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Camelina sativa, an oilseed crop in the Brassicaceae family, has inspired renewed interest due to its potential for biofuels applications. Little is understood of the nature of the C. sativa genome, however. A study was undertaken to characterize two genes in the fatty acid biosynthesis pathway, fatty acid desaturase (FAD) 2 and fatty acid elongase (FAE) 1, which revealed unexpected complexity in the C. sativa genome.
In C. sativa, Southern analysis indicates the presence of three copies of both FAD2 and FAE1 as well as LFY, a known single copy gene in other species. All three copies of both CsFAD2 and CsFAE1 are expressed in developing seeds, and sequence alignments show that previously described conserved sites are present, suggesting that all three copies of both genes could be functional. The regions downstream of CsFAD2 and upstream of CsFAE1 demonstrate co-linearity with the Arabidopsis genome. In addition, three expressed haplotypes were observed for six predicted single-copy genes in 454 sequencing analysis and results from flow cytometry indicate that the DNA content of C. sativa is approximately three-fold that of diploid Camelina relatives. Phylogenetic analyses further support a history of duplication and indicate that C. sativa and C. microcarpa might share a parental genome.
There is compelling evidence for triplication of the C. sativa genome, including a larger chromosome number and three-fold larger measured genome size than other Camelina relatives, three isolated copies of FAD2, FAE1, and the KCS17-FAE1 intergenic region, and three expressed haplotypes observed for six predicted single-copy genes. Based on these results, we propose that C. sativa be considered an allohexaploid. The characterization of fatty acid synthesis pathway genes will allow for the future manipulation of oil composition of this emerging biofuel crop; however, targeted manipulations of oil composition and general development of C. sativa should consider and, when possible take advantage of, the implications of polyploidy.
Interest in biofuels has prompted researchers to critically evaluate alternative feedstocks for biofuel production. One important, emerging biofuel crop is Camelina sativa L. Cranz (Brassicaceae), commonly referred to as "false flax" or "gold-of-pleasure". Renewed interest in C. sativa as a biofuel feedstock is due in part to its drought tolerance and minimal requirements for supplemental nitrogen and other agricultural inputs [1,2]. Similar to other non-traditional, renewable oilseed feedstocks such as Jatropha curcas L. ("jatropha"), C. sativa grows on marginal land. Unlike jatropha, which is a tropical and subtropical shrub, C. sativa is native to Europe and is naturalized in North America, where it grows well in the northern United States and southern Canada.
In addition to its drought tolerance and broad distribution, several other aspects of C. sativa biology make it well suited for development as an oilseed crop. First, C. sativa is a member of the family Brassicaceae, and thus is a relative of both the genetic model organism Arabidopsis thaliana and the oilseed crop Brassica napus. The close relationship between C. sativa and Arabidopsis [3,4] makes the Arabidopsis genome an ideal reference point for the development of genetic and genomic tools in C. sativa. Second, the oil content of C. sativa seeds is comparable to that of B. napus, ranging from 30 to 40% (w/w), suggesting that agronomic lessons from the cultivation of B. napus are applicable to C. sativa cultivation. Finally, the properties of C. sativa biodiesel are already well described , and both seed oil and biodiesel from C. sativa were used as fuel in engine trials with promising results [6,7].
Notwithstanding its potential for oil production, there is limited molecular and genomic information on this crop. Published studies detailing the biology of C. sativa and its closest relatives in the genus Camelina are few. However, several important findings can be drawn from the literature. Taxonomic treatments describe 11 species in the genus with a center of diversity in Eurasia , although C. sativa, C. rumelica, C. microcarpa, and C. alyssum are naturalized weeds with broad distributions. Camelina species can be annual or biennial, with some species requiring vernalization to induce flowering . Chromosome counts range from n = 6 in C. rumelica [10,11], or n = 7 in C. hispida , upwards to n = 20 in C. sativa, C. microcarpa, and C. alyssum [2,13]. Some Camelina species are interfertile; crosses of C. sativa with C. alyssum, and C. sativa with C. microcarpa, produce viable seed . In addition to these studies, a limited amount of molecular and sequence information is available for C. sativa [2,15-17].
Understanding the Camelina sativa genome is essential if agronomic properties are to be improved through molecular assisted breeding, mutation breeding, and/or genetic manipulation. For example, modification of the oil composition for superior biodiesel is a natural goal for this oilseed crop. C. sativa is high in polyunsaturated fatty acids such as linoleic acid (18:2; carbons:double bonds) and alpha-linolenic acid (18:3) as well as very long chain fatty acids (greater than 18 carbons) such as 11-eicosenoic acid (20:1) , while an ideal biodiesel blend is high in oleic acid (18:1) . Target genes for modification could therefore include FATTY ACID DESATURASE 2 (FAD2), a membrane bound delta-12-desaturase which converts oleic acid to linoleic acid [20-24], and FATTY ACID ELONGASE 1 (FAE1) which sequentially adds 2 carbon units to 18 carbon fatty acid CoA conjugates, resulting in very long chain fatty acids [25-29].
Manipulation of genes affecting traits of interest requires knowledge of their duplication status. Whole genome duplication is particularly relevant because it is common in plants, and because in the case of allopolyploidy it results in two or three independent copies of each gene. Allopolyploidy, such as found in wheat, cotton and peanut, is defined by the concurrent presence and maintenance in the same nucleus of two or more diploid genomes. In an allopolyploid, each chromosome pairs specifically to its own homolog, and not to any homoeolog, resulting in diploid inheritance [30,31]. Allopolyploids are usually formed by interspecific hybridization concurrent to genome duplication, but could also result from diploidization and divergence of genomic sets in an autopolyploid . Once formed, allopolyploids are relatively stable. Gene duplicates slowly decay over millions of years back to diploidy. For example, a distinct but partial duplication pattern still detectable in the Arabidopsis genome is thought to result from an approximately 25 million year old polyploidization event . The genomes of maize and soybean display widespread, but not universal duplication and are estimated to be 10 million year old polyploids [33,34]. Polyploids in which gene loss has advanced so far that duplication is no longer universal have been defined "paleopolyploids" although this term carries no precise temporal definition and could be extended to all known sequenced diploid angiosperms. Gene duplication is thus universal in a recent polypoid and becomes less and less pervasive in older polyploids as duplicates decay back to singletons. For a set of nearly 1000 genes the singleton pattern can be confirmed in all major sequenced diploid species .
We report the sequences of three copies of both FAE1 and FAD2 recovered from C. sativa. We used Southern blots to determine whether the recovered copies are allelic or if they represent multiple loci. Moreover, we performed phylogenetic analyses to infer the evolutionary history of the copies, and quantitative PCR (qPCR) to explore whether there is evidence of functional divergence among them. To better understand the C. sativa genome and to determine whether the multiple copies recovered are the result of polyploidization, we analyzed the genome sizes of C. sativa and its closest relatives in the genus Camelina by flow cytometry. Finally, we used next generation RNA sequencing data to demonstrate that well-characterized single-copy genes are present in triplicates. Collectively our results indicate that C. sativa is a hexaploid whose oil composition is likely influenced by more than one functional copy of FAE1 and FAD2. Thus in C. sativa, oil composition as well as other traits are likely to be determined by multiple copies of causative genes.
As a first step to characterize genes involved in fatty acid biosynthesis, we determined the copy number of FAD2 and FAE1 by Southern blot analysis. Since C. sativa is closely related to Arabidopsis thaliana [3,4], we designed primers based on Arabidopsis genomic sequence that amplified conserved regions of FAD2 and FAE1 (Additional File 1). Using these primers, we PCR amplified products of 225 base pairs (bp) (FAD2) and 403 bp (FAE1) from Arabidopsis and from C. sativa. The C. sativa products were cloned, sequenced, and compared with Arabidopsis FAD2 and FAE1 sequences  to confirm their identities. We used the C. sativa fragments as probes in Southern blot experiments (Figure (Figure1).1). Results of the Southern blots revealed three bands in C. sativa for both FAD2 (Figure (Figure1A)1A) and FAE1 (Figure (Figure1B),1B), whereas hybridization revealed only a single band in Arabidopsis for both genes (Figure (Figure1A1A &1B). These results suggest that FAD2 and FAE1 occur in at least three copies in C. sativa, while they are single copy in Arabidopsis . Fatty acid genes can be multi-copy in many species, including soybean , Brassica napus , olive (Olea europaea) , maize , and sunflower . Therefore, we designed a probe for Southern blot hybridization of the gene LEAFY (LFY), which is known to be single copy in a wide variety of species from several plant families . Three bands were observed following hybridization with the LFY probe of the same blot as was used for FAD2 and FAE1, suggesting LFY also exists as three copies in C. sativa (Figure (Figure1C1C).
We cloned and sequenced the full length genomic and cDNA sequences of C. sativa FAD2 and FAE1. Using primers designed from Arabidopsis FAD2 and Crambe abyssinica FAE1 (Additional File 1), we PCR amplified a band of approximately 1.2 kb for FAD2 and 1.5 kb for FAE1 from C. sativa. For each gene, we sequenced more than 60 clones. Three different versions of both CsFAD2 and CsFAE1 were recovered and designated A, B, and C. It should be noted that the A, B, and C copies were named independently for CsFAD2 and CsFAE1, and thus are not associated with a particular genome.
The three copies of C. sativa FAD2 are 1155 bp long, lack introns in the coding regions, are 97% identical at the nucleotide level, and encode proteins that are 99% identical in sequence (Table (Table1).1). One of the CsFAD2 copies, CsFAD2 A, contains a BamHI site (see Additional File 2), and thus this copy likely produced the smallest fragment in the Southern blot hybridization of FAD2 (Figure (Figure1A;1A; BamHI + EcoRI digest). The C. sativa nucleotide sequences of FAD2 are greater than 93% identical to Arabidopsis FAD2, and the putative encoded proteins from the two species share greater than 96% identity (Table (Table11).
The 5' untranslated region (utr) was recovered for all three copies of CsFAD2 by rapid amplification of cDNA ends (RACE) PCR. We then used primers designed from the 5' utr sequence (Additional File 1) to amplify an approximately 1.4 kb intron found within the 5' utr from all three copies of C. sativa FAD2. A similarly sized intron is present in Arabidopsis  and in Sesamum indicum (sesame) where it has been shown to be involved in regulating FAD2 expression .
All three copies of FAE1 in C. sativa are 1518 bp long and lack introns. When the nucleotide sequences and the putative encoded proteins of the three copies are compared they are more than 96% identical (Table (Table1).1). In comparison to Arabidopsis, the nucleotide sequences are more than 90% identical, while the encoded proteins are more than 91% identical (Table (Table1).1). Thus, the three copies of C. sativa FAD2 and the three copies of FAE1 are highly similar to each other and to their putative orthologs from Arabidopsis.
We aligned translated amino acid sequences from the three copies of C. sativa FAD2 with the FAD2 protein sequences from Arabidopsis; Brassica rapa, an agronomically important member of the Brassicaceae family; Glycine max, an agronomically important dicot; and Zea mays, an agronomically important monocot (Figure (Figure2A).2A). All three copies of C. sativa FAD2 have the three conserved HIS boxes found in all membrane-bound desaturases  as well as the ER localization signal described by McCartney et al . Furthermore, the conserved amino acids identified in an alignment of the FAD2 sequences from 34 different species  are also present in C. sativa with the exception of a positively-charged histidine at position number 44, which is substituted by a polar, uncharged glutamine in C. sativa. When we amplified the FAD2 gene from several Camelina and outgroup species and aligned the translated amino acid sequences, we found that the FAD2 proteins from Capsella rubella, Camelina microcarpa, Camelina laxa, and one copy from Camelina rumelica contain a glutamine at amino acid position 44, while the FAD2 proteins from Arabidopsis lyrata, Camelina hispida, and a second copy from Camelina rumelica contained a histidine (Additional File 3).
We aligned the translated amino acid sequences from the three copies of C. sativa FAE1 with the seed-specific FAE1 proteins from Arabidopsis, Crambe abyssinica, a high and low erucic acid Brassica rapa, Limnanthes alba, and Tropaeolum majus (Figure (Figure2B).2B). L. alba and T. majus are both in the order Brassicales and their seeds accumulate high levels of very long chain fatty acids [47,48]. Four conserved histidine residues and six conserved cysteine residues, including the active site at cysteine 223, as well as an asparagine residue at 424 required for FAE1 acitivity were previously identified by Ghanevati and Jaworski [49,50]. All conserved residues were found to be present in all three copies of C. sativa FAE1. More differences were apparent between the three C. sativa FAE1 sequences and the other FAE1 sequences than observed in the FAD2 comparison (Figure (Figure2A2A and and2B),2B), an observation consistent with the level of amino acid identity seen between Arabidopsis and C. sativa FAD2 versus FAE1 (Table (Table11).
The conservation of amino acids as well as the presence of the 5' regulatory intron in CsFAD2 suggests that all three copies of CsFAD2 and CsFAE1 could be functional. To determine whether these genes are also expressed, we first evaluated total CsFAD2 and CsFAE1 gene expression in developing seeds and in seedling tissue using real time quantitative PCR (qPCR) with primer/probe combinations designed to detect all three copies of each gene (Additional File 4). CsFAD2 expression in seedling tissue is present but minimal (0.4% of that seen in seeds at 20 days post-anthesis (DPA)), while CsFAE1 expression could not be detected in seedlings (Figure (Figure3A3A and and3B).3B). In developing seeds, both CsFAD2 and CsFAE1 expression peaks at 20 DPA and is reduced by 30 DPA (Figure (Figure3A3A and and3B).3B). In Arabidopsis, FAD2 peaks earlier and decreases sooner than FAE1 .
We wondered whether the expression of each of the FAD2 and FAE1 copies present in C. sativa are equally or differentially expressed in the seed. Duplicated genes are frequently silenced either throughout the plant or in a tissue-specific manner [52-55]; hence we hypothesized that one or more of the copies of each gene could be significantly down-regulated. We used the Sequenom MassARRAY™ method for determining allele-specific expression of a gene  to evaluate the relative expression of each of the copies of CsFAD2 and CsFAE1. We identified at least three single nucleotide polymorphisms (SNPs) specific to each of the CsFAD2 A, B, and C and the CsFAE1 A, B, and C copies (Additional File 5) and then calculated the frequency of each SNP in seed cDNA. Controls consisting of the cloned CsFAE1 A, B, and C copies combined to known frequencies showed that the method is greater than 80% accurate (data not shown). No evidence of silencing of any particular copy of either CsFAE1 or CsFAD2 was discovered. We did observe differential expression, especially of CsFAE1 A, which accounts for approximately 40-50% of CsFAE1 expression in seeds at 20-30 DPA (Figure (Figure3C3C and and3D3D).
To investigate whether the different copies of C. sativa FAD2 and FAE1 are the result of allelic variation or are in fact independent loci, we obtained sequence from the region upstream of CsFAE1 and downstream of CsFAD2. Assuming colinearity between C. sativa and Arabidopsis for the region around FAE1, we PCR amplified the region 5' to CsFAE1 using a forward primer for the upstream gene KCS17 with reverse primers for C. sativa FAE1 (Additional File 1). The resulting sequences we obtained for the putative C. sativa KCS17 were highly similar to the last 189 bp of Arabidopsis KCS17, suggesting that we had in fact amplified the orthologous C. sativa region upstream of FAE1, confirming colinearity between the two species. We then used a dot plot  to compare the three C. sativa upstream sequences to each other and to Arabidopsis with parameters set for perfect match on a sliding window of 9 bases (Additional File 6). The coordinates from the dot plot were used to define blocks of homology between Arabidopsis and the three C. sativa copies (Figure (Figure4).4). The results show a variable intergenic region containing potentially related blocks common to two or more genomes.
Colinearity with Arabidopsis was also found for a region downstream of FAD2 containing the ACTIN11 (ACT11) gene for two out of the three C. sativa copies (data not shown). For the third copy, the region downstream of CsFAD2 A could have been missed if the length of the amplified product was too large. Alternatively, the region downstream of CsFAD2 A might not exhibit colinearity with Arabidopsis and the possibility remains that two of the copies of CsFAD2 result from a tandem gene duplication.
To further explore the C. sativa genome, we determined the haplotype number of predicted single-copy genes in a 454 sequencing data set of cDNA expressed in 15 DPA C. sativa seeds. The reads were aligned to 956 genes identified by Duarte et al.  as single-copy genes shared in flowering plants. The six genes with the highest coverage (> 60 reads per gene) were selected for further evaluation. Remarkably, all 6 genes examined showed expression of three clear haplotypes (Additional File 7) as exemplified by the agmatine deiminase gene (Figure (Figure5),5), indicating that the triplication of the genes in the C. sativa genome is common and not limited to FAD2, FAE1, and LFY. When the genomic status of the same 6 genes was examined in the genomes of paleopolyploids such as maize and soybean, whose genome duplication is about 10 million years old [33,34], only a subset of these genes was retained as duplicates (Table (Table2).2). This lack of duplication in maize and soybean contrasted with the consistent pattern of triplication in C. sativa.
We calculated DNA content in several accessions of C. sativa and related species from flow cytometry analyses using propidium iodide-stained nuclei. We used Arabidopsis accession Col-0 (2X) and its tetraploid (4X) derivative as genome size standards. C. sativa, C. alyssum, and C. microcarpa diploid (2C) genomes had a haploid content between 650 and 800 Mb (Figure (Figure6).6). C. sativa accessions uniformly displayed a genome size close to 750 Mb. North American isolates of C. sativa, C. alyssum, and C. microcarpa have reported chromosome counts of n = 20 . The genomes of C. rumelica (600 Mb), C. hispida (300 Mb) and C. laxa (210 Mb) are smaller than those of C. sativa, C. alyssum, and C. microcarpa. Chromosome counts of both n = 6 [10,11] and n = 12  have been recorded for C. rumelica, while only a single count of n = 7 exists for C. hispida . To our knowledge, no published counts exist for C. laxa.
To understand the duplication history of the multiple FAD2 and FAE1 copies recovered from C. sativa, we amplified the FAD2 and FAE1 genes from several Camelina species and outgroup species, and inferred phylogeny for each gene. The sampling of taxa chosen allowed us to test whether FAD2 and FAE1 duplication events occurred after Camelina diverged from its closest relatives or within the genus. Results from the evaluation of 55 different models of sequence evolution using Modeltest 3.7  indicated that the FAD2 sequence data are best described by the TVM+I+Γ model, while the FAE1 data are best described by the HKY+I+Γ model. Likelihood phylogenetic analyses in PAUP* 4.b  produced a single FAD2 tree (-LnL 3665.277; Figure Figure7A),7A), and a single FAE1 tree (-LnL 5051.552; Figure Figure7B7B).
Phylogenies inferred from FAD2 and FAE1 data indicate a history of duplication for both markers. Both C. microcarpa and C. sativa have three distinct copies of FAD2 and FAE1. Moreover, for FAD2, the A and C copies from these two species are monophyletic with strong (100%) bootstrap support (bs); for FAE1 the A and B copies from these species are strongly monophyletic (100% bs). In contrast, neither the FAD2 B copies of C. sativa and C. microcarpa, nor the FAE1 C copies of these species form a monophyletic group with each other. Instead, our results indicate that C. rumelica has two distinct copies of FAD2 and that one of these copies (FAD2-2) is strongly monophyletic with C. microcarpa FAD2 B. We recovered only a single FAD2 copy for C. laxa and C. hispida. In contrast, we recovered at least two distinct copies of FAE1 from all sampled Camelina species. The FAE1-1 copy of C. laxa, C. hispida, and C. rumelica form a monophyletic group (91% bs), with the former two species sister to one another with strong support (100% bs). Similar to the results from FAD2, C. rumelica FAE1-2 is sister to one of the C. microcarpa copies (FAE1 C; 99% bs). Neither the C. sativa FAD2 B copy, nor the C. sativa FAE1 C copy, shows a well supported sister relationship to other FAD2 or FAE1 sequences. However, in the FAE1 tree, C. sativa FAE1 C is very weakly supported as sister to C. hispida FAE1-2 (53%). Finally, all recovered FAD2 and FAE1 copies from species of the genus Camelina are monophyletic and sister to other sampled members of the tribe Camelineae, consistent with phylogenies based on other markers [3,4].
Camelina sativa is a re-emerging oilseed with tremendous potential as an alternative biofuel crop and for which genomic information is becoming increasingly available. We have obtained molecular data for nine genes, characterized in detail two genes encoding fatty acid biosynthesis enzymes and, in the process, have discovered unexpected complexity in the C. sativa genome.
The close relationship between C. sativa and the model plant Arabidopsis thaliana [3,4] facilitates the manipulation of known pathways, such as the one regulating fatty acid biosynthesis. C. sativa seed oil is high in both polyunsaturated and long chain fatty acids [5,60,61], suggesting that both CsFAD2 and CsFAE1 are present and active. Three copies each of the FAD2 and FAE1 genes were isolated from an agronomic accession of C. sativa using primers designed from A. thaliana or Crambe abyssinica sequence. Previously identified conserved sites in CsFAD2 [44-46] and CsFAE1 [49,50,62] are present in all three copies of each gene and a 5' intron shown to be important in regulating FAD2 expression in sesame  was identified in all three CsFAD2 copies. Real time qPCR data and Sequenom MassARRAY SNP analysis of the CsFAD2 and CsFAE1 cDNA showed that all three copies of each gene are expressed in developing seeds. Thus, it seems likely that all three copies of FAD2 and FAE1 in C. sativa are functional.
The cloning of three copies of FAD2 and FAE1 from the C. sativa genome, as well as the observation of three LFY hybridization signals by Southern analysis and three expressed haplotypes for 6 more predicted single-copy genes in developing seeds, could be explained by at least two possible scenarios: segmental duplications of selected regions within a diploid genome either through tandem duplications or through transpositions, or whole genome duplications resulting from polyploidization. Segmental duplications or transpositions affecting all nine examined loci are improbable compared with the explanation of polyploidy. Furthermore, no evidence of recent segmental duplication involving multiple genes has been observed in sequenced plant genomes [36,63-65].
Triplication of the C. sativa genome therefore likely occurred through whole genome duplication, either through autopolyploidization or through allopolyploidization. An autopolyploidy event might have triplicated a single diploid genome resulting in an autohexaploid with a haploid genome of 18, 21, or 24 chromosomes. Given that C. sativa has a chromosome count of n = 20, chromosome splitting or fusion could then have increased the chromosomes from 18 to 20, or decreased the chromosomes from 21 or 24 to 20.
Alternatively, triplication of the C. sativa genome might have resulted from two allopolyploidy events, resulting in first a tetraploid then a hexaploid, similar to the origin of cultivated wheat. According to this hypothesis, the three copies of each gene diverged in different diploid genomes before converging through polyploidy events. Taking into consideration the reported chromosome counts of various Camelina species, the basal chromosome number of the diploid parental species contributing to the C. sativa haploid genome of 20 chromosomes could be 7+7+6 or 8+6+6. The allopolyploid hypothesis is supported by the observation that C. sativa demonstrates diploid inheritance [2,66], as would be expected for an allopolyploid . A hexaploid C. sativa could also be derived from the combination of an autotetraploid and a diploid species if, in an autopolyploidized genome, homologous chromosomes differentiated so that the subsequent chromosome-specific pairing mimicked an allopolyploid genome in its diploid inheritance patterns. Regardless of its evolutionary path, the C. sativa genome appears organized in three redundant and differentiated copies and can be formally considered to be an allohexaploid.
Results from our phylogenetic analyses support a history of duplication for both FAD2 and FAE1 in Camelina. For FAD2, duplications were only recovered for C. sativa, C. microcarpa, and C. rumelica. These data are consistent with genome size data, which indicate that all three genomes are larger than C. laxa and C. hispida, from which only a single FAD2 copy was recovered. Taken together, the results suggest that C. sativa, C. microcarpa, and C. rumelica are likely polyploids. Given the slightly smaller genome size of C. rumelica, and the fact that we recovered only two FAD2 copies from it, the C. rumelica sampled may be tetraploid while C. sativa and C. microcarpa are hexaploid. Interestingly, in both the FAD2 and FAE1 trees, one copy each of C. rumelica and C. microcarpa are strongly supported as sister. Thus, trees from these genes indicate that C. rumelica and C. microcarpa are closely related. The various placement of C. microcarpa FAD2 and FAE1 copies can be explained if C. microcarpa is the result of a hybridization event between C. rumelica and a currently unsampled, and thus unidentified species of Camelina. Two of the three copies of both FAD2 and FAE1 are identical, or nearly identical, in C. sativa and C. microcarpa, suggesting that C. sativa and C. microcarpa share a parental genome. Thus, we suggest that a Camelina species we did not sample contributed its genome to the hybrid formation of both C. sativa and C. microcarpa. In the case of C. microcarpa, the hybridization event likely involved C. rumelica. Given the chromosome count of n = 6 for C. rumelica, we expect the other putative parent to have an x = 7 genome, and furthermore to be tetraploid at n = 14. Such a cross would result in the observed C. microcarpa genome, with chromosome count n = 20. Interestingly, C. hispida is the only species we sampled with a chromosome count of n = 7, however no strong relationship between C. hispida and C. microcarpa is inferred in either gene tree. However, we do infer a weak relationship between C. sativa and C. hispida in the FAE1 tree, and thus the possibility that C. hispida is involved in the polyploid formation of C. sativa should be explored further.
What is the age of the polyploidization events likely to have formed the C. sativa genome? A complete answer will require a better understanding of its genome, but two findings suggest a recent origin. First, the chromosome number of C. sativa is inconsistent with extensive karyotype evolution and likely represents the sum of the ancestral contributions. Second, paleopolyploids such as soybean and maize display duplication of many, but not all genes as a sizeable number have decayed to singleton state. In contrast, the presence of triplicates for nine test genes of C. sativa is consistent with high retention of duplicates, as expected in recent polyploids.
The likely allohexaploid nature of the Camelina sativa genome has multiple implications. Its vigor and adaptability to marginal growth conditions may result at least in part from polyploidy. Polyploids are thought to be more adaptable to new or harsh environments, with the ability to expand into broader niches than either progenitor [67,68]. Indeed, C. hispida and C. laxa, both of which are likely diploids, are found only in Turkey, Iran, Armenia, and Azerbaijan, while C. microcarpa and C. sativa are distributed throughout Asia, Europe, and North Africa and are naturalized in North America [8,69]. The mechanisms behind this increased adaptability are not completely understood, but have been attributed to heterosis, genetic and regulatory network redundancies, and epigenetic factors [30,70].
Allohexaploidy might also affect any potential manipulations of the C. sativa genome, such as introgression of germplasm or induced mutations. Introgression of an exotic germplasm could be facilitated by the type of polyploidy-dependent manipulations that are possible in wheat, a potentially comparable allohexaploid [71,72]. In addition, polyploids have displayed excellent response to reverse genomics approaches such as Targeting Induced Local Lesions inGenomes (TILLING) [73,74]. As in wheat, any recessive induced mutations could be masked by redundant homoeologous loci that have maintained function [75,76]. This mutation masking implies that multiple knockout alleles at different homoeologous sites can be combined to achieve partial or complete suppression of a targeted function [77,78]. We also expect that single locus traits, whether transgenic or not, will display diploid inheritance due to preferential intragenomic pairing.
In a hexaploid oilseed crop such as C. sativa, manipulations of oil composition and/or yield should therefore be possible through transgenic or reverse genetic approaches, or through other genome manipulations similar to those performed in wheat. For example, the characterization of FAD2 and FAE1 in C. sativa could enable the use of TILLING techniques to isolate C. sativa plants with mutations in each of the three identified copies of both genes. We expect these mutations to result in plants with reduced levels of polyunsaturated fatty acids or long chain fatty acids, possibly in a dosage dependent manner. This will allow us to manipulate the seed oil composition of C. sativa, potentially creating a broad spectrum of C. sativa varieties possessing useful biodiesel properties, thereby further increasing the utility of this emerging biofuel crop.
The discovery of triplication and divergence of genes that in known diploids are present in single copy, the cytometrically determined genome size of Camelina species, the pattern of relationship and inferred duplication history in the gene trees, together with the previously known chromosome counts for this taxon, indicate a likely allohexaploid genomic constitution. The characterization of genes encoding key functions of fatty acid biosynthesis lays the foundation for future manipulations of this pathway in Camelina sativa. Targeted manipulations of oil composition and general development of this crop, however, need to consider the implications of polyploidy and when possible take advantage of this common condition in crop plants.
Camelina sativa Cs11 and Cs32, and Arabidopsis thaliana ecotype Col-0 (Additional File 8) seeds were germinated on Arabidopsis Growth Media (1× Murashige and Skoog (MS) mineral salts, 0.5 g/L MES, 0.8% PhytaBlend™ all from Caisson Labs, North Logan, UT; pH5.7) and allowed to grow for ~2 weeks under 16/8 hours day/night, 22/18°C and ~130 μE m-2 s-1 light intensity. A third Camelina sativa sample consisted of Cs32 leaf tissue from a fully grown plant (~1 month old) that allowed us to obtain a larger amount of DNA from a single plant. Genomic DNA was isolated according to the CTAB method  and 10 μg was digested overnight (~16 h) with EcoRI or a combination of EcoRI plus BamHI. DNA electrophoresis and blotting were carried out using standard molecular biology techniques . The probe was labelled with α-32P dCTP according to instructions of the DECAprime II kit (Ambion, Austin, TX). Hybridization was carried out overnight at 42°C. The blot was washed (30 minutes each) at 42°C in 2 × SSC, 0.1% SDS, followed by 55°C in 2 × SSC, 0.1% SDS, and then 55°C in 0.1 × SSC, 1% SDS, and exposed to a phosphorimager screen. The same blot was hybridized with different probes after stripping the membrane in boiling 0.1% SDS for 20 minutes each time.
FAD2 and FAE1 genes were amplified from C. sativa Cs32 DNA isolated as described above, using Pfu DNA polymerase (Stratagene, La Jolla, CA) and the primers listed in Additional File 1 with a PCR machine set for 30 cycles at 58°C annealing temperature and extension time of 3 minutes. For FAD2, buffer A from the SureBand PCR optimization kit (Bioline, Tauton, MA) was used. All intergenic regions were isolated using Phusion polymerase (New England Biolabs, Ipswich, MA). For the initial clones of the CsKCS17-CsFAE1 intergenic region, as well as the CsFAD2-CsACT11 intergenic region, the Phusion polymerase 3-step PCR protocol with an annealing temperature of 60°C, an extension time of 3 minutes, and 40 cycles was used. A Phusion polymerase 3-step PCR with annealing temperature of 60°C, extension time of 1 minute, and 30 cycles was used to obtain more clones for CsKCS17-CsFAE1 intergenic regions "B" and "C", while an annealing temperature of 55°C, extension time of 2 minutes and 30 cycles was used to obtain CsKCS17-CsFAE1 intergenic region "A". RACE PCR was performed using the SMART™ RACE cDNA Amplification kit and Advantage 2 Polymerase (Clontech, Mountain View, CA) according to the accompanying directions. All the amplified fragments were cloned using the Zero Blunt PCR Cloning kit (Invitrogen, Carlsbad, CA.)
Translated amino acid FAD2 and FAE1 sequences were aligned with AlignX (Invitrogen), with a gap opening penalty of 15, a gap extension penalty of 6.66, and a gap separation penalty range of 8. Alignments were imported into Boxshade  to highlight the conserved residues.
C. sativa Cs32 plants were grown under 24/18°C day/night conditions with a 16/8 hour photoperiod. Flowers were tagged and embryos harvested at the time points indicated. RNA was then isolated using the urea LiCl method described by Tai et al . cDNA were prepared from 0.5 μg of DNAsed RNA that was reverse transcribed with the High Capacity cDNA RT kit (Applied Biosystems, Foster City, CA) using random primers according to the manufacturer's instructions.
Relative expression of CsFAD2 and CsFAE1 cDNA was measured by real time qPCR and calculated according to the comparative CT method (2-ΔΔCT). In brief, separate reactions were prepared in duplicate or triplicate for each of the genes to be measured. Each reaction contained 8 μl of the appropriate primers (200 nM each) and probe (900 nM) listed in Additional File 4 for CsACTIN (reference gene) or CsFAD2 or CsFAE1 (target genes); 10 μl of Applied Biosystems 2× fast Taqman PCR mix; 2 μl of cDNA. The reactions were run on an Applied Biosystems 7900HT according to the manufacturer's fast PCR method.
Three single nucleotide polymorphisms (SNPs) for each of CsFAD2 A, B, and C and CsFAE1 A, B, and C were identified. Each identified SNP distinguishes one copy from the other two. An additional SNP, which distinguishes FAE1 A, B, and C copies from each other, was also identified (Additional File 5). SNP frequencies were determined in cDNA isolated as described above by the Sequenom MassARRAY™ allele-specific expression analysis method with no competitor, as described in Park et al .
Approximately 150 μg of total RNA from 15 DPA Camelina sativa CS32 seed was isolated as described above and sent to Agencourt Bioscience (now known as Beckman Coulter Genomics, Danvers, MA) for isolation of mRNA, library construction and 454 sequencing, according to their established protocols.
The cDNA sequences of the 956 single copy genes were obtained from the TAIR8 cDNA set using in each case the first cDNA model (ATNG00000.1). To compare this set of single copy genes to the 454 transcriptome data, an analysis was carried out by running the BLASTALL program version 2.2.16  in the UNIX environment of an Apple Powerbook Pro. The 956 sequences were BLASTed against a database made of all the 454 sequence reads. Alignment results with an E value > 10-11 were saved and parsed to eliminate reads that had single instances of SNP or indels and to rank the genes according to the number of read hits. The six genes that aligned to more than sixty reads were examined to identify "haplotypes" indicative of two or more copies.
Camelina lines (Additional File 8) were grown in the greenhouse at temperatures fluctuating between 16°C and 26°C with 16 hour day length supplemented by halogen lights. The nuclei were extracted from leaves according to Henry et al . Nuclei were also extracted from approximately 50 seeds of all species, except C. laxa and C. hispida, which are late flowering. The seeds were crushed with a pestle in 1.4 mL of the same extraction buffer used for the leaves. The fluid was then drawn through four layers of cheesecloth and strained and processed as for the leaf nuclei. Nuclei of diploid and tetraploids of Arabidopsis thaliana accession Col-0 (1 C genome size 157 Mb and 314 Mb, respectively ), and tetraploid Arabidopsis arenosa accession Care-1 (1C genome size 480 Mb [Dilkes, unpublished results]) were used as standards for DNA content. Data was collected on two different days and normalized separately to account for daily fluctuations in flow cytometer performance. The 2C, 4C, and 8C nuclear peaks were used in a regression analysis of measured fluorescence intensity versus nuclear DNA content, producing equations of genome size versus fluorescence that were used to estimate the 2C content of Camelina nuclei.
FAD2 and FAE1 were PCR amplified from several Camelina species and outgroups (Additional File 8) using primers designed from C. sativa FAD2 and FAE1 sequences (Additional File 1). Amplified fragments for FAD2 and FAE1 were cloned as described for C. sativa above, then aligned by translated amino acid sequences using MacClade 4.05 . ModelTest 3.7  in PAUP* 4.0 b  was used to determine the model of sequence evolution favored by the data for each gene. Subsequent maximum likelihood (ML) analyses were performed in PAUP* 4.0 b using a heuristic search with tree bisection reconnection (TBR) branch swapping. ML clade support using 100 bootstrap data sets were assessed and this support is presented on the most likely tree recovered from the ML heuristic search.
FAD2 and FAE1 sequences from Camelina species and outgroups have been deposited in Genbank at the NCBI [Genbank: GU929417 - GU929441].
CH carried out the amplification of C. sativa and Camelinae genomic sequences, participated in the sequence alignment, and helped draft the manuscript. RFD carried out the Southern blot analysis and the amplification of C. sativa genomic sequences, participated in the sequence alignment, and helped draft the manuscript. MB carried out the phylogenetic analyses and helped draft the manuscript. LC participated in the design and analysis of the study, analyzed the 454 transcriptome data, and helped draft the manuscript. JS carried out the qPCR analyses. EG carried out the flow cytometry analysis. CKS participated in the sequence alignment, in the design of the study, and helped draft the manuscript. TN, JD, and JK conceived of the study. All authors read and approved the final manuscript.
Primers used for amplification of genomic regions of C. sativa. Table of primers used in the amplification of genomic regions of Camelina sativa
FAD2 and FAE1 nucleotide alignments. (A) Nucleotide sequence comparison of the three Camelina sativa FAD2 sequences and the Arabidopsis thaliana FAD2 sequence [Genbank: NM_112047]. Green underlines indicate the start and stop codons, the blue underline indicates the BamHI site in CsFAD2 A and AtFAD2, the orange underline indicates the ER localization signal, and the grey underline indicates the glutamine at amino acid position 44. The three His boxes described by Tocher et al  are indicated with red boxes. (B) Nucleotide sequence comparison of the three Camelina sativa FAE1 sequences and the Arabidopsis thaliana FAE1 sequence [Genbank: NM_119617]. Green underlines indicate the start and stop codons. Blue underlines below the sequence indicate the asparagine at amino acid position 424 and the highly conserved histidine and cysteine residues described by Ghanevati and Jaworski [49,50]. The red box indicates the region highly conserved among condensing enzymes in very long chain fatty acid biosynthesis 
Camelineae FAD2 and FAE1 protein alignment. (A) Amino acid sequence comparison of FAD2 sequences from species in the tribe Camelineae. The amino acid at position 44 is indicated with a blue underline while the green underline indicates the ER localization signal . The three His boxes described by Tocher et al  are indicated with red boxes. The Arabidopsis thaliana FAD2 sequence was obtained from Genbank [Genbank:NP_187819]. (B) Amino acid sequence comparison of FAE1 sequences from species in the tribe Camelineae. Blue underlines below the sequence indicate the asparagine at amino acid position 424 and the highly conserved histidine and cysteine residues described by Ghanevati and Jaworski [49,50]. The red box indicates the region highly conserved among condensing enzymes in very long chain fatty acid biosynthesis . The Arabidopsis thaliana FAE1 sequence was obtained from Genbank [Genbank:NP_195178].
Primers used for qPCR analyses. List of primers used for qPCR analyses
SNPs distinguishing each copy of CsFAD2 and CsFAE1. List of SNPs used in Sequenom MassARRAY™ analyses to distinguish the three copies of CsFAD2 and of CsFAE1
Dot plots of KCS17-FAE1 intergenic region. Sequences obtained for CsKCS17-FAE1A, B and C were aligned with each other and with Arabidopsis orthologous region two at a time in a dot plot with parameters set for perfect conservation on a sliding window of 9 bases.
Deep sequencing reads for 6 predicted single-copy genes in C. sativa. Sequences determined by 454 sequencing of cDNA from 15 DPA C. sativa seeds, aligned with 6 genes predicted by Duarte et al  to be single-copy in flowering plants.
Plant species and sources. List of plant species used and their sources.
We are grateful to Dr. Marta Janer and Sarah Li from the Institute for Systems Biology, Seattle, WA for performing the Sequenom MASSArray™ analysis. We would also like to thank Teresa Stutzman for collecting C. sativa embryos for the qPCR study and Breanne Piehl for her help cloning Camelinae FAD2 and FAE1 sequences.