2.1.1. RiAOX complete gene isolation.

R. irregularis single spores, collected from the in vivo inoculum INOQ69 provided by INOQ GmbH company (Solkau, Schnega, Germany) (http://inoq.de), were directly crashed in Whatman FTA paper (GE Healthcare, Little Chalfont, England) and immediately used for total DNA amplification using the REPLI-g Mini Kit (Qiagen, Hilden, Germany). A first approach to amplify the gene was based on the design of primers located at the 5’ and 3’ -UTRs in order to isolate the full-length sequence (based on the sequence available at NCBI, acc. no. GW102706). However, due to the inefficiency of that strategy, a new set of primers located within the ORF was designed for amplification of a fragment with a size of ca. 700 bp (RiFw_80: 5’-CATTTACTATCCACGCATCACGA-3’ and RiRev_651: 5’-TCCAACCACACGATGAGC-3’). PCR was conducted with Ready-To-Go PCR Beads (GE Healthcare, Little Chalfont, England) using 3 μl of the amplified DNA (previously diluted 1:20) as template and 0.2 μM of each forward and reverse specific primers. PCR was carried out for 35 cycles in a 2720 Thermocycler (Applied Biosystems, Foster City, CA, USA), consisting each cycle in 94°C for 30 s, 50°C for 30 s and 72°C for 1 min. An initial step of 94°C for 5 min and a final step of 72°C for 10 min were performed.

In order to isolate the 5’ and 3’ -UTRs, total RNA was extracted from 1 cm³ of an in vitro culture of R. irregularis strain INOQ69, which included spores and mycelium. Total RNA was extracted using the RNeasy ® Micro Kit (Qiagen, Hilden, Germany) following manufacturer’s protocol. RNA purity and concentration were assessed in a NanoDrop-2000C spectrophotometer (Thermo Scientific, Wilmington, DE, USA). Ten ng of total RNA were used as template for cDNA synthesis using the SMARTer^TM RACE cDNA Amplification Kit (Clontech, Mountain View, USA). For 5’and 3’ -UTRs isolation, a reverse and a forward specific primers were designed (GSP2: 5’- GAAACTGTTGCCGCAGTTCCTGGTATG-3’ and GSP1a: 5’- GCGTTCCCACCAGGTAGGTTGTGAAAT-3’, respectively) to be used in combination with a universal primer provided by the manufacturer. PCR was performed according to the protocol of the RACE cDNA Amplification Kit using the Advantage^® 2 PCR Kit (Clontech, Mountain View, USA).

For complete gene isolation, a forward and a reverse primer set were designed in the previously obtained 5’ and 3’ -UTRs regions (RiORF105Fw: 5’-AATGATTCGCTCGGTTTTTC-3’ and RiORF1137Rev: 5’-TTATTTACTCCATTTCCATTTTTC-3’). Total DNA of a single in vitro spore of R. irregularis strain INOQ69 was amplified as described above and 1 μl was directly used as template for PCR using 0.2 μM of each specific primer. The enzyme Phusion™ High-Fidelity DNA Polymerase (Thermo Fisher Scientific, Waltham, MA, USA) was used according to the manufacturer’s protocol. The amplification consisted in 35 cycles of 98°C for 10 s, 50°C for 20 s and 72°C for 1 min. An initial step of 98°C for 2 min and a final step at 72°C for 10 min were performed. The obtained amplicons were cloned onto a pGEM^® –T Easy vector (Promega, Madison, Wisconsin, USA) and used for transformation of E. coli JM109 (Promega, Madison, WI, USA) competent cells. Selected recombinant clones were send for commercial sequencing (Macrogen, Seoul, Korea: www.macrogen.com) using T7 and SP6 primers (Promega, Madison, WI, USA).

2.1.2. RiAOX sequence analysis.

CLC Genomics workbench 7.5.1 platform (CLCbio, Aarhus N, Denmark) was used to edit the isolated AOX sequences. Homology of obtained sequences was confirmed in NCBI GenBank database (National Center for Biotechnology Information, Bethesda, MD, http://www.ncbi.nlm.nih.gov/) using BLASTn and BLASTp algorithm [23].

The exon-intron structure and the location of the AOX (Ferritin-like super family) conserved domain was compared between R. irregularis and other fungal species using the Fancy Gene v1.4 software (freely available at http://bio.ieo.eu/fancygene/). The genomic AOX sequences of Rozella allomycis, Agaricus bisporus, Laccaria bicolor, Macrophomina phaseolina, Cryptococcus neoformans, Coccidioides posadasii, Neurospora crassa, Lichtheimia corymbifera, Candida albicans, Talaromyces stipitatus and Spraguea lophii were retrieved from EMBL-EBI (http://www.ebi.ac.uk/) or NCBI (http://www.ncbi.nlm.nih.gov/).

The prediction of the fungal AOX N-termini that can support mitochondrial targeting sequence was performed on the translated peptide sequence of R. irregularis AOX and on other fungal AOX sequences using MITOPROT software (http://ihg.gsf.de/ihg/mitoprot.html).

A phylogenetic analysis of AOX proteins from R. irregularis and from other fungi and plant species was performed. AOX protein sequences from plant Monocots, Eudicots and Gymnosperm species were retrieved from PLAZA (http://bioinformatics.psb.ugent.be/plaza/), UniProt (http://www.uniprot.org/), Ensembl Plants (http://plants.ensembl.org/index.html) and/or NCBI (see accessions on S1 List). Fungi AOX sequences were retrieved from EMBL-EBI, UniProt and/or NCBI (accessions on S1 List). Sequence alignments were performed on MAFFT (http://mafft.cbrc.jp/alignment/server/) under the default parameters and a selection of best-fit models of amino acid (aa) replacement was performed using ProtTest 2.4 (http://darwin.uvigo.es/software/prottest2_server.html). Using the selected best-fit model (LG+I+G) a Maximum Likelihood phylogenetic analysis was performed on MEGA V6.0 [24], with 150 bootstraps. Two bacterial AOX sequences were used as outgroup (Rhodanobacter sp. and Afipia felis).

To identify distinctive features of fungi and plant AOX proteins, multiple alignments were performed using the CLC software on the helices α2, α3, α5 and α6, which form the four-helix bundle accommodating the diiron center, on the helices α1 and α4, which form the hydrophobic region on the AOX molecular surface, and on region 3, previously defined as possibly important for plant AOX activity [25]. The regions involving the two conserved cysteine residues (CysI and CysII) which in plants are responsible for the α-keto acid regulation were also compared between plant and fungal sequences.

2.2.1. Experimental design and sample collection.

To study the involvement of AOX at transcriptional level on both AMF and host plant during mycorrhizal colonisation, an experimental trial was set up using tomato (Solanum lycopersicum L. cv. MoneyMaker), which is often selected as model plant for experiments with AMF, and R. irregularis (BEG 121 isolate) (former Glomus intraradices).

Tomato seeds were surfaced-sterilised in 4% sodium hypochlorite containing 0.02% (v/v) Tween 20, rinsed thoroughly with sterile water and germinated for 2 days in a plate on moistened filter paper at 25°C in darkness. Subsequently, tomato seedlings were grown hydroponically in 3 L plastic containers with Long Ashton nutrient solution and at constant aeration. The nutrient solution was replaced once a week. After 2 weeks, plantlets were individually transferred to 0.45 L pots with sterile sand:soil:vermiculite (3:1:1) mixture (soil had a pH of 7.2, 1.6% organic matter, 2.1 μg Kg^-1 of N, 1.7 μg Kg^-1 of P and 0.8 μg Kg^-1 of K as nutrient concentration).

Half of the plants (24 plants) were inoculated by adding 10% (v:v) of R. irregularis inoculum, which consisted in R. irregularis kept in a soil-sand mixture containing extradical mycelium and spores, and mycorrhizal root fragments of Trifolium repens L. and Sorghum vulgare. This AMF had been isolated from a Mediterranean agricultural soil. The same amount of soil:sand mix, but free of AMF, was added to control non- mycorrhizal plants. Non-mycorrhizal plants received an aliquot of AM inoculum filtrated (< 20 μm) (meaning without propagules) to homogenize the microbial populations. Plants were randomly distributed in a greenhouse and grown at 24/16°C with 16 h photoperiod and 70% humidity, watered three times a week with Long Ashton nutrient solution [26] containing 25% of the standard P concentration.

Plants were harvested at different time points: 1, 2, 4 and 6 weeks post inoculation. Three plants (biological replicates) were collected per time point for both inoculated and non-inoculated plants (control). Samples taken from the root system were immediately frozen in liquid nitrogen and stored at -80°C for further analysis. A sample of each individual root system was also taken for mycorrhizal quantification through microscopy observation.

2.2.2. Determination of mycorrhizal colonisation.

Root samples of R. irregularis inoculated tomato plants were stained with trypan blue [27] and examined using a Nikon Eclipse 50i microscope and bright-field conditions. Root colonisation by the AMF was determined as previously described [28], using the MYCOCALC software (http://www.dijon.inra.fr/mychintec/Mycocal-prg/download.html). The parameters measured were the mycorrhizal colonisation frequency (F %) and intensity (M %), arbuscule (A %) and vesicle (V %) abundance, and the relative colonisation intensity (m %). At least five slides, containing 30 root pieces of 1 cm length, were analysed per biological replicate. Five replicates were analysed at each time point.

2.2.3. RNA isolation and gene expression analysis by quantitative real time RT-PCR (qPCR).

Total RNA was extracted using Tri-Reagent (Sigma-Aldrich, MO, USA) according to manufacturer’s instructions. RNA was treated with RQ1 DNase (Promega, Wisconsin, USA), purified through a silica column using the NucleoSpin RNA Clean-up kit (Macherey-Nagel, PA, USA). Before storage at -80°C, RNA was quantified using a NanoDrop-2000C spectrophotometer (Thermo Scientific, Wilmington, DE, USA) and its integrity was checked by gel electrophoresis. First strand cDNA was synthesised with 1 μg of purified total RNA using the iScript cDNA Synthesis kit (Bio-Rad, CA, USA) according to the manufacturer’s instructions. Real time qPCR was performed using 1 μl of single stranded cDNA (diluted 1:10) and specific primers for the four tomato AOX genes (SlAOX1a, SlAOX1b, SlAOX1c and SlAOX2), and the AOX gene of R. irregularis. The tomato phosphate transporter SlPT4, usually used as molecular marker for arbuscular functionality with direct link with mycorrhiza development in the roots [29] was also evaluated (see primer details on S1 Table). Reactions were carried out in a iCycler iQ5 system (Bio-Rad) for 40 cycles, consisting each cycle in 94°C for 15 s, 55°C for 20 s and 72°C for 20 s. An initial step at 94°C for 2 min was considered. Three independent biological replicates were analysed per treatment. Three independent biological replicates were analysed per treatment and each sample was analysed in duplicate. The specificity of the different amplicons was checked by a melting curve analysis at the end of the amplification protocol.

Two genes for tomato (SlEF-1 and SlActin2) and two genes for R. irregularis (RiTEF1a and RiBTub1) were used as reference genes for further normalisation of the transcript data achieved on the target genes. Evaluation of expression stability for the reference genes was done using the statistical application geNorm [30]. Expression of target genes was evaluated by relative quantification using the geometric normalisation factors obtained from geNorm. Standard curves of a 4-fold dilution series from pooled cDNAs were used for PCR efficiency calculations [31].

Differences in the expression level of target genes between non-mycorrhizal and mycorrhizal roots were examined by a t-test, or when the data did not meet the normality and/or equal variance requirements with a Mann-Whitney Rank Sum test. Transcript levels between weeks post-inoculation were examined by a one-way analysis of variance (ANOVA) with Holm–Sidak post-hoc tests. When the data did not meet the normality and/or equal variance requirements, a Kruskal–Wallis one-way ANOVA on ranks with a Dunn’s test for post-hoc comparisons was performed instead. All expression data were analysed with the SigmaStat statistical package (Systat software, London, UK). Significance levels were set at P < 0.05.

2.3.1. Isolate selection and DNA extraction at single spore level.

Three single spores from three different R. irregularis isolates were used to investigate the RiAOX genomic sequence variability. The isolates used were BEG72 (provided by the Institute of Agrifood Research and Technology, IRTA, Spain), BEG144 (provided by Prof. Daniel Wipf, Agroécologie INRA-Université de Bourgogne, Dijon, France), and one isolate provided by INOQ GmbH, hereafter designated by INOQ isolate. Those AMF were, respectively, originally isolated in 1996 in Northeastern Spain [32], in 1979 in St. Petersburg, Russia (according to the International Bank for the Glomeromycota (http://www.i-beg.eu/)) and in 1996 in Breiningerberg/Aachen, Germany. All three inocula have been propagated on in vivo cultures ever since.

In vivo inoculum of BEG72 used in the experiment consisted in a mixture of mycorrhizal root fragments and spores on Terragreen® (Oil-Dri, UK) carrier substrate. The BEG144 and INOQ isolates used in this experiment consisted of in vitro AMF cultures (in carrot root organ cultures, ROC) established in 2013 from the original in vivo inoculum. Inoculum samples were observed under a binocular lens and spores were individually picked (three spores per isolate) with a pipette tip and placed in 0.2 ml tube containing 1 μl of sterile tap water. Spores were then crushed using a sterile pipette tip and the entire DNA content was amplified using the GenomiPhi V2 Whole-Genome Amplification Kit (GE Healthcare, Canada) according to manufacturers’ instructions. Synthesised DNA was stored at – 20°C until further use.

2.3.2. Molecular identification of R. irregularis.

To confirm the identity of all 9 individual spores as belonging to R. irregularis, the ribosomal rRNA sequences including the ITS-LSU-SSU regions [33], were amplified by PCR using the enzyme Phusion™ High-Fidelity DNA Polymerase (Thermo Fisher Scientific), cloned onto a pGEM^® –T Easy vector and send for commercially Sanger sequencing. Sequences from the rRNA gene of several R. irregularis and R. intraradices isolates together with rRNA sequences of Glomus clarum described in Stockinger et al. [34] and publically available in the NCBI database, were used to perform the clustering analysis with the sequences from the INOQ, BEG72 and BEG144 isolates. The region used for the analysis comprised ~1400 bp of the small subunit, ITS, and large subunit of the rRNA which is suitable to differentiate very closely related species such as R. irregularis and R. intraradices [35].

The multiple sequence alignment was performed using the CLUSTALW program in the software MEGA V6.0 [24]. Genetic distances were inferred by the Neighbour-Joining method [36] and the bootstrap consensus tree was inferred from 100 replicates.

2.3.3. High throughput sequencing of RiAOX in single spores.

In order to obtain enough amount of RiAOX amplicon in the 9 single spores regarding the high throughput sequencing using the Ion Torrent™ platform, it was necessary to follow a nested PCR approach.

Two sets of specific primers were used: Ri_F1: ATGATTCGCTCGGTTTTTC and Ri_R1: TTATTTACTCCATTTCCATTTTTC for first PCR, followed by a second PCR using the Ri_F2: CATAACACATTTCTTCGTAACACAAC and Ri_R2: CAGGAGCCTCATTAGTCAAACCG primers. The obtained amplicon had a size of 1209 bp. In both cases the reactions were conducted with the enzyme Phusion™ High-Fidelity DNA Polymerase (Thermo Fisher Scientific) for 35 cycles, consisting each cycle in 98°C for 10 s, 59°C/63°C (first/second PCR, respectively) for 20 s and 72°C for 1 min. An initial denaturation step at 98°C for 5 min and a final extension of 10 min at 72°C were also performed.

A minimum of 500 ng of PCR products were directly sent for sequencing using the Ion Torrent™ platform at STAB VIDA (http://www.stabvida.com/). The obtained FASTQ reads have been deposited in the Sequence Read Archive (SRA) from NCBI database.

Obtained reads were uploaded into the CLC Genomics workbench. The quality of sequencing reads was enhanced by trimming and discarding low quality sequences and only high quality FASTQ sequences were used for further analysis. Reads were mapped to a consensus reference sequence previously obtained from cloned Sanger sequences of RiAOX from the 3 isolates, using the following parameters: masking mode = no masking, mismatch cost = 2, insertion cost = 3, deletion cost = 3, length fraction = 0.5 and similarity fraction = 0.8, global alignment = no, non-specific match handling = map randomly, output mode = create read tracks, create report = yes, collect unmapped reads = no.

Once the reads were mapped to the reference, the mapped reads files were used as input to discover low frequency variants using quality score with the following parameters: ignore broken pairs = yes, minimum coverage = 10, minimum variant frequency (%) = 1, neighborhood radius = 5, minimum neighborhood quality = 15, minimum central quality = 20, remove pyro-error variants = yes, in homopolymer regions with minimum length = 3, with frequency below = 0.8, create track = yes, create annotated table = yes, create report = yes.

A comparison of all variants was then performed, being classified as Single Nucleotide Variation (SNV), Multiple Nucleotide Variation (MNV), Deletion (Del), Insertion (Ins) and Replacement (Repl). Comparison of all possible variants from the 9 spores was performed setting a frequency threshold (%) = 0. With this threshold it was possible to identify variants that are present in only one spore. On the contrary, to identify variants that are common to all 9 spores, a frequency threshold of 100% was set.

The frequency (defined as read count divided by read coverage) distribution of all variants, in relation to the total number of variants found for each spore was performed. The SNV frequency (read count divided by read coverage) along the gene sequence was performed for the three isolates.

The prediction of variants (SNVs and MNVs) that could putatively induce aa substitutions in the protein sequence was performed for each spore.

3.4.1. Molecular identification of R. irregularis spores.

The phylogenetic analysis of the cloned sequences placed all spores in the R. irregularis clade, together with sequences retrieved from databases and already recognised as belonging to R. irregularis (S4 Fig). The R. intraradices group was completely separated from R. irregularis.

3.4.2. High throughput sequencing of AOX in R. irregularis single spores.

A total of 385 379 high quality reads were obtained from the 9 individual spores, with a mean percentage of mapped reads to the reference sequence of 97%. The mean length of mapped read in the 9 spores was of 143 bp (see details on Table 1). The mean variant coverage was of 3 856 and the mean SNV coverage was of 3 482 (Table 1).

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Table 1. Reads and variants statistics of the 9 R. irregularis single spores.

https://doi.org/10.1371/journal.pone.0142339.t001

When considering all 9 spores, a total of 288 nucleotide variants (including SNVs, MNVs, insertions, deletions and replacements) were found within the 1209 bp sequence length (Fig 5A). Of these 288 variants, 93 corresponded to SNVs (Fig 5A). Many polymorphisms accumulated in the region corresponding to intron 2: 92 of which 38 were SNVs; however, a large number were also found dispersed throughout the sequence, including all exons (Fig 5A, S5 Fig). Only 13 polymorphisms, consisting mostly of insertions or deletions of 1 bp and one SNV were identical between spores.

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Fig 5. Distribution of variants along the 1209 bp AOX sequence of R. irregularis.

All the 288 variants (SNVs, MNVs, deletions, insertions and replacements) and only the SNVs present in the 9 spores are shown in A). The variants present in INOQ, BEG144 and BEG72 isolates plus the variants unique to each isolate are presented in B), C) and D), respectively.

https://doi.org/10.1371/journal.pone.0142339.g005

In the three spores of the INOQ isolate, a total of 123 variants were identified, of which 47 were unique to this isolate (16% of the 288 variants) (Fig 5B). Regarding the BEG144 isolate, a total of 167 variants were found and 80 were exclusive to this isolate (28% of the 288 variants) (Fig 5C). For BEG72, 141 polymorphisms were found and 54 (19% of the 288 variants) were unique to this isolate (Fig 5D). When comparing the three spores from the same isolate, the percentage of unique polymorphisms in each spore varied with isolate: 33% (13% corresponding to SNVs), 37% (17% for SNVs) and 26% (7% for SNVs) for INOQ, BEG144 and BEG72, respectively.

The frequency (read count divided by read coverage) distribution of all variants (in relation to the total number of variants in one spore) was plotted on histograms, ranging from rare (<2% of frequency of occurrence) until variants that showed a frequency of occurrence of almost 100% (Fig 6). All isolates presented highly frequent polymorphisms (>80–100% of frequency of occurrence), particularly SNVs (Fig 6). Nevertheless, most of variants showed until 20% of frequency of occurrence. The frequency of SNVs was relatively similar amongst isolates, ranging from low frequency SNVs until highly frequent SNVs, with several of them showing frequencies close to 100% (Fig 7A–7C).

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Fig 6. Variants frequency (deletions, insertions, SNVs, MNVs and replacements) distribution on single spores of INOQ, BEG144 and BEG72 isolates.

Variants can range from less than 2% until almost 100% of frequency of occurrence (relatively to the total number of variants in one spore).

https://doi.org/10.1371/journal.pone.0142339.g006

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Fig 7. Frequency of SNVs along the RiAOX sequence on the INOQ, BEG144 and BEG72 isolates.

https://doi.org/10.1371/journal.pone.0142339.g007

Variants (SNVs and MNVs) that could induce putative aa substitutions were compared amongst spores (Fig 8, S3 Table, S6 Fig). These SNVs and MNVs ranged from low until highly frequent (S3 Table). Most of other type of variants induced frameshift mutations and not aa changes. In INOQ 2, 7 SNVs and one MNV that could lead to aa changes were identified, being located in exons 1, 3 and 4. One SNV was located in the AOX ferritin-like domain on exon 3. Five SNVs were identified in INOQ 3 spore (one within the AOX ferritin-like domain), and 10 variants (8 SNVs and 2 MNVs) in the INOQ 5 (two SNVs within the AOX ferritin-like domain) (Fig 8). BEG144 isolate showed 24, 12 and 13 SNVs or MNVs in spores 2, 3 and 8, respectively. Of these, several were located in the same positions of exons 1, 3 and 4 (Fig 8) and 9 were within the AOX domain. BEG72_1 showed 8 variants that could induce aa changes, and two were located in exon 3, inside the AOX ferritin-like domain. BEG72_2 and BEG72_4 showed 10 and 7 variants, respectively, of which two (either SNV or MNV) were located in the same position as in BEG72_1, in the exon 3 (Fig 8).

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Fig 8. Location of the putative amino acid changes induced by SNVs or MNVs within the AOX ferritin-like domain, in the INOQ, BEG72 and BEG144 isolates.

Exons are indicated by different colours. The 52 bp of the predicted N-terminal are underlined. The AOX ferritin-like domain, obtained by nucleotide search on CDD database is italicised. The putative amino acid changes are bold and underlined. The location of the four universally conserved glutamate residues (E) and the two universally conserved histidine residues (H) are presented in bold and enlarged.

https://doi.org/10.1371/journal.pone.0142339.g008

4.1.1. Regulatory motifs in fungi AOX.

Multiple alignments of AOX sequences revealed that N-termini of fungal and plant proteins are highly divergent, particularly on helix α1 and on the region containing the plant conserved CysI (S1 Fig). In plants, CysI and CysII are involved in the mechanism of α-keto acid (particularly pyruvate) regulation [55,56]. The more N-terminal CysI acts as a site for intermolecular bond formation and α-keto acid activation [57], but CysII has a less well defined role in this activation. None of these cysteines were found in fungi, indicating a different mode of AOX regulation. Also animals lack the N-terminal cysteine, important for plant AOX regulation [11]. Crichton et al. [25] showed also that the E/DNV motif may be crucial during pyruvate activation in non-thermogenic plants. It was suggested that the presence or not of a conserved CysI residue and/or E/DNV motif, and a preferential stimulation by pyruvate or succinate may be related to the thermogenic (or not) phenotype of plants [58]. Interestingly however, our results showed that R. allomycis has the ENV motif, identical to most of the plant species, and RiAOX presents the ENS motif, identical to some eudicot AOX1d. Contrarily to plants, AOXs of fungi are generally monomeric and subjected to post-translational regulation by purine nucleoside 5’ monophosphates GMP and/or AMP, and its induction is much dependent on cytochrome pathway restriction and triggering by ROS [51]. Therefore, the reasons for this similarity with plants remain elusive, but it does not seem likely that it indicates any similarity in regulation with plants.

4.1.2. Phylogenetic analysis of R. irregularis AOX.

The results obtained in the present study showed a clear division between plant and fungal AOX protein sequences (Fig 3). In plants, AOX is encoded by a small gene family composed by a maximum of six gene members distributed in two subfamilies, the AOX1 and AOX2-subfamily (Cardoso et al. 2015). Our results are in accordance with the recent plant AOX classification scheme proposed by Costa et al. [37]. AOX sequences were completely separated between the two AOX subfamilies, the AOX2 (only described in eudicot plant species) and AOX1-subfamily, and amongst the AOX1 it created three main groups (AOX1a-c/1e, AOX1d monocots and AOX1d eudicots).

Concerning fungi AOX, our results clearly show the existence of two major clades: the Dikarya subkingdom, which includes Basidiomycota and Ascomycota phyla and a clade comprising all the other studied phyla (Fig 3). The fungal AOX phylogenetic tree therefore resembles the general phylogeny constructed for fungi [59], thus seeming that AOX phylogeny echoes fungi lineage-specific events.

4.1.3. Phylogeny of AOX in fungi.

The position of R. irregularis AOX and of its sister group formed by members of the Zygomycota (sub-phylum Mucoromycotina, order Mucorales) (Fig 3) reflects the phylogenetic relation described by Ebersberger et al. [59], Tisserant et al. [42] and Lin et al. [60], where the Glomeromycota and particularly R. irregularis are referred as close to Mucorales. Interestingly, Tisserant and colleagues [42] have compared the genome of R. irregularis with Mucoromycotina and Chytridiomycota genomes and found similar patterns of absence of several genes related to diverse metabolisms and detoxification/stress responses, suggesting that this loss is a common feature of the early diverging fungi. However, whereas for instance Lin and colleagues define Mucoromycotina as the closest fungi to R. irregularis, when regarding only AOX sequences R. irregularis seems more related to Chytridiomycota and Cryptomycota. R. irregularis is an obligate biotrophic symbiont and R. allomycis is an endobiotic biotrophic parasite; whether the relative proximity between AOX of R. irregularis and R. allomycis indicates some resemblance in lifestyle is unknown but can be hypothesised. In any case, R. irregularis AOX sequence seems to relate with that of ancient fungi, given the fact that R. allomycis has been placed on the putative primary branch of the fungi, basal to Chytridiomycota [61].

Although the division between the clade containing R. irregularis and the sister clade of Zygomycota was clear, their position relatively to Microsporidia was unresolved. Nevertheless, a relatively close AOX phylogenetic relationship between ancient fungi and microsporidians seems to be supported by findings of James et al. [62], who related R. allomycis with Microsporidia through shared signatures of parasitism and genomic features.