Isolation and Characterization of Canthaxanthin Biosynthesis Genes from the Photosynthetic Bacterium Bradyrhizobium sp. Strain ORS278

doi:10.1128/JB.182.13.3850-3853.2000

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Journal of Bacteriology, July 2000, p. 3850-3853, Vol. 182, No. 13
0021-9193/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Isolation and Characterization of Canthaxanthin Biosynthesis Genes from the Photosynthetic Bacterium Bradyrhizobium sp. Strain ORS278

Laure Hannibal,¹ Jean Lorquin,²^, Nicolas Angles D'Ortoli,¹ Nelly Garcia,¹ Clemence Chaintreuil,¹ Catherine Masson-Boivin,¹ Bernard Dreyfus,¹ and Eric Giraud¹^,^*

Laboratoire des Symbioses Tropicales et Méditerranéennes, IRD, CIRAD, AGRO-M, INRA, 34398 Montpellier, France,¹ and Laboratoire de Microbiologie des sols, IRD/ISRA, 1386 Dakar, Senegal²

Received 2 February 2000/Accepted 17 April 2000

	ABSTRACT

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A carotenoid biosynthesis gene cluster involved in canthaxanthin production was isolated from the photosynthetic Bradyrhizobiumsp. strain ORS278. This cluster includes five genes identifiedas crtE, crtY, crtI, crtB, and crtW that are organized in at leasttwo operons. The functional assignment of each open reading framewas confirmed by complementationstudies.

	TEXT

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Bradyrhizobium strains isolated from Aeschynomene stem nodules are photosynthetic (4; see reference 6 for a review),which is a rare trait in Rhizobium bacteria. These strains exhibita photoheterotrophic and strictly aerobic photosynthesis (6;A. Vermeglio, personal communication). In culture, most of thesestem isolates show the same pink coloration, while a few strainsproduce orange pigmentation (12, 16). Pigment analyses showedthat bacteriochlorophyll and spirilloxanthin, two pigments ofthe light harvesting system, are common to all of these photosyntheticBradyrhizobium strains, whereas orange strains produce an additionalbicyclic carotenoid, canthaxanthin (4,4'-diketo- $beta$ -carotene) (12).This was the first report on the presence of this carotenoid inphotosynthetic bacteria. Bradyrhizobium sp. strain ORS278 producesthe highest quantity of canthaxanthin of all tested photosyntheticbacteria; canthaxanthin represents 85% of its total carotenoidcontent (12).

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FIG. 1. Scheme of the canthaxanthin (15) and spirilloxanthin (20) biosynthesis pathways.

Contrary to anaerobic purple phototrophic bacteria, aerobic phototrophic bacteria synthesize an unusually diverse varietyof carotenoids, including photosynthetic carotenoids such as spirilloxanthinor spheroidenone, and often a large amount of bicyclic carotenoid( $beta$ -carotene and hydroxyl derivatives) (24; see reference 26for a review). These carotenoids were shown to not be bound tothe photosynthetic apparatus of these aerobic bacteria (17,27) and their function is still unclear $---$ they could have a protectiverole against photo-oxidative damage, as already observed for severalcarotenoids (19, 25).

Synthetic canthaxanthin is applied for both direct and indirect food coloring (10, 23). In cosmetology and pharmacology,it is also combined with $beta$ -carotene for use as a dermal photoprotector(8). Canthaxanthin is, therefore, a pigment of high economicvalue, but its level in Bradyrhizobium sp. strain ORS278 (1.43mg/g of dry cell weight) remains insufficient for this organismto be a realistic candidate for natural canthaxanthin production(12). However, it could be possible to enhance the productionof canthaxanthin by cloning carotenoid biosynthesis genes of thisstrain.

In this paper, we describe the cloning and characterization of the canthaxanthin gene cluster of Bradyrhizobium sp. strainORS278.

Isolation of a carotenoid gene cluster. The genes crtB and crtI, encoding, respectively, phytoene synthase and phytoene desaturase, two enzymes involved in the initialsteps of carotenoid biosynthesis (Fig. 1), have been isolatedand characterized in various microorganisms (1, 9, 11,14, 15, 21). In all of these cases, these genes were foundto be adjacent and oriented in the same direction. Comparisonof the deduced amino acid sequences of the CrtI and CrtB proteinsfrom Erwinia uredovora, Erwinia herbicola, Flavobacterium sp.strain ATCC 21588, Rhodobacter sphaeroides, and Agrobacteriumaurantiacum revealed well-conserved domains at the C-terminalend of CrtI (LVGAGTHPG) and in the central region of CrtB (QLTNIARD).These motifs were chosen for designing the degenerated primersCrtIf (5'-GTNGGNGCRGGCACNCAYCC-3') and CrtBr (5'-TCGCGRGCRATRTTSGTSARRTG-3').PCR amplification was performed with a Perkin-Elmer model 2400thermocycler in a 50-µl (total volume) reaction mixture containing100 ng of strain ORS278 genomic DNA, each deoxynucleotide triphosphate(200 µM), primers (0.8 µM each), MgCl₂ (1.5 mM), 1.25 U of TaqDNA polymerase (Promega, Charbonières, France), and the buffersupplied with the enzyme. A touchdown PCR (3) was done as follows:initial denaturation at 94°C for 5 min followed by 20 cycles consistingof a 30-s denaturation at 94°C, 30 s at an annealing temperatureof 60 to 50°C, and a 1-min primer extension at 72°C, followedby 15 cycles consisting of a 30-s denaturation at 94°C, 30 s atan annealing temperature at 50°C, and a 1-min primer extensionat 72°C. After the final elongation step at 72°C for 7 min, theamplified 620-bp fragment obtained (probe A) was purified by aWizard procedure and was ligated into a pGEM-T vector (Promega).The ABI Prism BigDye Terminator Cycle Sequence Kit (Applied Biosystems,Foster City, Calif.) was used to sequence the cloned PCR productwith the universal oligonucleotides M13 forward and M13 reverse.Sequencing reactions were analyzed on an Applied Biosystems model310 DNA sequencer. The sequence of the amplified 620-bp fragmentwas highly similar to known CrtB sequences at the amino acidlevel.

Two specific primers, CrtIBfow.ORS278 (5'-ATTCGCAGCGGCTCGAAGAG-3') and CrtIBrev.ORS278 (5'-GATCGCCGACATCATCACGC-3'), basedon the sequence of the amplified DNA fragment, were designed forPCR screening of a library of the ORS278 strain constructed withthe SuperCos I cosmid vector kit (Stratagene, La Jolla, Calif.),as instructed by the manufacturer. Four positive clones were isolatedand confirmed by Southern blot analysis by using the 620-bp fragmentas a probe. Clone pSTM73, containing an insert of approximately35 kb, was used to characterize this crt genecluster.

Structure of the canthaxanthin crt gene cluster. A 6.5-kb region in the inserted DNA fragment of the pSTM73 cosmid, showing a positive hybridization signal to probe A, wassequenced and analyzed as shown in Fig. 2. This nucleotide sequencehad five open reading frames (ORFs) encoding proteins with similarityto known Crt enzymes (Fig. 3). Based on sequence similarity (45%amino acid identity with CrtY of E. herbicola), one of these ORFswas assigned to a crtY gene which encodes lycopene cyclase, akey enzyme that converts lycopene into the cyclic carotenoid $beta$ -carotene.Another ORF was similar in sequence to a crtW gene encoding a $beta$ -carotene ketolase that synthesizes canthaxanthin from $beta$ -carotenevia echinenone (15). This indicated that we had isolated a crtgene cluster involved in canthaxanthin biosynthesis. Four of thefive ORFs, identified as crtY, crtI, crtB, and crtW, were foundto be clustered in this order in the same orientation, whereasthe ORF crtE preceded these four but was oriented in the oppositedirection (Fig. 2). The crtY, crtI, and crtB genes are closelylinked physically; i.e., the stop codons of crtY and crtI overlapthe start codon of the following ORF, suggesting that these genesare translationally coupled (18). Note that the crtY, crtI,and crtB genes always occurred in this order and were orientedin the same direction in the other cyclic carotenoid biosynthesisclusters described previously (see Fig. 3).

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FIG. 2. Organization of the canthaxanthin biosynthesis gene cluster of Bradyrhizobium sp. strain ORS278 and locations of various subcloned fragments. The restriction fragments are inserted into pUC18 (pSTM108, pSTM107, and pSTM51) or pUC19 (pSTM462), the crt genes are transcribed from the lac promoter of the vector. In the plasmid pSTM78, the insert was obtained by Long PCR using the primers Crt.canta.f (5'-GCAACCGGTACCCGAGTTAATTCGCTCGGAATG-3') and Crt.canta.r (5'-ATGGTGAAGCTTATGCGGCAGCGGGTTTAGTC-3') and was cloned into pGEM-T (Promega). In pSTM78, the crtY, crtI, crtB, and crtW genes are under lac promoter control.

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FIG. 3. Comparison of the organization of the cyclic carotenoid gene clusters of Bradyrhizobium sp. strain ORS278, A. aurantiacum (15), Flavobacterium sp. strain R1534 (21), E. uredovora (14), and E. herbicola (9). Arrows represent the orientations of ORFs. The percentage values below the genes indicate the percentages of amino acid identity compared to Bradyrhizobium sp. strain ORS278.

Phylogenetic trees were constructed with available CrtI and CrtB sequences. The CrtB proteins (Fig. 4) and the CrtI proteins(data not shown) formed two distinct clusters which do not correlatewith the taxonomical position of the strains, but rather withthe nature of the carotenoid (cyclic or noncyclic) synthesizedunder the control of crtI and crtB. The fact that $alpha$ - and $gamma$ -Proteobacteriaand Flavobacteria group in the same cluster (Fig. 4) suggeststhat lateral gene transfer has occurred between these phylogeneticallyunrelated bacteria. Moreover, the fact that strain ORS278 genesare clustered with crtI and crtB genes from nonphotosyntheticstrains producing cyclic carotenoids rather than with photosyntheticstrains producing photosynthetic carotenoids raises the questionof whether an additional copy of the crtI and crtB genes involvedin the biosynthesis of spirilloxanthin does exist. The crtC andcrtD genes, which were reported to be involved in the biosynthesisof spirilloxanthin from lycopene (20), have just been isolatedin another cosmid which did not overlap the pSTM73 cosmid (E.Giraud and B. Dreyfus, unpublished data). We are currently investigatingif another copy of the crtI and crtB genes is physically linkedto these crtC and crtD genes, as has been found in photosyntheticbacteria (1, 11).

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FIG. 4. Phylogenetic tree based on the CrtB sequences and constructed by using the neighbor-joining method (22). Bootstrap values (5), expressed as percentages of 1,000 replications, are given at the branching points. P, Proteobacteria; F, Flavobacteria; a, bicyclic carotenoid; b, acyclic carotenoid; c, monocyclic carotenoid. GenBank accession numbers are as follows: AF218415, Bradyrhizobium sp. strain ORS278; D58420, A. aurantiacum; Y15112, Paracoccus marcusii; U62808, Flavobacterium sp.; M87280, E. herbicola EHO10; M90698, E. herbicola 557; D90087, E. uredovora; AF195122, R. sphaeroides; X52291, Rhodobacter capsulatus; U87626, Rubrivivax gelatinosus; Z211955, Myxococcus xanthus.

Carotenoid production in Escherichia coli transformants. E. coli transformants carrying the entire crt gene cluster of canthaxanthin from strain ORS278, cloned in pGEMT (pSTM78) orSuperCosI (pSTM73), did not produce any carotenoids (Table 1),suggesting that these genes are not expressed or that their productsare not functional in E. coli. Misawa et al. (15) constructedE. coli transformants which accumulate each precursor of the zeaxanthinbiosynthesis pathway by introducing various combinations of E.uredovora crt genes. To check the functionality of the differentORFs identified in strain ORS278, we complemented several carotenoid-accumulatingE. coli transformants with plasmids carrying various crt genesof strain ORS278 and analyzed carotenoids synthesized by high-pressureliquid chromatography (Table 1). The conditions were as follows:5-µm Hypersil C₁₈ column (250 by 4.6 mm; Alltech, Templemars,France), eluent of acetonitrile-methanol-isopropanol (85/10/5,vol/vol/vol), flow rate of 1 ml/min, and detection at 470 nm (450nm for $beta$ -carotene). Peaks were compared and coeluted with standardcompounds then identified by their visible spectra and partitioncoefficients (12).

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TABLE 1. Analysis of carotenoids accumulated in E. coli transformants carrying various combinations of crt genes from E. uredovora and Bradyrhizobium sp. strain ORS278^a

When plasmid pSTM78 carrying the complete crt cluster of Bradyrhizobium sp. strain ORS278 was introduced into the E. colitransformant that had accumulated geranylgeranyl pyrophosphate(GGPP) as a result of the presence of the crtE gene of E. uredovora,the new transformant obtained was shown to accumulate canthaxanthin.This result indicates that the crtY, crtI, crtB, and crtW genesare functional and allow the production of canthaxanthin in E.coli. Nevertheless, the amount of canthaxanthin produced remainslower than in the wild-type strain ORS278. When plasmid pSTM462carrying the crtE gene of Bradyrhizobium sp. strain ORS278 underthe lac promoter was introduced into an E. coli transformant containingthe crtI, crtB, and crtY genes of E. uredovora, the new transformantaccumulated $beta$ -carotene, showing the functionality of the crtEgene.

In this study, we cloned and characterized all of the crt genes of Bradyrhizobium sp. strain ORS278 necessary for canthaxanthinbiosynthesis. This is the first report of a cyclic carotenoidbiosynthesis gene cluster in a photosynthetic bacterium. It wouldbe interesting to determine the genetic links of this canthaxanthincrt gene cluster to the photosynthetic gene cluster. In Bradyrhizobiumsp. strain ORS278, canthaxanthin production is stimulated by light(13), suggesting that the expression of canthaxanthin biosynthesisgenes is regulated by photoinduction, as already reported forother pigments in different organisms (2, 7). Productionof this pigment could be optimized by identifying the signal transductionsystem controlling canthaxanthin biosynthesis. However, characterizationof the entire crt gene cluster necessary for canthaxanthin biosynthesisalready provides a basis for the construction of a recombinantstrain that could overproduce thiscarotenoid.

Nucleotide sequence accession number. The DNA sequence obtained in this study has been deposited in the GenBank database under accession no. AF218415.

	ACKNOWLEDGMENTS

We thank N. Misawa for kindly providing the plasmids carrying the crt genes of E. uredovora used in thisstudy.

	FOOTNOTES

^* Corresponding author. Mailing address: LSTM TA 10/J, Campus de Baillarguet, 34398 Montpellier Cedex 5, France. Phone: (33)467593783. Fax: (33) 467593802. E-mail: Giraud{at}mpl.ird.fr.

Present address: IRD, Université de Provence, 13288 Marseille,France.

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1.	Armstrong, A. G., M. Alberti, F. Leach, and J. E. Hearst. 1989. Nucleotide sequence, organization, and nature of the protein products of the carotenoid biosynthesis gene cluster of Rhodobacter capsulatus. Mol. Gen. Genet. 216:254-268[CrossRef][Medline].
2.	Bramley, P. M., and A. Mackenzie. 1988. Regulation of carotenoid biosynthesis. Curr. Top. Cell Regul. 29:291-343[Medline].
3.	Don, R. H., P. T. Cox, B. Wainwright, K. Baker, and J. S. Mattick. 1991. "Touchdown" PCR to circumvent spurious priming during gene amplification. Nucleic Acids Res. 19:4008[Free Full Text].
4.	Eaglesham, A. R. J., J. M. Ellis, W. R. Evans, D. E. Fleischman, M. Hungria, and R. W. F. Hardy. 1990. The first photosynthetic N₂-fixing Rhizobium: characteristics, p. 805-811. In P. M. Gresshoff, L. E. Roth, G. Stacey, and W. L. Newton (ed.), Nitrogen fixation: achievements and objectives. Chapman and Hall, New York, N.Y.
5.	Felsenstein, J. 1985. Confidence limits on phylogenies: an approach using the bootstrap. Evolution 39:783-791[CrossRef].
6.	Fleischman, D., and D. Kramer. 1998. Photosynthetic rhizobia. Biochim. Biophys. Acta 1364:17-36[Medline].
7.	Fontes, M., R. Ruiz-Vázquez, and F. J. Murillo. 1993. Growth phase dependence of the activation of a bacterial gene for carotenoid synthesis by blue light. EMBO J. 12:1265-1275[Medline].
8.	Goralczyk, R., S. Buser, J. Bausch, W. Bee, U. Zühlke, and F. M. Barker. 1997. Occurrence of birefringent retinal inclusions in cynomolgus monkeys after high doses of canthaxanthin. Investig. Ophthalmol. Vis. Sci. 38:741-752[Abstract/Free Full Text].
9.	Hundle, B., M. Alberti, V. Nievelstein, P. Beyer, H. Kleinig, G. A. Armstrong, D. H. Burke, and J. E. Hearst. 1994. Functional assignment of Erwinia herbicola Eho10 carotenoid genes expressed in Escherichia coli. Mol. Gen. Genet. 245:406-416[CrossRef][Medline].
10.	Kläui, H. 1982. Industrial and commercial uses of carotenoids, p. 309-328. In G. Britton, and T. W. Goodwin (ed.), Carotenoid chemistry and biochemistry. Pergamon Press, Inc., Oxford, England.
11.	Lang, H. P., R. J. Cogdell, A. T. Gardiner, and C. N. Hunter. 1994. Early steps in carotenoid biosynthesis: sequence and transcriptional analysis of crtI and crtB genes of Rhodobacter sphaeroides and overexpression and reactivation of crtI in Escherichia coli and R. sphaeroides. J. Bacteriol. 176:3859-3869[Abstract/Free Full Text].
12.	Lorquin, J., F. Molouba, and B. L. Dreyfus. 1997. Identification of the carotenoid canthaxanthin from photosynthetic Bradyrhizobium strains. Appl. Environ. Microbiol. 63:1151-1154[Abstract].
13.	Lorquin, J., F. Molouba, N. Dupuy, S. Ndiaye, D. Alazard, M. Gillis, and B. L. Dreyfus. 1993. Diversity of photosynthetic Bradyrhizobium strains from stem nodules of Aeschynomene species, p. 683-689. In R. Palacios, J. Mora, and W. E. Newton (ed.), New horizons in nitrogen fixation. Kluwer Academic Publishers, Dordrecht, The Netherlands.
14.	Misawa, N., M. Nagakawa, K. Kobayashi, S. Yamano, Y. Izawa, K. Nakamura, and K. Harashima. 1990. Elucidation of the Erwinia uredovora carotenoid biosynthetic pathway by functional analysis of gene products expressed in Escherichia coli. J. Bacteriol. 172:6704-6712[Abstract/Free Full Text].
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