Cloning and Characterization of Genes Involved in Nostoxanthin Biosynthesis of Sphingomonas elodea ATCC 31461

Liang Zhu; Xuechang Wu; Ou Li; Chaodong Qian; Haichun Gao

doi:10.1371/journal.pone.0035099

Abstract

Most Sphingomonas species synthesize the yellow carotenoid nostoxanthin. However, the carotenoid biosynthetic pathway of these species remains unclear. In this study, we cloned and characterized a carotenoid biosynthesis gene cluster containing four carotenogenic genes (crtG, crtY, crtI and crtB) and a β-carotene hydroxylase gene (crtZ) located outside the cluster, from the gellan-gum producing bacterium Sphingomonas elodea ATCC 31461. Each of these genes was inactivated, and the biochemical function of each gene was confirmed based on chromatographic and spectroscopic analysis of the intermediates accumulated in the knockout mutants. Moreover, the crtG gene encoding the 2,2′-β-hydroxylase and the crtZ gene encoding the β-carotene hydroxylase, both responsible for hydroxylation of β-carotene, were confirmed by complementation studies using Escherichia coli producing different carotenoids. Expression of crtG in zeaxanthin and β-carotene accumulating E. coli cells resulted in the formation of nostoxanthin and 2,2′-dihydroxy-β-carotene, respectively. Based on these results, a biochemical pathway for synthesis of nostoxanthin in S. elodea ATCC 31461 is proposed.

Citation: Zhu L, Wu X, Li O, Qian C, Gao H (2012) Cloning and Characterization of Genes Involved in Nostoxanthin Biosynthesis of Sphingomonas elodea ATCC 31461. PLoS ONE 7(4): e35099. https://doi.org/10.1371/journal.pone.0035099

Editor: Eric A. Johnson, University of Wisconsin, Food Research Institute, United States of America

Received: December 7, 2011; Accepted: March 8, 2012; Published: April 11, 2012

Copyright: © 2012 Zhu et al. This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.

Funding: The authors have no support or funding to report.

Competing interests: The authors have declared that no competing interests exist.

Introduction

Carotenoids are isoprenoid pigments that are widely distributed in nature [1]. They can be synthesized by all known phototrophic organisms and by some non-phototrophic fungi, bacteria, and archaea [1], [2]. Due to their unique physiochemical properties, they have diverse biological functions in different organisms that either produce or consume them. These functions include their anticarcinogenic and antioxidant activity, protection against photo-oxidative damage, contribution to the light-harvesting process in photosynthesis, provitamin A property of β-carotene and as nutritional factors important for chronic disease prevention [3]–[5]. The interesting properties and beneficial effects on human health have drawn much attention. Over recent years, some identified carotenoids have been used as colorants, nutritional supplements and nutraceuticals for food, cosmetic and pharmaceutical purposes [6].

Carotenoid biosynthetic pathway has been extensively studied in various organisms and remarkable progress has been made. All carotenoids are derived from the isoprenoids pathway. The first step in the carotenoid biosynthetic pathway is the formation of geranylgeranyl pyrophosphate (GGPP) from farnesyl pyrophosphate (FPP) by GGPP synthase. Then two GGPP molecules are condensed head to head by phytoene synthase, resulting in the formation of the first carotene phytoene. After phytoene formation the biosynthetic pathways vary in different organisms resulting in a wide carotenoid diversity. In most bacteria, the colorless phytoene is desaturased by the phytoene desaturase through four consecutive steps to produce the red pigment lycopene. Various further modifications by cyclases, hydroxylases, ketolases and other enzymes lead to the formation of different carotenoids [7]–[9].

Sphingomonas elodea ATCC 31461 (originally designated as Pseudomonas elodea, also referred to as Sphingomonas paucimobilis) was isolated as a Gram-negative bacterium capable of producing gellan gum [10]. It synthesizes a yellow carotenoid identified as nostoxanthin ((2R,3R,2′R,3′R)-β,β-Carotene-2,3,2′,3′-tetrol) [11]. Nostoxanthin is a poly-hydroxy derivative of β-carotene isolated only from some prokaryotes, including some species of cyanobacteria [12], the novel bacteriochlorophyll a-containing bacterium Sandarakinorhabdus limnophila [13], the moderately thermophilic aerobic photosynthetic bacterium Porphyrobacter tepidarius [14], the marine bacterium Brevundimonas sp. strain SD212 [15], the strictly aerobic photosynthetic bacterium Erythrobacter longus [16], and most Sphingomonas species [11]. Although all the necessary genes required to synthesize nostoxanthin have been identified from Brevundimonas sp. strain SD212, Brevundimonas vesicularis strain DC263 and Thermosynechococcus elongatus strain BP-1 [12], [15], [17], genetic data on nostoxanthin biosynthesis are limited and the carotenoid biosynthetic pathway of Sphingomonas species remains unclear.

We previously cloned and identified the crtI gene encoding phytoene desaturase in S. elodea ATCC 31461 [18]. In the present study, we describe the cloning and characterization of the other genes involved in the nostoxanthin biosynthetic pathway of this organism. Using gene inactivation together with chromatographic and spectroscopic analysis of the pigments, we determined the functions of four carotenoid biosynthesis genes. In particular, the crtG gene encoding the 2,2′-β-hydroxylase, was also found in the carotenoid biosynthesis gene cluster of S. elodea ATCC 31461. Moreover, the functions of the two hydroxylase genes, crtZ and crtG, both responsible for hydroxylation of β-carotene were confirmed by complementation studies using Escherichia coli producing different carotenoids. As a result, the nostoxanthin biosynthetic pathway has been proposed.

Results

Cloning of the nostoxanthin biosynthetic genes

From SiteFinding-PCR [19], a 9.6-kb fragment containing a carotenoid biosynthesis gene cluster was obtained by assembly of the PCR products. However, the crtZ gene is not contained as a member of this cluster. Although we performed several rounds of SiteFinding-PCR (obtained about 22 kb sequence data), we could not amplify the crtZ gene. Because the crtZ gene is not linked to the carotenoid biosynthesis gene cluster, the CODEHOP strategy was used to generate PCR primers for partial crtZ fragment amplification. An internal crtZ fragment of 266 bp was isolated by PCR amplification using primers deduced from conserved internal domains of CrtZs of sphingomonadales (see Materials and Methods), providing sequence information for designing specific primers for SiteFinding-PCR that generated full-length crtZ. Sequences have been deposited in GenBank under accession number JN224892 for the carotenoid biosynthesis gene cluster and JN224893 for crtZ.

Sequence analysis of the nostoxanthin biosynthetic genes

The carotenoid biosynthesis gene cluster is 8,412 bp long and contains 7 putative ORFs. Based on the alignments of the deduced amino acid sequences with those of known carotenogenic enzymes, four of these ORFs were respectively identified as putative genes encoding carotenoid biosynthetic enzymes (Table 1). The translated amino acid sequence of ORF3 showed the highest sequence identity (55%) to Caulobacter crescentus CB15 TonB-dependent receptor. The deduced amino acid sequences of the other two ORFs (ORF2 and ORF6) exhibit no overall homology with any other known enzymes. These four carotenogenic genes have been tentatively assigned as crtG, crtY, crtI and crtB, encoding respectively putative 2,2′-β-hydroxylase, lycopene cyclase, phytoene desaturase and phytoene synthase. Similar to other Sphingomons genes, the carotenogenic genes displayed a high GC content (66% to 73%), and a high frequency of G or C in the position of codons [20]. The gene direction and the percent amino acid identity were compared among the carotenoid biosynthetic genes of Brevundimonas (Fig. 1). The individual ATCC 31461 carotenogenic gene products showed moderate identity to the corresponding proteins derived from Brevundimonas, ranging from 43% to 58%. Among the different carotenogenic genes, crtI appeared to be the most conserved gene. Compared with the organization of the carotenoid biosynthesis gene clusters isolated from other nostoxanthin-producing bacteria, this gene cluster organization was different. The crtY, crtI, and crtB were found to be in the same orientation, whereas the crtG gene preceded these three but was oriented in the opposite direction. The stop codon of the crtY gene is followed immediately by the start of crtI combined with a frameshift. Except these two genes, other carotenogenic genes are not closely physically linked.

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Figure 1. Comparison of the carotenoid biosynthetic genes for S. elodea ATCC 31461 and the Brevundimonas strains.

The GenBank accession numbers are as follows: JN224892 and JN224893, S. elodea ATCC 31461; AB181388, Brevundimonas sp.SD212 [15]; DQ309446, Brevundimonas vesicularis DC263 [17]. The genes are presented as arrows pointing in the direction of their transcriptions. The percentage values below each gene designate the percent amino acid identity between the S. elodea ATCC 31461 nostoxanthin biosynthetic enzymes and the corresponding gene from the Brevundimonas strains.

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Table 1. Homology analysis of the nostoxanthin biosynthetic genes in S. elodea ATCC 31461.

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Carotenoid identification of knockout mutants

HPLC analysis of the carotenoids isolated from the cells of ATCC 31461 showed several peaks at 475 nm. On the basis of previous studies as well as mass spectrometic analysis, peaks 1 through 4 were identified as nostoxanthin, caloxanthin, zeaxanthin and β-carotene, respectively (Fig. 2A). The other peaks might be impurities of the carotenoid extract.

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Figure 2. HPLC elution profiles of the pigments extracted from the wild-type and the knockout mutants.

Solid lines, the wild-type and the knockout mutants; dashed lines, the control assays. A, wild-type; B, ΔcrtZ; C, ΔcrtG; D, ΔcrtZG; E, ΔcrtY. The major pigments were identified as nostoxanthin (peak 1, λ_max: 274, 450, 476; [M+H]⁺: 601), caloxanthin (peak 2, λ_max: 276, 450, 476; [M+H]⁺: 585), zeaxanthin (peaks 3, 8 and 10, λ_max: 275, 450, 476; [M+H]⁺: 569), 2,2′-dihydroxy-β-carotene (peak 5, λ_max: 272, 450, 476; [M+H]⁺: 569), β-carotene (peaks 4, 6, 7, 9,11 and 12, λ_max:452, 476; [M+H]⁺: 537) and lycopene (peak 13 and 14, λ_max:296, 362, 446, 470, 502; [M+H]⁺: 537).

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Targeted deletions of the candidate carotenogenic genes in S. elodea ATCC 31461 were performed by double-crossover recombination. All knockout mutants were analyzed for carotenoid identification by LC-APCI-MS. Compared to the wild-type strain, ΔcrtZ did not produce 3-hydroxy carotenoids, and the pigments were separated into three major peaks. Peaks 5 and 6 were determined to be 2, 2′-dihydroxy-β-carotene and β-carotene respectively (Fig. 2B). These results demonstrated that an inactive crtZ gene inhibited 3,3′-hydroxylation of β-carotene synthesis. In mutant ΔcrtG, nostoxanthin and caloxanthin were not detected. The major pigment was identified as zeaxanthin (peak 8, Fig. 2C), and a small amount of its precursor β-carotene was present (peak 9, Fig. 2C). These data indicate that in this mutant the 2,2′-hydroxylation step was missing. The HPLC elution profile of the carotenoids accumulated by double knockout mutant ΔcrtZG showed a single major peak. This peak correspond to non-hydroxylated β-carotene (peak 11, Fig. 2D), indicating that CrtZ and CrtG were responsible for hydroxylation of the β-ionone rings to produce nostoxanthin. The crtY knockout mutant exhibited a light red pigmentation, distinct from the yellow one of the wild-type strain. This mutant, called ΔcrtY, accumulated lycopene that was absent from the wild-type strain (peak 13, Fig. 2E), suggesting that lycopene cyclization was impaired in this mutant. In addition, a knockout mutant of crtI accumulating phytoene instead of the final nostoxanthin has been described earlier [18]. Because phytoene is colorless, this mutant forms white colonies. Similarly, the colonies formed by the mutant ΔcrtB were also white, which serve as a visible marker for screening. HPLC analysis monitored at 475 or 284 nm showed that the crtB knockout mutant did not produce any carotenoids, indicating that knockout of crtB blocked carotenoid synthesis.

In order to determine whether the two ORFs (ORF2 and ORF6) were involved in carotenoid biosynthesis, we further deleted these two ORFs respectively. Knockout of ORF2 or ORF6 had no effect on the formation of nostoxanthin, indicating that these two ORFs were not related to carotenoid biosynthesis.

Functional complementation of CrtZ and CrtG in E. coli

In order to further determine the function of CrtZ, plasmid pACCAR16ΔcrtX-Z was constructed and then introduced in E. coli JM109. The transformant formed bright yellow colonies on LB agar plates containing requisite antibiotics. HPLC analysis of the carotenoids extracted from the transformant indicated that zeaxanthin was the predominant carotenoid (peak 1, Fig. 3A). A control culture, with the pACCAR16ΔcrtX plasmid, contained only β-carotene (peak 2, Fig. 3B). Therefore, we confirmed that this gene encoded the β-carotene hydroxylase converting β-carotene to zeaxanthin. To confirm the biological role of CrtG and to identify the molecular mechanism for β-carotene 2,2′-hydroxylation, we expressed the gene in zeaxanthin and β-carotene-accumulating E. coli cells and analyzed the carotenoid content by HPLC. The zeaxanthin and β-carotene-accumulating E. coli transformats to be used in this study was made by the introduction of plasmid pACCAR16ΔcrtX-Z or pACCAR16ΔcrtX in strain JM109. These two plasmids contain the p15A replication origin which is compatible with pUC18, making them amenable to replicate in conjunction with pUC18G within the same cell [21]. When plasmid pUC18G was introduced into the β-carotene-accumulating E. coli transformant, the new transformant accumulated 2,2′-dihydroxy-β-carotene (peak 3, Fig. 3C). In the transformant carrying pACCAR16ΔcrtX-Z and pUC18G, CrtG catalyzed the formation of nostoxanthin (peak 5, Fig. 3D). As the negative controls, E. coli cotransformed with pUC18 plus either pACCAR16ΔcrtX or pACCAR16ΔcrtX-Z was used, resulting in the accumulation of β-carotene or zeaxanthin (peak 7, Fig. 3E; peak 8, Fig. 3F). These results show that crtG encoding 2,2′-dihydroxy-β-carotene hydroxylase, was capable of hydroxylating β-carotene and zeaxanthin.

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Figure 3. HPLC elution profiles of the pigments extracted from the E. coli JM109 transformants.

A, pACCAR16ΔcrtX-Z; B, pACCAR16ΔcrtX; C, pACCAR16ΔcrtX and pUC18G; D, pACCAR16ΔcrtX-Z and pUC18G; E, pACCAR16ΔcrtX and pUC18; F, pACCAR16ΔcrtX-Z and pUC18. The pigments were identified as β-carotene (peaks 2, 4 and 7), 2,2′-dihydroxy-β-carotene (peak 3), zeaxanthin (peak 1, 6 and 8) and nostoxanthin (peak 5).

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Discussion

Bacterial strains of the genus Sphingomonas are often isolated from contaminated environments [22], and most Sphingomonas species produce nostoxanthin [11]. The precise function of this unique carotenoid in these bacteria is unclear, likely it is associated with tolerance to environmental stress due to the antioxidant activity of carotenoids. In this study, the carotenogenic genes involved in the nostoxanthin biosynthetic pathway of S. elodea ATCC 31461 have been cloned and identified. Based on our results, we propose a biochemical pathway for synthesis of nostoxanthin in S. elodea ATCC 31461 (Fig. 4). The CrtG enzyme was first found in Brevundimonas species and the homologs of this hydroxylase was later found in cyanobacteria [12], [15]. The carotenoid biosynthetic genes in cyanobacteria are dispersed throughout the whole genome, while in typical bacteria, these genes are often clustered into large operons [23]. In the Brevundimonas carotenoid gene clusters, the crtG and crtZ genes were found to be adjacent to each other but oriented in the opposite direction [15], [17]. However, the crtZ gene of ATCC 31461 was not linked to crtG but located outside the carotenoid biosynthesis gene cluster. The genes crtI and crtB have been isolated from a variety of organisms. These two genes were often closely physically linked, whereas the crtI and crtB in the cluster of ATCC 31461 were separated by an unknown gene (ORF6). The relatively loose organization of these carotenogenic genes might have occurred through a rare event during evolution.

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Figure 4. The pathway of carotenoid biosynthesis in S. elodea ATCC 31461.

The gene products responsible for each enzymatic reaction are indicated.

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Various crtZ genes have been isolated from α-proteobacteria, γ-proteobacteria, eubacteria and cyanobacteria. A molecular phylogenetic tree was established based on the β-carotene hydroxylase sequences (Fig. 5). According to the phylogenetic tree, the β-carotene hydroxylases from the Sphingomonadaceae family constituted a group independent from the others, and ATCC 31461 CrtZ formed a distinct lineage within this group, indicating that ATCC 31461 CrtZ was in an independent phylogenetic position from the other genera.

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Figure 5. Neighbor-joining tree based on the β-carotene hydroxylase sequences.

Bootstrap values expressed as percentage of 1000 replications are shown next to each node (values below 50% are not shown). The GenBank accession numbers are given in parentheses.

https://doi.org/10.1371/journal.pone.0035099.g005

The crtG gene from Brevundimonas sp. SD212 has been reported to exhibit undetectable activity on β-carotene [15]. In contrast, ATCC 31461 CrtG could convert β-carotene into 2,2′-dihydroxy-β-carotene. This result was consistent with that of the CrtG from Brevundimonas aurantiaca [17]. Similar to CrtGs from Brevundimonas species, CrtG from S. elodea ATCC 31461 also exhibits intriguingly partial homology with the middle region of animal sterol-C5-desaturase involved in cholesterol biosynthesis. BLAST was used to search the GenBank database with the ATCC 31461 CrtG protein sequence as query. We found CrtG homologs, which have several annotations, depending on the source genome, as encoding sterol desaturases, fatty acid hydroxylases, or C-5 sterol desaturases. The ATCC 31461 CrtG shares a larger degree of sequence identity (76%–78%) with the homologs from the Sphingomonadaceae family, suggesting these homologs may play the similar role in carotenoid-producing bacteria of this family.

S. elodea ATCC 31461 is used for biotechnological production of the commercial exopolysaccharide gellan gum. Gellan gum has a wide range of applications in food, pharmaceutical, and other industries due to its excellent rheological characteristics and unique structure [18], [24]. However, its costly downstream purification process limits its economic viability. To reduce process costs, several colorless mutants have been isolated by random mutagenesis and gene knockout [18], [25]. The knowledge about the biosynthesis of nostoxanthin in this bacterium can be used to obtain colorless mutants to further test for gellan production. Heterologous carotenoid production in E. coli or higher plants is a powerful method for the biosynthesis of natural carotenoids of interest [26]. In particular, the 2-hydroxy and 2,2′-dihydroxy carotenoids which are difficult to synthesis chemically have improved antioxidant activity [15]. The crtG gene identified here can be used for heterologous production of these novel carotenoids through combinatorial biosynthesis.

Materials and Methods

Bacterial strains and culture conditions

Table 2 gives the bacteria strains and plasmids used in this study. Except otherwise indicated, the wild-type and mutant strains of S. elodea ATCC 31461 were cultured in the yeast extract-peptone-glucose (YPG) medium (0.3% yeast extract, 0.5% peptone and 2% glucose, w/v) at 30°C for 72 h and stored at 4°C. E. coli S17-1 and E. coli DH5α were the hosts for genetic manipulation whereas E. coli JM109 was used either for production of carotenoids or complementation experiments. E. coli strains were cultured aerobically in Luria-Bertani (LB) medium at 37°C or 30°C. The solid medium contained agar (15 g/L). For carotenoid production by Sphingomonas strains, inoculum was developed by transferring one loop full of the organism from slant culture to the YPG medium in 500 mL Erlenmeyer flasks. The flasks were incubated on a rotary shaker at 200 rpm and 30°C for 24 h for inoculum development. Then 10 mL broth was used as inoculum for 100 mL of yeast extract-glucose (YG) medium (0.05% yeast extract, 1% glucose, 0.015% K₂HPO₄, 0.01% NaHPO₄, 0.01% MgSO₄·7H₂O, w/v) in 500 mL Erlenmeyer flasks and incubated on a rotary shaker at 200 rpm and 30°C for 48 h. E. coli strains for pigment analysis were grown in LB medium at 37°C over night, of which 6 mL was used to inoculate 100 mL LB medium in 500 mL Erlenmeyer flasks and incubated at 30°C for 2 days. Isopropyl-β-D-thiogalactopyranoside (IPTG) was used at 1 mM for induction of the culture as required. When necessary, antibiotics were used at the following concentrations (µg/mL): streptomycin (25), kanamycin (50), ampicillin (15 for Sphingomonas and 100 for E. coli), chloramphenicol (25), and tetracycline (5 for Sphingomonas and 25 for E. coli).

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Table 2. Bacterial strains and plasmids used in this study.

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Recombinant DNA techniques

Plasmid preparations, PCR reactions, transformations and other standard molecular biology techniques were carried out as described elsewhere [27] or as instructed by suppliers. The restriction enzymes, DNA polymerase and DNA ligation kit were purchased from Takara (Dalian, China).

Cloning of the carotenoid biosynthesis genes

The phytoene desaturase gene of S. elodea ATCC 31461 was previously cloned and identified [18]. To clone other carotenoid biosynthesis genes from this organism, the sequences obtained previously were extended using the SiteFinding-PCR method [19]. From SiteFinding-PCR, a carotenoid biosynthesis gene cluster was obtained by merging the sequences of different DNA fragments. The CODEHOP (Consensus-degenerate hybrid oligonucleotide primers) strategy (http://blocks.fhcrc.org/blocks/codehop.html) was used to generate PCR primers for partial crtZ fragment amplification [28]. Primer design was based on a created set of blocks that represented highly conserved regions of homologous proteins. Specific blocks were made using the Block Maker program (http://blocks.fhcrc.org/blocks/make_blocks.html) by submitting eight bacterial β-carotene hydroxylase sequences: ABO10434 from Erythrobacter gaetbuli, ABC62608 from Erythrobacter litoralis HTCC 2594, EAQ28084 from Erythrobacter sp. NAP1, BAD 99406 from Brevundimonas sp. SD 212, ABO10432 from Brevundimonas bacteroides, ABC50108 from Brevundimonas vesicularis, EAS50417 from Aurantimonas manganoxydans SI85-9A1, and ABS69756 from Xanthobacter autotrophicus Py2. Several sets of primers were designed by the CODEHOP program, using the default parameters of the CODEHOP server. Primers crtZsense and crtZantisense were selected to amplify the expected sequences. The 3′-terminal and 5′-terminal sequences of crtZ were also acquired by SiteFinding-PCR method. Specific primers used for SiteFinding-PCR were designed according to the 3′-end and 5′-end sequences. The primers used for cloning of the biosynthesis genes are shown in Table S1. All PCR fragments were cloned using the pMD19-T vector for sequencing. To reveal any mispairing and sequencing error, the genes were cloned from genomic DNA by PCR with Pyrobest DNA polymerase, an enzyme with high fidelity (Takara, Dalian, China). These PCR fragments were subsequently cloned and characterized by DNA sequencing.

Comparative sequence analysis and phylogenetic tree construction

Database searches were run with the BLAST server at the National Center for Biotechnology Information (http://www.ncbi.nlm.nih.gov/BLAST). Multiple sequence alignments were performed with the ClustalW program at the European Molecular Biology Laboratory (http://www.ebi.ac.uk/clustalw). Subsequent adjustments of these alignments were done manually. A phylogenetic tree was constructed by the neighbor-joining (NJ) method using MEGA version 4.0 from ClustalW alignment. Bootstrap support was estimated using 1000 replicates for distance analysis.

Construction of knockout mutants

The candidate carotenoid biosynthetic genes and ORFs were inactivated by double-crossover homologous recombination. The upstream and downstream flanking sequences of genes selected for knockout were amplified by PCR using genomic DNA templates isolated from wild-type S. elodea ATCC 31461 with the primers described in Table S2. The primers used to amplify the flank fragments of the target genes contained SacI, XbaI, or PstI restriction sites. PCR products of respective gene were digested with the appropriate restriction enzymes, ligated to a suicide vector pLO3 [29], and used to transform E. coli S17-1.

Transfer of the respective recombinant plasmids (pLO3B, pLO3Y, plO3Z, and pLO3G) to S. elodea was performed by triparental filter mating using E. coli HB101/pRK2013 as the help strain [30], [31]. E. coli S17-1 containing the recombinant plasmid was used as a conjugal donor, whereas pRK2013 can mobilize and promote conjugal transfer. The protocol for triparental filter mating was performed as described elsewhere [32]. Transconjugants were selected on YM plates containing tetracycline at 5 µg/mL and subsequent YPG plates containing 8% sucrose. The knockout mutants were isolated by selecting for lost of sucrose toxicity encoded by the sacB gene of pLO3 [33] and antibiotic susceptibility, followed by PCR screening using the verification primers for those with the correct excision and DNA sequencing.

Construction of plasmids for expression of crtZ and crtG in E. coli

The candidate β-carotene hydroxylase (CrtZ) and 2,2′-β-hydroxylase (CrtG) enzymes were assayed by expressing the genes in E. coli JM109 engineered to accumulate different carotenoid substrates. Plasmid for expression of crtZ (pACCAR16ΔcrtX-Z) was constructed as follows. The candidate crtZ gene was amplified by PCR with the primers AvaI-crtZ-sense and HindIII-crtZ-anti, which were designed to contain AvaI and HindIII restriction sites, respectively. The Pantoea ananatis crtE gene was amplified from plasmid pACCAR16ΔcrtX by PCR with the primers HindIII-crtE-sense and SalI-crtE-anti, which were designed to contain HindIII and SalI restriction sites, respectively. The plasmid pACCAR16ΔcrtX carrying the carotenoid biosynthetic genes responsible for synthesis of β-carotene (crtE, crtB, crtI, and crtY of pantoea ananatis) was kindly provided by Dr. Norihiko Misawa [34]. The above PCR products were digested with the appropriate restriction enzymes, and plasmid pACCAR16ΔcrtX was excised with AvaI and SalI. Then the two PCR fragments were ligated with the larger fragment of pACCAR16ΔcrtX carrying P. ananatis crtB, crtI, and crtY, to give plasmid pACCAR16ΔcrtX-Z.

For expression of candidate crtG in E. coli, plasmid pUC18G was constructed. Primers EcoRI-crtG-sense and BamHI-crtG-anti were used to amplify the candidate crtG gene with engineered EcoRI and BamHI restriction sites, and cloned into the EcoRI/BamHI site of pUC18 vector to create the expression vector pUC18G. The expressed CrtG protein was fused to a lead sequence of β-galactosidase under the control of the lac promoter by pUC18 [15]. Primers used for heterologous expression of crtZ and crtG in E. coli are listed in Table S3.

Isolation and identification of carotenoids

Cells grown as described above were harvested by centrifugation (6,000× g at 4°C for 15 min) and washed three times with sterilized water. The pigments were extracted from the cells with acetone/methanol (2∶1, v/v) under N₂ at 4°C and centrifuged to collect the supernatant. The extraction was repeated three times in dark to ensure all pigments were transferred to the liquid phase. Subsequently, the extracts were dried under vacuum and then saponified as described elsewhere [11]. After drying, the pigment was stored under N₂ at −80°C until further analysis. The saponified extracts were resuspended in 1 mL choloform/2-propanol (1∶1, v/v). Carotenoids were identified by HPLC using an Agilent 1200 high performance liquid chromatography (Agilent, USA) equipped with a diode-array detector and a Hypersil ODS-C18 column (4.6 mm×250 mm, 5 µm). Pigments were eluted with 85% methanol/5% 2-propanol/10% water for the first 20 min, then a linear gradient to 70% methanol/30% 2-propanol within 30 min, and maintained these final conditions for 10 min. The flow rate was 1 mL/min. HPLC-purified compounds were analyzed by LC-MS with an Agilent 1200 series LC/MSD Trap SL mass spectrometer system. The system control and data acquisition were performed using LC/MSD Trap Software 4.2 (Bruker). The MS parameters were set as follows: ion source, atmospheric pressure chemical ionisation (APCI); nebulisher, 60 psi; drying gas, nitrogen; drying gas temperature, 350°C; drying gas flow, 5.0 L/min; APCI temperature, 350°C; HV capillary, 3500 V; and scan range, 100 to 2200 m/z. Carotenoids were identified by retention time, features of absorption spectra and mass spectra in comparison to standard compounds or with reported data [11], [12], [15]–[17], [35], [36]. The standards of β-carotene, zeaxanthin and lycopene were obtained from CaroteNature (Lupsingen, Switzerland).

Supporting Information

Table S1.

DNA oligonucleotide primers used for cloning.

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Table S2.

Primers designs for gene knockout constructs. Nucleotides which are in bold show changes that were made in the sequence to engineer restriction sites for cloning. Restriction sites are underlined.

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(DOC)

Table S3.

Primers used for heterologous expression of crtZ and crtG in E. coli. Nucleotides which are in bold show changes that were made in the sequence to engineer restriction sites for cloning. Restriction sites are underlined.

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(DOC)

Acknowledgments

We thank Dr. Figurski for providing pRK2013, Dr. Lenz for providing pLO3, Dr. N. Misawa for providing pACCAR16ΔcrtX, and Xinhang Jiang of Zhejiang University for assisting in the HPLC analysis.

Author Contributions

Conceived and designed the experiments: LZ XW OL. Performed the experiments: LZ OL. Analyzed the data: LZ XW OL. Contributed reagents/materials/analysis tools: LZ OL CQ HG. Wrote the paper: LZ OL HG.

References

1. Britton G, Liaaen-Jensen S, Pfander H (2004) Carotenoids handbook. Basel: Birkhauser.
2. Frank HA, Cogdell RJ (1996) Carotenoids in photosynthesis. Photochem Photobiol 63: 257–264.
- View Article
- Google Scholar
3. Landrum JT, Bone RA (2001) Lutein, zeaxanthin, and the macular pigment. Arch Biochem Biophys 385: 28–40.
- View Article
- Google Scholar
4. Olson JA, Krinsky NI (1995) Introduction: The colorful, fascinating world of the carotenoids: important physiologic modulators. FASEB J 9: 1547–1550.
- View Article
- Google Scholar
5. Walter MH, Strack D (2011) Carotenoids and their cleavage products: Biosynthesis and functions. Nat Prod Rep 28: 663–692.
- View Article
- Google Scholar
6. Johnson E, Schroeder W (1996) Microbial carotenoids. Adv Biochem Eng Biotechnol 53: 119–178.
- View Article
- Google Scholar
7. Armstrong GA, Alberti M, Hearst JE (1990) Conserved enzymes mediate the early reactions of carotenoid biosynthesis in nonphotosynthetic and photosynthetic prokaryotes. Proc Natl Acad Sci U S A 87: 9975–9979.
- View Article
- Google Scholar
8. Misawa N, Nakagawa M, Kobayashi K, Yamano S, Izawa Y, et al. (1990) Elucidation of the Erwinia uredovora carotenoid biosynthetic pathway by functional analysis of gene products expressed in Escherichia coli. J Bacteriol 172: 6704–6712.
- View Article
- Google Scholar
9. Sandmann G (2001) Carotenoid biosynthesis and biotechnological application. Arch Biochem Biophys 385: 4–12.
- View Article
- Google Scholar
10. Kang K, Veeder G, Mirrasoul P, Kaneko T, Cottrell I (1982) Agar-like polysaccharide produced by a Pseudomonas species: production and basic properties. Appl Environ Microbiol 43: 1086–1091.
- View Article
- Google Scholar
11. Jenkins C, Andrewes A, McQuade T, Starr M (1979) The pigment of Pseudomonas paucimobilis is a carotenoid (nostoxanthin), rather than a brominated aryl-polyene (xanthomonadin). Curr Microbiol 3: 1–4.
- View Article
- Google Scholar
12. Iwai M, Maoka T, Ikeuchi M, Takaichi S (2008) 2, 2′-β-Hydroxylase (CrtG) is involved in carotenogenesis of both nostoxanthin and 2-hydroxymyxol 2′-fucoside in Thermosynechococcus elongatus strain BP-1. Plant Cell Physiol 49: 1678–1687.
- View Article
- Google Scholar
13. Gich F, Overmann J (2006) Sandarakinorhabdus limnophila gen. nov., sp. nov., a novel bacteriochlorophyll a-containing, obligately aerobic bacterium isolated from freshwater lakes. Int J Syst Evol Microbiol 56: 847–854.
- View Article
- Google Scholar
14. Hanada S, Kawase Y, Hiraishi A, Takaichi S, Matsuura K, et al. (1997) Porphyrobacter tepidarius sp. nov., a moderately thermophilic aerobic photosynthetic bacterium isolated from a hot spring. Int J Syst Evol Microbiol 47: 408–413.
- View Article
- Google Scholar
15. Nishida Y, Adachi K, Kasai H, Shizuri Y, Shindo K, et al. (2005) Elucidation of a carotenoid biosynthesis gene cluster encoding a novel enzyme, 2, 2′-β-Hydroxylase, from Brevundimonas sp. strain SD212 and combinatorial biosynthesis of new or rare xanthophylls. Appl Environ Microbiol 71: 4286–4296.
- View Article
- Google Scholar
16. Takaichi S, Shimada K, Ishidsu J (1990) Carotenoids from the aerobic photosynthetic bacterium, Erythrobacter longus: β-carotene and its hydroxyl derivatives. Arch Microbiol 153: 118–122.
- View Article
- Google Scholar
17. Tao L, Rouviere PE, Cheng Q (2006) A carotenoid synthesis gene cluster from a non-marine Brevundimonas that synthesizes hydroxylated astaxanthin. Gene 379: 101–108.
- View Article
- Google Scholar
18. Zhu L, Wu X, Li O, Chen Y, Qian C, et al. (2011) Cloning and knockout of phytoene desaturase gene in Sphingomonas elodea ATCC 31461 for economic recovery of gellan gum. J Ind Microbiol Biotechnol 38: 1507–1513.
- View Article
- Google Scholar
19. Tan G, Gao Y, Shi M, Zhang X, He S, et al. (2005) SiteFinding-PCR: a simple and efficient PCR method for chromosome walking. Nucleic Acids Res 33: e122.
- View Article
- Google Scholar
20. Videira P, Cortes L, Fialho A, Sa-Correia I (2000) Identification of the pgmG gene, encoding a bifunctional protein with phosphoglucomutase and phosphomannomutase activities, in the gellan gum-producing strain Sphingomonas paucimobilis ATCC 31461. Appl Environ Microbiol 66: 2252–2258.
- View Article
- Google Scholar
21. Misawa N, Satomi Y, Kondo K, Yokoyama A, Kajiwara S, et al. (1995) Structure and functional analysis of a marine bacterial carotenoid biosynthesis gene cluster and astaxanthin biosynthetic pathway proposed at the gene level. J Bacteriol 177: 6575–6584.
- View Article
- Google Scholar
22. Leys NMEJ, Ryngaert A, Bastiaens L, Verstraete W, Top EM, et al. (2004) Occurrence and phylogenetic diversity of Sphingomonas strains in soils contaminated with polycyclic aromatic hydrocarbons. Appl Environ Microbiol 70: 1944–1955.
- View Article
- Google Scholar
23. Liang C, Zhao F, Wei W, Wen Z, Qin S (2006) Carotenoid biosynthesis in cyanobacteria: structural and evolutionary scenarios based on comparative genomics. Int J Biol Sci 2: 197–207.
- View Article
- Google Scholar
24. Fialho AM, Moreira LM, Granja AT, Popescu AO, Hoffmann K, et al. (2008) Occurrence, production, and applications of gellan: Current state and perspectives. Appl Microbiol Biotechnol 79: 889–900.
- View Article
- Google Scholar
25. Wu X, Li O, Chen Y, Zhu L, Qian C, et al. (2011) A carotenoid-free mutant strain of Sphingomonas paucimobilis ATCC 31461 for the commercial production of gellan. Carbohydr Polym 84: 1201–1207.
- View Article
- Google Scholar
26. Osawa A, Harada H, Choi SK, Misawa N, Shindo K (2011) Production of caloxanthin 3′-β-D-glucoside, zeaxanthin 3, 3′-β-D-diglucoside, and nostoxanthin in a recombinant Escherichia coli expressing system harboring seven carotenoid biosynthesis genes, including crtX and crtG. Phytochem 72: 711–716.
- View Article
- Google Scholar
27. Sambrook J, Russell DW (2001) Molecular cloning: A laboratory manual. New York: Cold Spring Harbor Laboratory Press.
28. Rose TM, Schultz ER, Henikoff JG, Pietrokovski S, McCallum CM, et al. (1998) Consensus-degenerate hybrid oligonucleotide primers for amplification of distantly related sequences. Nucleic Acids Res 26: 1628–1635.
- View Article
- Google Scholar
29. Lenz O, Friedrich B (1998) A novel multicomponent regulatory system mediates H₂ sensing in Alcaligenes eutrophus. Proc Natl Acad Sci U S A 95: 12474–12479.
- View Article
- Google Scholar
30. Figurski DH, Helinski DR (1979) Replication of an origin-containing derivative of plasmid RK2 dependent on a plasmid function provided in trans. Proc Natl Acad Sci U S A 76: 1648–1652.
- View Article
- Google Scholar
31. Fialho AM, Monteiro GA, Sá-Correia I (1991) Conjugal transfer of recombinant plasmids into gellan gum-producing and non-producing variants of Pseudomonas elodea ATCC 31461. Lett Appl Microbiol 12: 85–87.
- View Article
- Google Scholar
32. Harding N, Patel Y, Coleman R (2006) Targeted gene deletions for polysaccharide slime formers. US Patent 0199201.
33. Gay P, Le Coq D, Steinmetz M, Berkelman T, Kado C (1985) Positive selection procedure for entrapment of insertion sequence elements in gram-negative bacteria. J Bacteriol 164: 918–921.
- View Article
- Google Scholar
34. Misawa N, Kajiwara S, Kondo K, Yokoyama A, Satomi Y, et al. (1995) Canthaxanthin biosynthesis by the conversion of methylene to keto groups in a hydrocarbon β-carotene by a single gene. Biochem Biophys Res Commun 209: 867–876.
- View Article
- Google Scholar
35. Takaichi S, Shimada K (1992) Characterization of carotenoids in photosynthetic bacteria. Methods Enzymol 213: 374–385.
- View Article
- Google Scholar
36. Takaichi S (2000) Characterization of carotenes in a combination of a C₁₈ HPLC column with isocratic elution and absorption spectra with a photodiode-array detector. Photosynth Res 65: 93–99.
- View Article
- Google Scholar
37. Simon R, Priefer U, Pühler A (1983) A broad host range mobilization system for in vivo genetic engineering: Transposon mutagenesis in Gram-negative bacteria. Nat Biotechnol 1: 784–791.
- View Article
- Google Scholar

[ref1] 1. Britton G, Liaaen-Jensen S, Pfander H (2004) Carotenoids handbook. Basel: Birkhauser.

[ref2] 2. Frank HA, Cogdell RJ (1996) Carotenoids in photosynthesis. Photochem Photobiol 63: 257–264.
View Article
Google Scholar

[3] View Article

[4] Google Scholar

[ref3] 3. Landrum JT, Bone RA (2001) Lutein, zeaxanthin, and the macular pigment. Arch Biochem Biophys 385: 28–40.
View Article
Google Scholar

[6] View Article

[7] Google Scholar

[ref4] 4. Olson JA, Krinsky NI (1995) Introduction: The colorful, fascinating world of the carotenoids: important physiologic modulators. FASEB J 9: 1547–1550.
View Article
Google Scholar

[9] View Article

[10] Google Scholar

[ref5] 5. Walter MH, Strack D (2011) Carotenoids and their cleavage products: Biosynthesis and functions. Nat Prod Rep 28: 663–692.
View Article
Google Scholar

[12] View Article

[13] Google Scholar

[ref6] 6. Johnson E, Schroeder W (1996) Microbial carotenoids. Adv Biochem Eng Biotechnol 53: 119–178.
View Article
Google Scholar

[15] View Article

[16] Google Scholar

[ref7] 7. Armstrong GA, Alberti M, Hearst JE (1990) Conserved enzymes mediate the early reactions of carotenoid biosynthesis in nonphotosynthetic and photosynthetic prokaryotes. Proc Natl Acad Sci U S A 87: 9975–9979.
View Article
Google Scholar

[18] View Article

[19] Google Scholar

[ref8] 8. Misawa N, Nakagawa M, Kobayashi K, Yamano S, Izawa Y, et al. (1990) Elucidation of the Erwinia uredovora carotenoid biosynthetic pathway by functional analysis of gene products expressed in Escherichia coli. J Bacteriol 172: 6704–6712.
View Article
Google Scholar

[21] View Article

[22] Google Scholar

[ref9] 9. Sandmann G (2001) Carotenoid biosynthesis and biotechnological application. Arch Biochem Biophys 385: 4–12.
View Article
Google Scholar

[24] View Article

[25] Google Scholar

[ref10] 10. Kang K, Veeder G, Mirrasoul P, Kaneko T, Cottrell I (1982) Agar-like polysaccharide produced by a Pseudomonas species: production and basic properties. Appl Environ Microbiol 43: 1086–1091.
View Article
Google Scholar

[27] View Article

[28] Google Scholar

[ref11] 11. Jenkins C, Andrewes A, McQuade T, Starr M (1979) The pigment of Pseudomonas paucimobilis is a carotenoid (nostoxanthin), rather than a brominated aryl-polyene (xanthomonadin). Curr Microbiol 3: 1–4.
View Article
Google Scholar

[30] View Article

[31] Google Scholar

[ref12] 12. Iwai M, Maoka T, Ikeuchi M, Takaichi S (2008) 2, 2′-β-Hydroxylase (CrtG) is involved in carotenogenesis of both nostoxanthin and 2-hydroxymyxol 2′-fucoside in Thermosynechococcus elongatus strain BP-1. Plant Cell Physiol 49: 1678–1687.
View Article
Google Scholar

[33] View Article

[34] Google Scholar

[ref13] 13. Gich F, Overmann J (2006) Sandarakinorhabdus limnophila gen. nov., sp. nov., a novel bacteriochlorophyll a-containing, obligately aerobic bacterium isolated from freshwater lakes. Int J Syst Evol Microbiol 56: 847–854.
View Article
Google Scholar

[36] View Article

[37] Google Scholar

[ref14] 14. Hanada S, Kawase Y, Hiraishi A, Takaichi S, Matsuura K, et al. (1997) Porphyrobacter tepidarius sp. nov., a moderately thermophilic aerobic photosynthetic bacterium isolated from a hot spring. Int J Syst Evol Microbiol 47: 408–413.
View Article
Google Scholar

[39] View Article

[40] Google Scholar

[ref15] 15. Nishida Y, Adachi K, Kasai H, Shizuri Y, Shindo K, et al. (2005) Elucidation of a carotenoid biosynthesis gene cluster encoding a novel enzyme, 2, 2′-β-Hydroxylase, from Brevundimonas sp. strain SD212 and combinatorial biosynthesis of new or rare xanthophylls. Appl Environ Microbiol 71: 4286–4296.
View Article
Google Scholar

[42] View Article

[43] Google Scholar

[ref16] 16. Takaichi S, Shimada K, Ishidsu J (1990) Carotenoids from the aerobic photosynthetic bacterium, Erythrobacter longus: β-carotene and its hydroxyl derivatives. Arch Microbiol 153: 118–122.
View Article
Google Scholar

[45] View Article

[46] Google Scholar

[ref17] 17. Tao L, Rouviere PE, Cheng Q (2006) A carotenoid synthesis gene cluster from a non-marine Brevundimonas that synthesizes hydroxylated astaxanthin. Gene 379: 101–108.
View Article
Google Scholar

[48] View Article

[49] Google Scholar

[ref18] 18. Zhu L, Wu X, Li O, Chen Y, Qian C, et al. (2011) Cloning and knockout of phytoene desaturase gene in Sphingomonas elodea ATCC 31461 for economic recovery of gellan gum. J Ind Microbiol Biotechnol 38: 1507–1513.
View Article
Google Scholar

[51] View Article

[52] Google Scholar

[ref19] 19. Tan G, Gao Y, Shi M, Zhang X, He S, et al. (2005) SiteFinding-PCR: a simple and efficient PCR method for chromosome walking. Nucleic Acids Res 33: e122.
View Article
Google Scholar

[54] View Article

[55] Google Scholar

[ref20] 20. Videira P, Cortes L, Fialho A, Sa-Correia I (2000) Identification of the pgmG gene, encoding a bifunctional protein with phosphoglucomutase and phosphomannomutase activities, in the gellan gum-producing strain Sphingomonas paucimobilis ATCC 31461. Appl Environ Microbiol 66: 2252–2258.
View Article
Google Scholar

[57] View Article

[58] Google Scholar

[ref21] 21. Misawa N, Satomi Y, Kondo K, Yokoyama A, Kajiwara S, et al. (1995) Structure and functional analysis of a marine bacterial carotenoid biosynthesis gene cluster and astaxanthin biosynthetic pathway proposed at the gene level. J Bacteriol 177: 6575–6584.
View Article
Google Scholar

[60] View Article

[61] Google Scholar

[ref22] 22. Leys NMEJ, Ryngaert A, Bastiaens L, Verstraete W, Top EM, et al. (2004) Occurrence and phylogenetic diversity of Sphingomonas strains in soils contaminated with polycyclic aromatic hydrocarbons. Appl Environ Microbiol 70: 1944–1955.
View Article
Google Scholar

[63] View Article

[64] Google Scholar

[ref23] 23. Liang C, Zhao F, Wei W, Wen Z, Qin S (2006) Carotenoid biosynthesis in cyanobacteria: structural and evolutionary scenarios based on comparative genomics. Int J Biol Sci 2: 197–207.
View Article
Google Scholar

[66] View Article

[67] Google Scholar

[ref24] 24. Fialho AM, Moreira LM, Granja AT, Popescu AO, Hoffmann K, et al. (2008) Occurrence, production, and applications of gellan: Current state and perspectives. Appl Microbiol Biotechnol 79: 889–900.
View Article
Google Scholar

[69] View Article

[70] Google Scholar

[ref25] 25. Wu X, Li O, Chen Y, Zhu L, Qian C, et al. (2011) A carotenoid-free mutant strain of Sphingomonas paucimobilis ATCC 31461 for the commercial production of gellan. Carbohydr Polym 84: 1201–1207.
View Article
Google Scholar

[72] View Article

[73] Google Scholar

[ref26] 26. Osawa A, Harada H, Choi SK, Misawa N, Shindo K (2011) Production of caloxanthin 3′-β-D-glucoside, zeaxanthin 3, 3′-β-D-diglucoside, and nostoxanthin in a recombinant Escherichia coli expressing system harboring seven carotenoid biosynthesis genes, including crtX and crtG. Phytochem 72: 711–716.
View Article
Google Scholar

[75] View Article

[76] Google Scholar

[ref27] 27. Sambrook J, Russell DW (2001) Molecular cloning: A laboratory manual. New York: Cold Spring Harbor Laboratory Press.

[ref28] 28. Rose TM, Schultz ER, Henikoff JG, Pietrokovski S, McCallum CM, et al. (1998) Consensus-degenerate hybrid oligonucleotide primers for amplification of distantly related sequences. Nucleic Acids Res 26: 1628–1635.
View Article
Google Scholar

[79] View Article

[80] Google Scholar

[ref29] 29. Lenz O, Friedrich B (1998) A novel multicomponent regulatory system mediates H₂ sensing in Alcaligenes eutrophus. Proc Natl Acad Sci U S A 95: 12474–12479.
View Article
Google Scholar

[82] View Article

[83] Google Scholar

[ref30] 30. Figurski DH, Helinski DR (1979) Replication of an origin-containing derivative of plasmid RK2 dependent on a plasmid function provided in trans. Proc Natl Acad Sci U S A 76: 1648–1652.
View Article
Google Scholar

[85] View Article

[86] Google Scholar

[ref31] 31. Fialho AM, Monteiro GA, Sá-Correia I (1991) Conjugal transfer of recombinant plasmids into gellan gum-producing and non-producing variants of Pseudomonas elodea ATCC 31461. Lett Appl Microbiol 12: 85–87.
View Article
Google Scholar

[88] View Article

[89] Google Scholar

[ref32] 32. Harding N, Patel Y, Coleman R (2006) Targeted gene deletions for polysaccharide slime formers. US Patent 0199201.

[ref33] 33. Gay P, Le Coq D, Steinmetz M, Berkelman T, Kado C (1985) Positive selection procedure for entrapment of insertion sequence elements in gram-negative bacteria. J Bacteriol 164: 918–921.
View Article
Google Scholar

[92] View Article

[93] Google Scholar

[ref34] 34. Misawa N, Kajiwara S, Kondo K, Yokoyama A, Satomi Y, et al. (1995) Canthaxanthin biosynthesis by the conversion of methylene to keto groups in a hydrocarbon β-carotene by a single gene. Biochem Biophys Res Commun 209: 867–876.
View Article
Google Scholar

[95] View Article

[96] Google Scholar

[ref35] 35. Takaichi S, Shimada K (1992) Characterization of carotenoids in photosynthetic bacteria. Methods Enzymol 213: 374–385.
View Article
Google Scholar

[98] View Article

[99] Google Scholar

[ref36] 36. Takaichi S (2000) Characterization of carotenes in a combination of a C₁₈ HPLC column with isocratic elution and absorption spectra with a photodiode-array detector. Photosynth Res 65: 93–99.
View Article
Google Scholar

[101] View Article

[102] Google Scholar

[ref37] 37. Simon R, Priefer U, Pühler A (1983) A broad host range mobilization system for in vivo genetic engineering: Transposon mutagenesis in Gram-negative bacteria. Nat Biotechnol 1: 784–791.
View Article
Google Scholar

[104] View Article

[105] Google Scholar

Figures

Abstract

Introduction

Results

Cloning of the nostoxanthin biosynthetic genes

Sequence analysis of the nostoxanthin biosynthetic genes

Carotenoid identification of knockout mutants

Functional complementation of CrtZ and CrtG in E. coli

Discussion

Materials and Methods

Bacterial strains and culture conditions

Recombinant DNA techniques

Cloning of the carotenoid biosynthesis genes

Comparative sequence analysis and phylogenetic tree construction

Construction of knockout mutants

Construction of plasmids for expression of crtZ and crtG in E. coli

Isolation and identification of carotenoids

Supporting Information

Table S1.

Table S2.

Table S3.

Acknowledgments

Author Contributions

References