Correction to: Assessment of Polygala paniculata (Polygalaceae) characteristics for evolutionary studies of legume–rhizobia symbiosis

A correction to this paper has been published: https://doi.org/10.1007/s10265-021-01295-3


Introduction
Symbiotic relationships between plants and soil microbes (fungi and bacteria) are a fundamental topic in biology. Symbioses between plants and mycorrhizal fungi are common among plant taxa; about 70% of flowering plant families form symbiotic relationships with arbuscular mycorrhizal (AM) fungi (Bonfante and Genre 2010;Brundrett 2009;Zhu et al. 2006). On the other hand, root nodule (RN) symbiosis with the nitrogen-fixing bacteria, rhizobia and Frankia, has been observed only in four orders (Fabales, Fagales, Cucurbitales and Rosales) within the subclade Fabids, which has been called the nitrogen-fixing clade (Doyle 2011;Griesmann et al. 2018;Kistner and Parniske 2002;Soltis et al. 1999;van Velzen et al. 2018van Velzen et al. , 2019. It has been predicted that genetic predisposition to RN symbiosis was acquired once in a common ancestor of these orders (Doyle 2011;Soltis et al. 1999;Werner et al. 2014). Phylogenomic analyses conducted in recent studies have shown that RN symbiosis was lost several times independently in ancestral lineages; therefore, RN symbiosis has been retained only in a few scattered members of the nitrogen-fixing clade (Griesmann et al. 2018;van Velzen et al. 2018). Two symbiotic systems originated in different eras; based on fossil evidence (Remy et al. 1994;Stubblefield et al. 1987) and molecular clock estimates (Simon et al. 1993), AM symbiosis originated over 400 million years ago (MYA), while the hypothesised predisposition to RN symbiosis first occurred ca. 100 MYA (Doyle 2011;Soltis et al. 1999). RN symbiosis is believed to have evolved through the recruitment of early signalling components of AM symbiosis (Kistner and Parniske 2002). However, details of the evolutionary process involved are still under investigation.
The Fabales, an order of Fabids, comprises four families: Fabaceae, Polygalaceae, Quillajaceae and Surianaceae (The Angiosperm Phylogeny Group 2016; Bello et al. 2009). Fabaceae is a family of leguminous plants species, about 90% of which engage in RN symbiosis with rhizobia. The other three families of the Fabales do not engage in this symbiosis (de Faria et al. 1989). The molecular basis of both RN and AM symbioses has been revealed using two model Fabaceae plants, Lotus japonicus and Medicago truncatula (Kouchi et al. 2010;Madsen et al. 2010;Oldrody 2013;Parniske 2008;Sato et al. 2008;Young et al. 2011). Comparative studies in Fabales between model legumes and closely related non-leguminous species belonging to the same order are useful for elucidating the evolutionary process of RN symbiosis. Herbs might be the most appropriate plant life form for laboratory-based experiments. The life forms of Polygalaceae include trees, shrubs and herbs, while Quillajaceae and Surianaceae are found only as trees (Stevens 2001). Thus, Polygalaceae species may be the most appropriate non-leguminous Fabales plants for comparative genomics and molecular genetic analysis to understand the evolution of the RN symbiotic system.
Polygala paniculata L. (subgenus Polygala, section Timutua) is an herbaceous plant belonging to the tribe Polygaleae and natively distributing in South America (Paiva 1998). This species has expanded its distribution as an introduced species in pan-tropical regions and some subtropical areas of Asia, such as the island of Taiwan and the Okinawa Islands (Yang and Chen 2013). Because this species has shown antifungal and analgesic activities in mice, local people in Brazil and areas to which it has been introduced have utilised this species to treat injuries, dislocations, etc. (Andrew et al. 2012;Frescura et al. 2012;Johann et al. 2011;Nogueira et al. 2005). The plant can grow to 10-50 cm tall and produces numerous racemes with over 100 flowers per inflorescence (Coelho et al. 2008). The flower is self-fertile and has a white, legume-like petal structure with two ovules per flower; one or two mature seeds can be obtained per fruit. The chromosome number of this species is reported as 2n = 52 or 56 (Favarger and Huynh 1965;Huynh 1965).
A previous study mentioned the contents of only one germination medium for in vitro propagation (Nogueira et al. 2005) and there are no descriptions of the characteristics of P. paniculata as an experimental plant.
In the present paper, we characterised P. paniculata, a non-leguminous plant closely related to legumes, to assess its potential as a model plant for study of the evolution of plant-microbe interactions. To investigate the characteristics of this species as a model plant, we conducted molecular phylogenetic analysis and examined responses to AM fungal and rhizobial infections. We found that the estimated genome size of P. paniculata was similar to that of L. japonicus and M. truncatula. Additionally, a hairy root transformation method using Agrobacterium rhizogenes was established in P. paniculata. We introduce P. paniculata as a suitable experimental plant for reconstruction biology for the study of RN symbiosis.

Plant materials
Seeds of P. paniculata used in this study were originally derived from the Republic of Palau (permission no. ROP-018-2014). Seeds were planted on vermiculite and cultured at 24 °C under a 16 h light and 8 h dark (16L: 8D) cycle in a growth chamber (Biotron, LPH-350S, NK system, Osaka, Japan). We harvested seeds from plants collected in Palau and used them for the following analyses.

Phylogenetic analysis using chloroplast rbcL sequences
The genomic DNA of P. paniculata was extracted from the leaves of three individuals separately using a total protein solubilisation buffer [10 mM EDTA, 100 mM Tris-HCl buffer (pH 8.0), 1 M KCl] and chloroform (Wako, Japan) and resolved with Tris-EDTA (TE) buffer after ethanol precipitation. Primers used for both cloning and sequencing of the P. paniculata rbcL gene were designed with reference to the NCBI database and published papers on Polygala spp. (Bello et al. 2009;Fay et al. 1998;Forest et al. 2007;Käss and Wink 1996;Sulaiman et al. 2003). Then, P. paniculata rbcL DNA fragments were amplified with PrimeSTAR GXL DNA Polymerase (Takara, Japan) and the following primer set: 5′-ATG TCA CCA CAA ACA GAA ACT AAA GC-3′ and 5′-TAT CCA TTG CTT CGA AGA CAA ATT TG-3′ (Käss and Wink 1996). The DNA region amplified with these primers (1365 bp) included all the sequences of the rbcL gene for DNA barcoding (552 bp; CBOL Plant Working Group 2009). PCR was performed using an Applied Biosystems Veriti Thermal Cycler (Thermo Fisher Scientific, MA) with the following programme: 3 min at 98 °C, 30 cycles of 10 s at 98 °C, annealing at 55 °C for 15 s, 1 min at 68 °C a final extension of 7 min at 68 °C. After A-tailing with Ex-Taq DNA polymerase (Takara), PCR products were cloned into pGEM T-easy vector (Promega, Japan) and then insert DNA sequences were determined using Applied Biosystems 3130xl Genetic Analyzers (Thermo Fisher Scientific) with two sequencing primers specific to rbcL genes as follows: 5′-GCG TTG GAG AGA CCG TTT CT-3′ (Fay et al. 1998) and 5′-TCG CAT GTG CCC GCA GTA GC-3′ (Sulaiman et al. 2003).
Phylogenetic analysis of P. paniculata and other species belonging to Polygalaceae and Fabaceae was conducted. The nucleotide sequence data were searched using the keywords 'Polygalaceae' and 'rbcL' in the GENBANK database (accessed 30 March, 2017: NCBI Resource Coordinators 2016). Our search identified 408 sequences, from which we removed non-rbcL sequences and those that were too short for comparison. In total, 175 sequences, including those of our samples, were used for analyses (Table S1). DNA sequences were translated into amino acid sequences and multiple sequence alignment was conducted using the MAFFT programme (Katoh et al. 2019). Aligned sequences were then converted to nucleotide sequences again using PAL2NAL (Suyama et al. 2006). Because six of the sequences were in fact three pairs of identical sequences, only 172 sequences were used for the following analysis (Table S1). A maximum likelihood (ML) tree was constructed using RAxML version 8.2.6 with the GTRGAMMA model based on nucleotide sequences (Stamatakis 2014). Support values were calculated with 1000 bootstrap samples.

Sterile culture conditions
Seeds were washed with 100% ethanol for a second and sterilised with 2-10% (w/w) hypochlorite solution (Wako) containing 0.2% Tween-20 (Amersham Biosciences, Sweden) for 40 min. The sterilised seeds were washed with sterilised water and planted on Murashige and Skoog (MS) medium [MS salt (4.6 g l −1 ), 0.2% (w/v) gellan gum (Wako), 0.1% (v/v) Gamborg's vitamin solution (Sigma-Aldrich Co. LLC, MO), pH 5.8]. Sterilisation time, gellan gum concentration and sucrose concentration differed depending on the purpose of the experiment. Details of these differences are described in the result section separately. To determine the appropriate germination conditions, three replications were conducted for each treatment with ca. 30 seeds per plate. Plates were incubated at 24 °C under a 16L: 8D cycle.

AM fungal inoculation
To confirm the AM fungal infection of P. paniculata, inoculation experiments were conducted using Rhizophagus irregularis (DAOM197198; Premier Tech, Canada) as previously described . The inoculation pot consisted of three plastic parts: a lid, a soil container and a liquid medium reservoir. The soil was prepared by mixing vermiculite, gardening moulding and river sand in a ratio of 1:1:2 by volume, respectively and 100 ml one-tenth-strength Hoagland solution supplemented with 0.1 mM KNO 3 (pH 5.8) was added. Extra medium fell into the reservoir from a pore at the bottom of the soil container. A Kimwipe (Crecia, Japan) was hung from the pore into the reservoir to transfer extra medium solution into the soil. R. irregularis spores (4000) were mixed in the soil. Four P. paniculata seedlings were planted in each pot with two replications and cultured in a growth chamber (24 °C, 16L: 8D) for 4 weeks. Roots were stained with ink as previously reported  and fungal infection was observed under a stereomicroscope (SZX7, Olympus, Japan).

Rhizobial inoculation
Seedlings of P. paniculata were grown on modified Broughton and Dilworth (B&D) medium (Broughton and Dilworth 1971) plates containing 0.5% sucrose, 0.6% gellan gum and 0.5 mM KNO 3 . To facilitate root hair formation, the concentration of KH 2 PO 4 was reduced from 0.5 mM to 0.1 mM. Since B&D medium containing 0.6% gellan gum was hard to solidify, 0.5% plant agar was further added and the final concentration of MgSO 4 7H 2 O was adjusted to 1.5 mM. A bacterium with a broad host range, Mesorhizobium loti strain NZP2037 (Pankhurst et al. 1987), was used for the rhizobial infection experiment. Rhizobia were cultured in tryptone-yeast extract liquid medium at 28 °C for 2-3 d. The collected rhizobia were suspended in B&D medium at approximately 50-fold dilution, then spread on sucrose-free modified B&D plates. For the control of this experiment, B&D medium without rhizobia was spread on the plates. Seedlings with roots (1-3 cm in length) forming root hairs were transferred to these plates. Plates were stood and incubated at 24 °C under a 16L: 8D cycle. The area of the plates where roots elongated was shaded with black paper. Root hairs were observed 6-7 d after inoculation using a BX50 microscope (Olympus, Tokyo, Japan).

Genome size estimation
Flow cytometric analysis was performed to estimate the size of the P. paniculata genome using CyFlow SL (Sysmex Partec, Japan). Three different organs (leaf, flower and inflorescence stem) from two different individuals were chopped up using a razor in nuclei extraction buffer (Sysmex Partec) and filtered through a 50 μm CellTrics filter (Sysmex Partec). Staining solution containing staining buffer, propidium iodide and RNase (Sysmex Partec) was added to samples. Arabidopsis thaliana leaves were used as an internal standard. The number of nuclei was measured using 488 nm blue lasers. A regression formula of genome size and peak intensities was constructed using A. thaliana, which has a genome size of 125 Mbp. Then, genome size of each P. paniculata sample was estimated from the regression formula.

Hairy root transformation
Hairy root induction in P. paniculata seedlings was assessed using A. rhizogenes AR1193 transformed with a pCAMBIA1300GFP binary vector carrying the green fluorescent protein (GFP) gene driven by the cauliflower mosaic virus (CaMV) 35S promoter, which serves as a transformation marker for plant cells (Yano et al. 2017). Before transformation, P. paniculata seedlings were grown on MS medium (4.6 g l −1 MS salt, 0.2% gellan gum, 0.1% Gamborg's vitamin solution, 0.1-1% sucrose, pH 5.8) under dark conditions for 1-2 weeks. A. rhizogenes was streaked on LB medium with 20 μg ml −1 kanamycin, incubated at 28 °C for 3 d and suspended in distilled water. P. paniculata seedlings were cut in the middle of the hypocotyls in the suspension to remove roots. Seedlings were incubated on co-culture medium (4.6 g l −1 MS salt, 0.2 g l −1 sucrose, 0.9% agar, pH 5.8) for 5-6 d in darkness then transplanted to root elongation medium [4.6 g l −1 MS salt, 1.0 g l −1 sucrose, 0.9% agar, 1 ml l −1 Gamborg's vitamin solution, 12.5 mg l −1 meropen (Sumitomo Dainippon Pharm Co. Ltd., Japan), pH 5.8]. After 8 weeks of incubation, infections and hairy root generation were observed using a fluorescence stereomicroscope (SZX7, Olympus). Experiments were conducted three times under modified conditions, in the presence of 0.1 mM acetocyringone (AS) and/or 0.05 μM 1-naphthaleneacetic acid (NAA).

Statistical analysis
Differences in genome sizes among organs were tested by the Kruskal-Wallis rank sum test. To test the effects of different treatments on germination efficiency and seedling viability, generalised linear model based analyses were conducted for each treatment. The explanatory variables of each treatment and link functions were set as the log of the binomial distribution. Significant differences in explanatory variables were tested by ANOVA and Tukey multiple tests were conducted for the significant explanatory variables in post hoc analysis. These analyses were performed in R software version 3.3.2. (R Core Team 2016). For comparative analyses of the number of deformed root hairs, significant differences were tested by Welch's t test.

Phylogenetic analysis
We investigated the phylogenetic relationships between the plants used in this study and Polygalaceae and Fabaceae species. We analysed the morphology and rbcL sequences of 172 plants, including three P. paniculata sequences from different individuals, and confirmed whether our sample was P. paniculata (Figs. 1, S1). The Polygala sample in this study and three P. paniculata sequences were monophyletic. Thus, the plant sample in this study was morphologically and molecularly confirmed as P. paniculata.
In the phylogenetic tree, interspecies relationships among Polygalaceae and Fabaceae plants were resolved. The results strongly support an interfamilial relationship between Fabaceae and Polygalaceae. Inter-tribe relationships among four Polygalaceae tribes were also strongly supported with high confidence values (bootstrap score: 99-100), except for the relationship between the tribes Polygaleae and Moutabeae (bootstrap score: 22, Table S1, Fig. S1). The genus Polygala was not monophyletic within the tribe Polygaleae; other genera, such as Monnina, Securidaca and Comesperma nested in Polygala. These results are supported by previous studies on phylogenetic relationships in Polygalaceae (Bello et al. 2009(Bello et al. , 2012Forest et al. 2007).

Plant characteristics
Plant characteristics and growth conditions in culture rooms or incubators constitute basic information used to deal with certain plants in laboratories. It was possible to cultivate P. paniculata in a plastic pot under our laboratory conditions (Fig. 2a), and the plants reached a final height of ca. 50 cm (Table 1, Fig. 2b, Paiva 1998). An initial inflorescence was observed 8 weeks after germination (Fig. 2c, d). P. paniculata is self-fertile and one or two seeds are produced from each flower. It took about 3 months to harvest new seeds. Over 5000 seeds were obtained from a mature plant with numerous inflorescences. The seeds were small (1.5 mm length) and had arilloids and dense hairs (Fig. 2e, f) that often repelled water. Plants were able to grow under both long-day (16L: 8D) and short-day (8L: 16D) conditions. Although long-day conditions were more effective for initial growth, the length of internodes gradually shortened and the plants could not produce mature seeds even after flowering. On the other hand, plants grown under 12L: 12D or 8L: 16D cycles continuously produced inflorescences. Therefore, for rapid growth and mass production of seeds, it would be better to culture plants under long-day conditions until initial inflorescence production, and then shift the light cycle to short-day conditions during seed harvesting periods.

Sterile culture conditions
Plant handling in vitro is a basic technique for transformation and experiments to assess plant interactions with microorganisms of interest. Although a previous study showed  Fig. S1. The accession number and organism name of each gene were indicated on the leaf of the tree. The lineage of the genus Polygala and the species P. paniculata were respectively emphasized by yellow and red background colours. The leaves indicated with a hand arrow were of the Polygala plant used in this study. The lineage including the genus Polygala also includes nine other genera (highlighted with different colours). The number provided at a node corresponds with the bootstrap support greater than or equal to 50% from the ML analysis. The scale bar represents 0.01 substitutions per site germination of P. paniculata on MS medium (Nogueira et al. 2005), the authors did not describe the detailed conditions for seed sterilisation and germination on the plate. We determined that the suitable condition for seeds sterilisation was 40 min incubation with a sterile solution of 2% sodium hypochlorite containing 0.2% Tween-20.
Next, we examined the concentrations of gellan gum and sucrose in the germination medium. Following the method detailed by Nogueira et al. (2005), we used MS medium supplemented with vitamins as the basic germination medium. Germinated seeds of P. paniculata sometimes displayed leaf yellowing or vitrification, and could not survive. Thus, we investigated not only germination rate but also their viability  Table 2). Although the germination efficiency did not differ among the four levels of gellan gum (P = 0.32, Table 2), viable seedling percentages increased with the amount of gellan gum (P < 0.01). The highest percentage of viable seedlings was observed on a 0.8% gellan gum plate [71.1 ± 6.1% (mean ± SE)]. However, the roots of the germinated seeds sometimes struggled to elongate into the medium, resulting in a growth delay. Leaves remained small and deposited anthocyanin as a stress response. Thus, the appropriate concentration of gellan gum was considered to be 0.6-0.8%.
Like gellan gum, sucrose did not influence germination efficiency (P = 0.91, Table 2), but did increase the proportion of viable seedlings (P < 0.01). The three different sucrose concentrations (0.2-1.0%) conferred different viabilities on seedlings. Thus, the concentrations of gellan gum and sucrose critically influence the survival rate of seedlings immediately after germination. These two factors are very important in improving viability.

Infection with AM fungi
RN symbiosis evolved through the recruitment of early signalling components essential for AM symbiosis. Therefore, both symbioses share common factors involved in the regulation of early responses to microsymbionts (Kistner and Parniske 2002). To confirm the ability of P. paniculata to form a symbiotic relationship with AM fungi, 6-weekold plants were inoculated with R. irregularis. The roots were observed 4 weeks after inoculation. Although fungal infection did not fully expand to the entire root (Fig. 3a), all P. paniculata samples we observed were successfully infected by AM fungi (N = 4). Hyphae and arbuscules were developed in the cortex of infected roots (Fig. 3b). Thus, P. paniculata was able to be a host in AM symbiosis.

Root hair responses to rhizobia
Although it is closely related to Fabaceae, P. paniculata is considered not to establish RN symbiosis with nitrogenfixing bacteria. However, it may have partially retained the genes necessary for the symbiosis. Therefore, we examined whether P. paniculata responded to rhizobia. Since leguminous plants and rhizobia often show host specificity at the species level, we used a rhizobial strain with a broad host range, M. loti NZP2037, for inoculation (Pankhurst et al. 1987). This strain possesses additional nod genes not found in narrow host range M. loti strains (Kasai-Maita et al. 2013; Kelly et al. 2014). Rhizobial inoculation is usually carried out under nitrogen starvation conditions to facilitate infection from root hairs and subsequent formation of RNs. When P. paniculata seeds were germinated on a nitrogen-deficient B&D agar medium, almost no root hairs were observed in the primary roots, at least in the early stages of seedling growth. To improve the productivity of root hairs, P. paniculata was grown on a B&D agar medium supplemented with 0.5% sucrose and a reduced amount of phosphorus. In this condition, ca. 80% of seedlings developed root hairs. Then, seedlings were transferred to a sucrose-free B&D agar medium and inoculated with rhizobia. There were no apparent differences in the growth and morphology of roots after inoculation with rhizobia when compared with non-inoculated roots. However, detailed observation revealed the occurrence of root hair deformation that was not seen in control plants (Fig. 4a, b).
The seedlings were inoculated with M. loti strain NZP2037 for 6-7 d to observe root hair responses. The tips of root hairs were occasionally observed to be swollen in both control and inoculated roots (Fig. 4c). There was no significant difference in the frequency of root hairs with tip swelling between control and inoculated roots (Fig. 4d). No clear root hair curling, which occurs to entrap rhizobia in leguminous roots, was observed in either control or inoculated roots (Fig. 4a, b). However, root hair branching was clearly observed only in roots inoculated with M. loti NZP2037 (Fig. 4b, e). The frequency of root hair branching in inoculated roots was significantly higher than that in control roots (Fig. 4f). This suggests that P. paniculata has the potential to recognise and respond to rhizobia.

Genome size estimation
Genome size is an important factor that affects the efficiency of genetic studies and genome surveys. We performed flow cytometry to estimate the genome size of P. paniculata using three different organs (leaf, flower and inflorescence stem).
Histograms of fluorescent intensities showed two peaks in leaf samples of P. paniculata: a large, sharp peak and a small, broad peak (Fig. 5a). The relative intensity of the small peak was approximately two-fold higher than that of the large peak, suggesting that the large peak represented nuclei with 2C and the small peak corresponded to 4C nuclei. Arabidopsis thaliana leaves had four peaks, with each peak representing each polyploidy (2, 4, 8 and 16C, Fig. 5b) and the regression formula had large R 2 values ranging from 0.9996 to 0.9999. In mixed samples of P. paniculata and A. thaliana leaves, a peak corresponding to the 2C of the P. paniculata was positioned between the 4C and 8C peaks of A. thaliana (Fig. 5c). We repeated the same experiment using flowers and inflorescence stems of P. paniculata. Both samples had a single large peak corresponding to 2C. The estimated values slightly differed among P. paniculata organs, ranging from 389.4 Mbp C −1 in the inflorescence stem to 423.1 Mbp C −1 in the flower (Table 3); however, these differences in estimated genome size were not statistically significant (χ 2 = 2.75, degree of freedom = 2, P = 0.25). The average genome size was 403.5 Mbp C −1 (N = 9, Table 3), which is comparable to those of L. japonicus and M. truncatula.

Hairy root transformation of P. paniculata
Hairy root transformation is an efficient method to investigate gene functions in the root system. Therefore, we assessed hairy root transformation in P. paniculata seedlings. According to procedures for the hairy root transformation of L. japonicus (Okamoto et al. 2013), roots were cut off from the middle parts of etiolated seedlings that were cultured in darkness and shoots were inoculated with A. rhizogenes carrying a plasmid with the GFP gene driven by the CaMV 35S promoter as a transformation marker for roots.
We initially co-cultured P. paniculata shoots with A. rhizogenes on MS medium without AS for 5 d and then transferred the shoots to hairy root-inducing plates without any phytohormones to sterilise the bacterium strain and to induce hairy roots. Only one inoculated shoot in 53 individuals (1.9%) produced a gall-like tissue expressing GFP on the hypocotyl and hairy root induction was not observed (Table 4). To improve the low transformation efficiency, the co-culture medium was supplemented with AS. Additionally, NAA was added either into the hairy root-inducing plates or into both the co-culture medium and the hairy root-inducing plate to facilitate hairy root induction. The simultaneous treatment with AS and NAA increased the transformation efficiency of seedlings to 30.6% and stimulated hairy root generation in 17.5% of plants (Table 4; Fig. 6a, b). Hairy roots were successfully generated from P. paniculata hypocotyls using these procedures.

Characteristics of P. paniculata
Our research results provide fundamental knowledge about P. paniculata characteristics and suggest the possibility of further study using this plant species.
Analyses of phylogeny used 172 sequences obtained from the NCBI database, and relationships among the species in the family Polygalaceae were resolved. Polygalaceae comprises four tribes and ca. 900 species (Christenhusz and Byng 2016). The Polygalaceae plant species have diverged and some genera (Bredemeyera, Muraltia, Nylandtia, Heterosamara, Salomonia, Acanthocladus, Monnina, Comesperma, Securidaca, Bredemeyera) were nested in the genus Polygala (Figs. 1, S1). Similar results of the relationships among the Polygala clade and other genera are described in previous articles (Bello et al. 2009(Bello et al. , 2012Forest et al. 2007), indicating that our results based on rbcL analysis are reliable. To understand the evolution of legume-rhizobia symbiosis, knowledge of evolution of the four families within the order of Fabales was thought to be important (Doyle 2011). The evolution of the families has been in the middle of discussion and many studies strenuously analysed phylogenetic relationships among the families in this order (e.g., Banks et al. 2008;Bello et al. 2009Bello et al. , 2012Forest et al. 2007;Qiu et al. 2010). These studies analysed several mitochondrial genes, such as matK, matR, rbcL, the trnL intron, trnL-F spacer, atp1, nad5 and rps3. One of the studies which analysed matK and rbcL with several phylogenetic methods Fig. 4 Root hair responses of P. paniculata to rhizobial inoculation. Broad views of root hairs in the control root (a) and the M. loti strain NZP2037-inoculated root (b). A typical image of swollen root hair tips (c) and the number of root hairs with swollen tips (d). A remarkable root hair branching observed in a M. loti NZP2037-inoculated root (e) and the number of branched root hairs (f). Statistical significance tests were performed using Welch's t test (N ≥ 10). An asterisk indicates significant difference (P < 0.05). N.S.: not significant. Scale bars; 100 µm proposed that the families Polygalaceae, Fabaceae, Quillajaceae and Surianaceae arose under the orders listed above and that the Polygalaceae lineage diverged from other lineages of Fabales plants ca. 84 MYA (Bello et al. 2009). Doyle (2011) also postulated that Polygalaceae seems to have diverged ca. 80 MYA from other Fabales plants and that Fabaceae and Surianaceae arose ca. 10 million years later. Future studies using the whole genome information of P. paniculata and comparative studies with other Fabales plants including model legumes may resolve the phylogenetic relationships of the four families in Fabales.
Species in the genus Polygala are often associated with a wide taxonomical range of AM fungi within Glomeraceae 1 (GlGrA). Some genera in Polygalaceae, such as Epirixanthes spp., include species that exhibit mycoheterotrophy with AM fungi (Mennes et al. 2015;Rath et al. 2013Rath et al. , 2014. Thus, the relationship between Polygala and mycorrhizal fungi has diversified. We confirmed that R. irregularis successfully infected P. paniculata roots. Molecular genetic analyses of model legumes and non-leguminous plants have identified factors and signalling pathways involved in the symbiosis (Choi et al. 2018;Handa et al. 2015;Takeda et al. 2013). Comparative studies on the functional and molecular mechanisms of AM symbiosis between model legumes and P. paniculata may reveal differences in symbiotic mechanisms between Fabaceae and Polygalaceae.
The genome size of P. paniculata was estimated at 403.5 Mbp C −1 , which is comparable with those of model plants in Fabaceae, L. japonicus (442 and 472 Mbp C −1 ) and M. truncatula (465 Mbp C −1 ) (Ito et al. 2000;Tang et al. 2014). Thus, the whole genome of P. paniculata could be analysed. Although the species diversity of the Polygala genus has been estimated (ca. 900 species), genome size has scarcely been determined (Castro et al. 2007;Coelho et al. 2008). According to a study on the genome sizes of two Polygala species by flow cytometry (Castro et al. 2007), one species P. calcarea belonging to subgenus Polygala, has relatively small genome size (481 Mbp C −1 in 34 chromosomes) and the other belonging to different subgenus, P. vayredae (subgenus Chamaebuxus), has relatively large size (1325 Mbp C −1 in 28 chromosomes). As well as the variety of genome sizes of plants of the genus Polygala, n-chromosome numbers also diverge greatly within the species of this genus (from 14 to 96 per 2n). Sharma and Mehra (1978) and Lack (1995) suggested that the burst of aneuploidy by hybridisation and expansion of their distribution cause the great inter-subgenus differences of n-chromosome numbers of Polygala spp. Lewis and Davis (1962) hypothesised that the basic number of chromosomes is 7, based on analysis of 52 Polygala spp. However, the critical data have not been shown until now. Analysing genome information of P. paniculata may clear inter-subgenus differences in genome size and chromosome number.

Sterile culture and molecular genetic experiments
The germination method for other Polygala species were previously described as follows: seeds are embedded in agar for approximately 2 months after a short sterilisation (< 10 min) to absorb water and transplanted to germination medium for several further weeks (Royal Botanic Gardens Kew 2017). However, our germination protocol with longer period of sterilization treatment of seeds with sodium hypochlorite shortened the period necessary for P. paniculata seed germination. We also determined the appropriate concentrations of gellan gum and sucrose for P. paniculata viability were 0.6% and 0.2-1.0%, respectively. P. paniculata seedlings reached sizes enough for the other experiments, such as inoculation tests and hairy root transformation, within 2 weeks of germination under these conditions. Furthermore, we examined the hairy root transformation in P. paniculata using A. rhizogenes. L. japonicus seedlings usually produce hairy roots in more than 50% of individuals under our experimental conditions (Okamoto et al. 2013). On the other hand, only one individual of P. paniculata seedlings (1.9% of all) produced gall-like tissues but did not induce any hairy roots on the same conditions (Table 4). Our analysis showed the importance of AS and NAA for the hairy root induction in P. paniculata seedlings. AS is one of the phenol-like products exuded from wounded plant organs. AS treatment often enhances the virulence of Agrobacterium spp., leading to the high transformation percentage in other plant species (Godwin et al. 1991;Kumar et al. 2006;Sheikholeslam and Weeks 1987). Requirement of AS for efficient Agrobacteriun infection varies according to plants (Godwin et al. 1991). Nicotiana tabacum shows that more than 20% of individuals are infected by A. rhizogenes without AS (Aoki and Syono 1999;Kumar et al. 2006). In the case of P. paniculata, we succeeded to increase frequencies of the infection and hairy root generation by simultaneous treatment of AS and NAA (Table 4); the infection rate and hairy root generation were 36.5% and 17.5% of P. paniculata seedlings. The successful induction of hairy roots would facilitate to analyse gene functions of interest and enable P. paniculata to be more useful as a model plant.

Root hair responses to rhizobial infection
Leguminous plants evolved root hair infection to introduce rhizobia into host cells. The root hair infection requires root hair curling in response to the Nod factor secreted from rhizobia. Rhizobia are thereby entrapped in curled root hairs, allowing them to form an infection chamber and an infection thread (Oldrody 2013). In symbiotic mutants at the early stages of nodulation, curling of the root hairs does not occur and the root hair deformation such as branching, tip swelling, waving, etc. is frequently observed in an infection-dependent manner. We predicted that root hair deformation would not occur even when the non-leguminous plant P. paniculata was infected with broad host range rhizobia, but unexpectedly, clear branching was observed at a relatively high frequency only in roots infected with M. loti NZP2037 (Fig. 4e,  f). This result indicates that P. paniculata has the potential to respond to rhizobia. In previous research, it has been shown that legume mutants deficient in the Nod factor signalling pathway such as castor, ccamk and nup85 exhibit root hair branching in an infection-or Nod factor treatment-dependent manner (Imaizumi-Anraku et al. 2005;Miwa et al. 2006;Saito et al. 2007). When we infected plants with the AM fungus R. irregularis in the present study, arbuscules were formed (Fig. 3a, b). Thus, we predict that genes of the common symbiosis signalling pathway are maintained in the P. paniculata genome. On the other hand, in M. truncatula, root hair branching is induced in the symbiotic mutants of Nod factor receptors such as LYK3 (Smit et al. 2007). Therefore, in P. paniculata, it is predicted that mutations occur in RN-specific symbiotic genes. In the future, deciphering the genome of P. paniculata will define missing symbiotic genes and mutations at the microsynteny level.
In this paper, we proposed P. paniculata as a candidate experimental plant for the study of the evolution of RN symbiosis. P. paniculata is a species closely related to model legumes and it would be easier to conduct comparative genomics at microsynteny levels. This non-leguminous species has a small genome and a relatively short lifecycle. We showed that it can be cultured under sterile conditions in the laboratory. Hairy root transformation enables gene function analyses in P. paniculata. It is expected that P. paniculata will lead to better understanding of the evolution of RN symbiosis.
Acknowledgements The seed samples were permitted to export by Palau Government with the certificate (No. ROP-018-2014). Authors thank Ms. Sachiko Tanaka (NIBB) for preliminary experiments and kind support on germination condition, seedling growth and seed harvesting. We thank Mr. Naoki Morooka and model plant research facility at NIBB for the analyses of genome size using CyFlow SL. This study was financially supported by Grant-in-Aid for Scientific Research on Innovative Areas (16H01248 to HF and 16H06279 to WI) of the Ministry of Education, Culture, Sports, Science and Technology, Japan (MEXT) and Grant-in-Aid for Scientific Research (C) (16K08149 to TS and 17K07509 to SA) of Japan Society for the Promotion of Science.
Open Access This article is licensed under a Creative Commons Attribution 4.0 International License, which permits use, sharing, adaptation, distribution and reproduction in any medium or format, as long as you give appropriate credit to the original author(s) and the source, provide a link to the Creative Commons licence, and indicate if changes were made. The images or other third party material in this article are included in the article's Creative Commons licence, unless indicated otherwise in a credit line to the material. If material is not included in the article's Creative Commons licence and your intended use is not permitted by statutory regulation or exceeds the permitted use, you will need to obtain permission directly from the copyright holder. To view a copy of this licence, visit http://creativecommons.org/licenses/by/4.0/. Fig. 6 Hairy root transformation from a P. paniculata hypocotyl. A bright field (a), and its fluorescent image (b) depicting hairy roots. Arrowheads indicate hairy roots expressing GFP. Scale bars; 2 mm