tissue or cell fate specification defects in fat-3 worms. The pharyngeal, intestinal, hypodermal, muscular, neuronal, and reproductive tissues appear normal and their cell nuclei maintain their distinctive characteristics. We performed one trial to examine if fat-3 worms exhibited shorter or longer life spans than wild type and found that their life span was very similar to that of wild type, in contrast to the long-lived control age-1(hx546) (data not shown). Thus, although the fat-3 worms require one extra day to develop from embryo to fertile adult, their overall life span is not significantly different from wild-type worms.
fat-3 worms exhibit neuromuscular defects:
C. elegans has four major muscle groups: the body-wall muscles used for locomotion, the pharyngeal muscles used for feeding, the vulval and uterine muscles used for egg laying, and the enteric muscles used for defecation (
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The pharyngeal and enteric muscle groups are also affected by a lack of C20 PUFAs. We found that although the fat-3 worms exhibit a regular pharyngeal pumping pattern, the rate is reduced to 70% of that of wild type (Table 2). In addition, the enteric muscle contraction, which expels gut contents during defecation, is reduced in fat-3 mutants. Young adult wild-type animals exhibit a contraction during 99% of defecation cycles, while the enteric muscle contraction fails in 31% of defecation cycles in fat-3 animals. The fat-3 mutants lay eggs at approximately half the rate of wild type (2.9 eggs/hr vs. 5.6 eggs/hr at their peak egg-laying period, 40 hr after the L4 to adult molt). However, newly laid eggs are at similar developmental stages as those laid by wild type. Mutants with hyperactive egg-laying muscles lay eggs at very early stages, while egg-laying defective mutants lay eggs that have developed to late stages of embryogenesis or fail to lay eggs and the retained embryos often hatch inside the parent (
Dumpy body shape of fat-3 is likely due to cuticle defects:
The fat-3 worms exhibited a somewhat Dumpy (short and fat) body shape. The average body length of fat-3(wa22) L4 animals is 80% that of wild-type L4s (Table 2). The Dumpy (Dpy) phenotype can result from disruption of several unrelated systems. Dpy body shape occurs in animals carrying mutations in genes with roles in dosage compensation or mutations that result in hypercontraction of muscles. It is unlikely that fat-3 mutants have abnormal dosage compensation as fat-3 males and hermaphrodites do not display sex-specific phenotypic differences common in dosage-compensation mutants (
We hypothesize that the fat-3 Dpy phenotype is due to defects in cuticle composition resulting from C20 PUFA deficiency. We found that fat-3 worms are more sensitive than wild type to a chemical treatment that disrupts the nematode cuticle. The fat-3 worms showed major cuticle disruption after an average of 2.0 (±0.1) min in alkaline hypochlorite solution, while wild type did not show a break in the cuticle until an average of 5.4 (±0.1) min. The lipid components of the C. elegans cuticle are complex and include polar phospholipids, unesterified fatty acids, triacylglycerides, and complex glycolipids (6 desaturase deficiency reported skin and hair abnormalities in the patient as well as slow growth (
fat-3 mutants display an abnormal defecation rhythm:
Defecation is an ultradian rhythm that occurs every 45 sec in wild-type hermaphrodites (
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The length of the defecation cycle is regulated by periodic calcium release in the intestine that is mediated by an inositol triphosphate (IP3) receptor, an intracellular calcium channel (
fat-3 is expressed in multiple tissues throughout the life of the worm:
To determine the tissues where the fat-3 gene is expressed, we constructed a gene fusion between fat-3 and the GFP gene sequences. The fusion included the upstream regulatory region and the entire fat-3 coding sequence fused to GFP. Both N2 and fat-3 (wa22) were transformed with this construct and the GFP fluorescence pattern was similar in both genotypes. Normal body shape and movement were restored to the transgenic fat-3 worms and lipid analysis revealed that 19% of the total fatty acids consisted of 18:3n6, 20:3n6, 20:4n6, and 20:5n3, PUFAs that are undetectable in untransformed fat-3 animals.
GFP expression is first apparent in comma-stage embryos in intestinal cells and continues throughout all larval stages and into adulthood (Fig 2). L1 larvae carrying the fat-3::GFP constructs showed GFP expression in the intestine, pharynx, and body-wall muscles. In L2–L4 larvae and adults, in addition to intestinal, pharyngeal, and body-wall muscle expression, faint expression is observed in several head and tail neurons. This wide range of expression underscores the importance of lipids for storage fuel and as components of membranes critical to cell function. In C. elegans, the intestine is the organ responsible for nutrient uptake, digestion, nutrient distribution, and fat storage. The high level of intestinal expression of the FAT-3 6 desaturase suggests that significant fatty acid modifications occur in this organ as well. In addition, the muscular and neuronal expression is consistent with defects in these tissues that are observed in fat-3 mutants.
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Biochemical complementation of fat-3 defects by dietary supplementation of PUFAs:
To determine if the physiological effects of PUFA deficiency could be reversed by dietary supplementation of fatty acids, we included fatty acids in the nematode culture plates. Early embryos were plated onto media containing various PUFAs solubilized with tergitol. Growth, movement, and defecation were characterized after 3–4 days, when the embryos developed into young adults. Supplementation with 18:3n3, a fatty acid substrate of the 6 desaturase that already accumulates in fat-3 mutants, had little effect on growth rate, and the supplemented worms performed only slightly better than unsupplemented fat-3 controls in the movement assay. However, the addition of 80 µM of 18:3n6, 20:3n6, 20:4n6, or 20:5n3 completely rescued the slow growth and Dpy body-shape defects caused by the 6 desaturase deficiency (Fig 3). The rescue of the Dpy body shape also correlated with the rescue of the sensitivity of the cuticle to alkaline hypochlorite treatment (Fig 4A). In addition, the defecation cycle of the rescued worms was similar to wild type for all of these fatty acids (Fig 4C). Finally, the body-wall, pharyngeal, and enteric muscle functions were also rescued with a range of dietary fatty acids in the fat-3 worms (Fig 4D). Rescue with dietary fatty acids assures us that these defects arise solely as a result of a 20-carbon PUFA deficiency. Similarly, the human patient with a 6 desaturase deficiency was given dietary supplements of 20:4n6 and 20:5n3, which cured her growth failure and greatly improved her skin condition (
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Biochemical complementation with 6-desaturated dietary fatty acids also restored, or nearly restored, normal brood size in the fat-3 mutants (Fig 4B). However, fatty acid supplements had an adverse affect on wild-type brood size. The most severe effect was observed with supplementation with 18:3n6, which shifted the n6/n3 ratio from 0.47 to 1.22 and resulted in only 66% as many eggs as produced by unsupplemented wild-type worms. This suggests that the proper balance of C20 n6 and n3 PUFAs may be a prerequisite for optimal egg production.
Finally, to test if dietary fatty acids could rescue the various defects in adult worms that had already completed development, we placed 1-day adults that had commenced laying eggs onto plates containing 0.1 mM 18:3n6, 20:3n6, or 20:5n3 supplements. The defecation cycle, enteric muscle contractions, thrashing, and pharyngeal pumping were scored after 24 hr. The worms retained their Dpy body shape, since their final cuticle molt had already occurred, but they were visibly more active on the plates than the control worms. The fatty acid composition of the 24-hr-supplemented adults was similar to worms that were grown on supplements for their entire lives (data not shown). After 24 hr the length of the defecation cycle was restored to wild type in the animals fed 18:3n6, 20:3n6, or 20:5n3 (average of 44 sec for all). Quantitation of movement, pharyngeal pumping, and enteric muscle contraction revealed significant improvement over fat-3 control worms with both fatty acids, but not complete rescue (Fig 4E). Therefore, dietary fatty PUFAs are capable of restoring biological rhythms and neuromuscular functions even in worms that have completed development without them.
Determination of the fatty acid composition of supplemented worms reveals a significant uptake of dietary fatty acids (Fig 3). Supplementation of fat-3 mutants with fatty acids normally synthesized late in the PUFA biosynthetic pathway, such as 20:5n3, result in dramatically altered fatty acid composition compared to wild type, since nematodes cannot rehydrogenate double bonds to convert 20:5n3 to 20:3n6 or 20:4n6. In wild type, supplementation with 18:3n6, 20:3n6, or 20:4n6 resulted in an increased n6/n3 ratio, while supplementation with 20:5n3 resulted in a decrease in this ratio. Despite these alterations in fatty acid composition, growth on these supplements was sufficient to rescue the fat-3 defects and the altered n6/n3 ratio had few adverse effects on wild-type worms. Therefore, the precise fatty acid composition observed in wild-type worms is not a requirement for optimal neuromuscular function, growth, and body-shape determination; rather, our data show that the presence of a combination of the fatty acids 20:3n6, 20:4n6, and 20:5n3 is sufficient for these functions.
In mammals, eicosanoid products derived from C20 PUFAs are effective short-range signaling molecules that mediate pain, inflammation, and reproductive processes. It is not known whether C. elegans produces eicosanoid effectors from C20 PUFAs. The fat-3 defects described in this work could arise from a deficiency of eicosanoids derived from C20 PUFAs by cyclooxygenase and P450 monooxygenase enzymes (C. elegans apparently lacks lipoxygenase-like genes). The ability of 20:5n3 to rescue most defects as well as 20:4n6 argues against the importance of cyclooxygenase products, since in mammals 20:5n3 is a poor substrate for these enzymes. However, C. elegans contains 80 cytochrome P450 genes, some of which may be capable of forming epoxy (EET), hydroxy (HETE), and lipoxin products from PUFAs (
| ACKNOWLEDGMENTS |
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We thank Jim Thomas for suggestions and advice, Andy Fire for vectors, and Jim Wallis for helpful comments on the manuscript. Some of the strains were provided by the Caenorhabditis Genetics Center, which is funded by the National Center for Research Resources of the National Institutes of Health. Funding was provided by National Institutes of Health R01 GM62521, National Science Foundation postdoctoral fellowship DBI-9804195 to J.L.W., and the Agricultural Research Center, Washington State University.
Manuscript received July 12, 2002; Accepted for publication November 11, 2002.
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