Increases in Genistein in Medicago sativa Confer Resistance against the Pisum Host Race of Acyrthosiphon pisum

Interspecific interaction with host plants have important consequences for the host race formation of herbivorous insects. Plant secondary metabolites, particularly those that are involved in host races specializing on plants, warrant the theory of host specialization. Acyrthosiphon pisum comprises various host races that adapt to different Fabaceae plants, which provides an ideal system for determining the behavioral and physiological mechanisms underlying host-adaptive diversification. The current study evaluated the effects of host transfer on population fitness, feeding behavior and the transcriptome-wide gene expression of the two host races of A. pisum, one of which was originally from Medicago sativa and the other from Pisum sativum. The results showed that the Pisum host race of A. pisum had a lower population abundance and feeding efficiency than the Medicago host race in terms of a longer penetration time and shorter duration times of phloem ingestion when fed on M. sativa. In contrast, few differences were found in the population abundance and feeding behavior of A. pisum between the two host races when fed on P. sativum. Meanwhile, of the nine candidate phenolic compounds, only genistein was significantly affected by aphid infestation; higher levels of genistein were detected in M. sativa after feeding by the Pisum host race, but these levels were reduced relative to uninfested controls after feeding by the Medicago host race, which suggested that genistein may be involved in the specialization of the aphid host race on M. sativa. Further exogenous application of genistein in artificial diets showed that the increase in genistein reduced the survival rate of the Pisum host race but had little effect on that of the Medicago host race. The transcriptomic profiles indicated that the transcripts of six genes with functions related to detoxification were up-regulated in the Pisum host race relative to the Medicago host race of A. pisum. These results suggested that the inducible plant phenolics and associated metabolic process in aphids resulted in their differential adaptations to their Fabaceae host.


Introduction
Host race is considered to be one of several intermediates in the continuum between polymorphisms and the full species [1]. Aphids (Hemiptera: Aphididae) are a group of phytophagous insects that exclusively consume the phloem sap from host plants. There are approximately 4700 species [2], some of which consist of diverging populations, host races, biotypes, or even potential forms of incipient speciation [3,4]. Acyrthosiphon pisum, a specialist aphid that feeds on legume plants, has at least 15 different host races [5]. Each is restricted to one or a few species of Fabaceae and is prone M. persicae. However, it is still unclear which detoxification-related genes are involved in the specificity adaptation of different aphid host races to host plants.
To determine why some host races of A. pisum could not perform well on non-specialized host plants, it is very important to measure the plant secondary metabolites levels to determine the level of plant defense. The different responses in plant secondary metabolites levels influenced by the two host races would favor the hypothesis that the low performance of A. pisum on non-specialized host plants is due to their susceptibility to phenolics. The present study aimed (1) to compare the feeding behavior and population abundance of the Medicago and Pisum host races of A. pisum on their specialized and non-specialized legume hosts; (2) to determine whether the levels of defensive phenolic contents, such as phenols and flavonoids, change in response to aphid feeding and have detrimental effects on the performance of the two host races; and (3) to quantify the transcriptome-wide gene expression of the two host races of A. pisum when fed on M. sativa and to further screen the candidate genes that are involved in the differential host adaptation between the two host races of A. pisum.

Aphids and Host Plants
Two host races of A. pisum were used in this study. The clone Pisum host race was collected from P. sativum in Yunnan Province, China. The clone Medicago host race was collected from M. sativa in Ningxia Province, China. The field-collected colonies (Medicago host race and Pisum host race) were individually established from a single parthenogenetic female. We verified that these two populations are specialized on different host plants by investigating the aphid population abundance and detecting the aphid feeding behavior using the electrical penetration graph (EPG) technique when fed on their own host plant and the alternative plant. The two field-collected colonies (Medicago host race and Pisum host race) were reared on their own host plant in the laboratory for more than five years. The two host races of A. pisum are well adapted to their own host plant. When we transferred the two host races of aphids to the alternative plant (Medicago host race to P. sativum and Pisum host race to M. sativa), we found that they cannot perform well on alternative host plants, especially for the Pisum host race on M. sativa. Two legume plant species, M. sativa and P. sativum, were grown in 12-cm diameter plastic pots with a standardized soil mixture (75 g/kg organic carbon; 500 mg /kg N; 200 mg/kg P; 300 mg /kg K) in climate chambers (Safe PRX-450C, Ningbo, China) at 22 ± 0.8 • C, 70% ± 5% relative humidity, and a 16 h light/8 h dark photoperiod. P. sativum was grown individually in order to get enough plant material for plant secondary metabolites analyses (approximately 4 leaf whorls), while M. sativa was grown three plants per pot (approximately 10 leaf whorls). P. sativum was used in experiments of aphid abundace 12 days after sowing, and M. sativa was used 25 days after sowing [15].

Aphid Population Abundance
To determine how the host plants affected the population abundance of specialized and non-specialized aphid clones, two legume host plants were randomly selected and infested with two apterous 4th instar nymphs. Each aphid-plant combination was replicated six times. The plants were covered with air permeable gauze, and the nymphs developed and produced offspring freely on each plant for 14 days. The aphid numbers were measured 7 and 14 days after infestation. The rearing conditions were the same as those described in Section 2.1.

Aphid Feeding Behavior
The electrical penetration graph (EPG) technique was employed to detect the feeding behaviors of the two host races of A. pisum on M. sativa. For each EPG recording, a wingless adult aphid was immobilized on ice, and then the aphid dorsum was attached to a gold wire (2 cm in length, 18.5 µm in diameter) using hand-mixed, water-based silver conducting paint glue (EPG Systems). The other side of the gold wire was then glued with a droplet of paint to a copper extension wire (2 cm in length), Insects 2019, 10, 97 4 of 14 which was inserted into the input of the EPG head stage amplifier. Another copper electrode (10 cm in length, 2 mm in diameter) was inserted into the soil of the plant container. Aphids were starved for 2 h as an adaptation period between the time of wiring and the beginning of the EPG recording. Aphids were then placed on the abaxial side of the leaf. The plants, aphids and amplifier were placed in a Faraday cage to avoid noise. For each aphid-plant combination, the 8 h EPG waveform recordings of 15 aphids were performed by a Giga-8 DC EPG System (EPG Systems, Wageningen, The Netherlands). The EPG waveforms were manually analyzed using the Stylet + analysis module as previously described: nonpenetration, stylets are outside the plants; pathway, mostly intramural probing activities between mesophyll or parenchyma cells; potential drops (pd), aphids briefly puncture cells during plant penetration; phloem salivation (E1), aphids are injecting watery saliva into the sieve element; phloem ingestion (E2), aphids are ingesting the phloem sap; xylem ingestion (G), aphids are ingesting the xylem sap [24].

Plant Material Sampling and Extraction of Phenolics
At the end of the aphid abundance experiment, the aphids were removed from the plants. Above-ground parts of three plant seedlings were harvested and dried. The plants without aphid infestation (called "uninfested") were used as a control. Each treatment had three replicates. For a typical extraction, approximately 50 mg samples were soaked with 1 mL 70% aqueous MeOH for 1 h in a 60 • C water bath. The extract was centrifuged at 12,000 rpm for 5 min, and the supernatant was filtered by a 0.22-µm filter. The samples were stored in a freezer at −20 • C until chemical analysis.

Quantification of Plant Secondary Metabolites by HPLC
The foliar phenolic compounds for chemical analysis were determined according to the previous method [25]. We quantified nine phenolic compounds in M. sativa by using HPLC: (1) phenolic acids, which includes protocatechuic acid, chlorogenic acid, caffeic acid, 4-hydroxycinnamic acid, syringic acid and ferulic acid; (2) flavonoids, which include rutoside; (3) isoflavones, which includes genistein and genistin. The determination of compounds was performed on a water system with a diode array detector. Chromatograms were registered and integrated at 280, 350, and 254 nm for phenolic acid, flavonoids, and isoflavone, respectively. The mobile phase consisted of 1% H 3 PO 4 -AcN (a linear gradient of 15-100% AcN) with a flow rate of 1 mL/min for 60 min. Compounds were identified by comparing the retention times to those of authentic standards.

Bioassay with Pure Compound
Artificial diets [26] were used to measure the effects of genistein on the survival of the two host races of A. pisum. All chemicals were purchased from Sigma-Aldrich (Missouri, MO, USA). Genistein was added into the diet at 0, 1 and 10 µg/mL concentrations. A diet without genistein, called "0", was used as a control. There were five biological replicates for each treatment. The solutions were enclosed in parafilm stretched across a tube (2 cm in height and 4 cm in diameter). During this experiment, the artificial diets were changed every two days. Twenty 2nd instar nymphs were exposed to a 100 µL diet containing genistein. For each group, the numbers of surviving aphids were counted after five days.

Transcriptomics Analyses
At the end of aphid abundance experiment, the two host races of A. pisum collected from M. sativa were used for transcriptomics analyses. Three replicates were employed.
For each replicate, Trizol (Life) was used to extract the total RNA of 10 adults according to the manufacturer's instructions. The total RNA was sent to the Beijing Genomics Institute (BGI) Company (Shenzhen, China) for an RNA-seq analysis. RNA was checked for purity and integrity using an Agilent 2100 Bioanalyzer. RNA-seq libraries were prepared following Illumina's protocols and were sequenced on the Illumina HiSeq 4000 sequencer (Illumina, Inc., San Diego, CA, USA) with a 150-bp paired-end reads. At least 10 million clean reads were obtained for each sample. These reads were mapped to the A. pisum genome using Hierarchical Indexing for Spliced Alignment of Transcripts (HISAT) version: v0.1.6-beta (Parameters: -phred64 -sensitive -no-discordant -no-mixed-I 1-X 1000) [27]. The genome sequence and gene annotation data sets were downloaded from AphidBase Official Gene Set v2.1 (http://www.aphidbase.com/). The gene expression levels were measured using RNA-Seq by Expectation-Maximization (RSEM) [28]. Differentially expressed genes were analyzed using the Noiseq package [29] with a fold change ≥ 2 and a divergence probability ≥ 0.8. Blast2GO software was used for gene ontology (GO) annotations [30]. The hypergeometric test was performed with whole transcriptome as the reference set and differentially expressed genes as the test set. GO terms with false discovery rate (FDR) corrected p values ≤ 0.01 were considered significantly enriched. Kyoto Encyclopedia of Genes and Genomes (KEGG) analyses were performed to identify significantly enriched pathways represented by differentially expressed genes. The hypergeometric test was performed in the same way to that for GO enrichment analysis. The terms were determined as enriched pathways according to FDR corrected p values ≤ 0.01 [31].

Quantification of Gene Expression
Trizol (Life) was used to isolate the total RNA from the two host races of A. pisum, and 1 µg RNA was used to synthesize the cDNAs, by using FastQuant RT Kit with gDNase (TianGen Biotech, Beijing, China). OligoDTs were used for the RT reaction. Real-time quantitative PCR (RT-qPCR) was used to quantify the expression levels of candidate genes of A. pisum. Reactions were performed in a PikoReal Real-time PCR Detection System (Thermo Scientific, Vantaa, Finland) using 10 µL reaction mixture which included 5 µL SuperReal PreMix Plus (TianGen Biotech, Beijing, China), 0.5 µL 10 uM forward, 0.5 µL 10 uM reverse primers, 2 µL 10-fold diluted cDNA template, and 2 µL ddH 2 O. The thermo protocol included preheating at 95 • C for 15 min, followed by 40 cycles of denaturation at 95 • C for 30 s, annealing at 60 • C for 30 s, and elongation at 72 • C for 40 s, and then a final cycle at 95 • C for 30 s, at 55 • C for 30 s and at 95 • C for 30 s. A standard curve was derived from serial dilutions to quantify the copy numbers of target mRNAs. The relative level of each target gene was standardized after comparing the copy numbers of target mRNA with copy numbers of the reference gene ribosomal protein L27 due to its stability of expression [32]. The specific primers for the genes were designed from A. pisum expressed sequence tags using PRIMER6 software (Table S1, Supporting information). There were three biological replicates for each host race. Each biological replicate contained four technical repeats. The fold-changes of the candidate genes were calculated by using the 2 −∆∆Ct normalization method.

Statistical Analysis
Statistical analyses were performed with SPSS 18.0. Student's t-tests were used to analyze the aphid abundance, aphid feeding behavior, and quantification of gene expression for two-group comparisons. A one-way ANOVA was used to analyze the amount of secondary plant metabolites of M. sativa and the survival of the two host races of A. pisum that were fed on the diet with genistein. The differences were considered to be statistically significant when p < 0.05. All of the data were checked for normality and equality of residual error variances and were appropriately transformed if needed to satisfy the assumptions of an analysis of variance.

Aphid Performance
There was little difference in aphid abundance between the two host races when fed on P. sativum. The Medicago host race of A. pisum exhibited a higher population abundance than the Pisum host race at one-week post-infestation (1.4-fold larger than the Pisum host race, p < 0.05) and two weeks post-infestation (1.3-fold larger than the Pisum host race, p < 0.05) when fed on M. sativa (Figure 1). The EPG data showed that, before the stylet reached the phloem, the Pisum host race of A. pisum spent more time in potential drops (aphids briefly puncture cells during plant penetration) than the Medicago host race (16 min vs. 27 min), as indicated by the "total pd" in Table 1. The time for the stylet to reach the phloem did not differ between the two host races, as indicated by the "time to first E1". Regarding the phloem-related parameters, the total duration of the E2 (aphids are ingesting the phloem sap) waveform were significantly reduced on average, from approximately 239 min in the Medicago host race to 123 min in the Pisum host race, as indicated by the "total E2". The total duration of E1 (aphids are injecting watery saliva into the sieve element) and the number of E1 or E2 did not differ between the two host races. The remaining parameters had little significance between the two host races of A. pisum (Table 1). The EPG data showed that, before the stylet reached the phloem, the Pisum host race of A. pisum spent more time in potential drops (aphids briefly puncture cells during plant penetration) than the Medicago host race (16 min vs. 27 min), as indicated by the "total pd" in Table 1. The time for the stylet to reach the phloem did not differ between the two host races, as indicated by the "time to first E1". Regarding the phloem-related parameters, the total duration of the E2 (aphids are ingesting the phloem sap) waveform were significantly reduced on average, from approximately 239 min in the Medicago host race to 123 min in the Pisum host race, as indicated by the "total E2". The total duration of E1 (aphids are injecting watery saliva into the sieve element) and the number of E1 or E2 did not differ between the two host races. The remaining parameters had little significance between the two host races of A. pisum (Table 1).

Concentrations of Foliar Phenolics in M. sativa
To explore the response of plant phenolics to the Medicago host race and the Pisum host race of A. pisum infestation, we analyzed the levels of the phenolics of M. sativa. The results showed that the foliar genistein content in M. sativa significantly increased when infested by the Pisum host race (5.4-fold larger than uninfested treatment, p < 0.05) but decreased in response to infestation by the Medicago host race relative to the uninfested plants (p < 0.05). Furthermore, the content of other foliar phenolics were unaffected by infestation with A. pisum (Figure 2).   To determine the effect of genistein on the two host races of A. pisum and the different responses of the two host races, we tested their survival rate on the diet with genistein. The exogenous application of 1 µg/cm −3 or 10 µg/cm −3 genistein into the artificial diet significantly reduced the survival rate of the Pisum host race of A. pisum relative to the control without genistein (p < 0.05), but the two concentrations of genistein did not affect those of the Medicago host race. There was no significant difference between the two host races of A. pisum when they fed on the diet without genistein. The survival rate of the Pisum host race of A. pisum was lower than Medicago host race with diets containing 1 µg/cm −3 (p < 0.05) or 10 µg/cm −3 (p < 0.05) genistein ( Figure 3).

Figure 2.
Concentrations of phenolics in the leaves of Medicago sativa with the infestation of the two host races of Acyrthosiphon pisum. The level of genistein induced by the Medicago host race was not detected. Each value represents the average (±SE). Different lowercase letters indicate significant differences among the aphid treatments, as determined by Tukey's multiple range tests at p < 0.05.

Figure 3.
Survival rate of the two host races of Acyrthosiphon pisum fed on artificial diets with the application of different concentrations of genistein. Each value represents the mean (±SE) of five replicates. "0" indicates the diets without genistein, which were used as a control. Different uppercase letters indicate significant differences among the genistein treatments within the same host races, as determined by Tukey's at p < 0.05. Different lowercase letters indicate significant differences between the two host races within the same genistein treatment, as determined by Student's t-test at p < 0.05. Figure 3. Survival rate of the two host races of Acyrthosiphon pisum fed on artificial diets with the application of different concentrations of genistein. Each value represents the mean (±SE) of five replicates. "0" indicates the diets without genistein, which were used as a control. Different uppercase letters indicate significant differences among the genistein treatments within the same host races, as determined by Tukey's at p < 0.05. Different lowercase letters indicate significant differences between the two host races within the same genistein treatment, as determined by Student's t-test at p < 0.05.  (Table S2, Supporting information). The overall variation in gene expression between the two host races was high. A total of 198 genes were differentially expressed between the two host races of A. pisum with a probability > 0.8 (probability, an odds value of 4:1 means that the gene is four times more likely to be differentially expressed than nondifferentially expressed) and a fold change threshold ≥ 2 (Figure 4a). Of the 198 genes in the two host races samples, 161 genes had higher expression in the Pisum host race relative to the Medicago host race, and 37 genes had lower expression (Tables S3 and S4, Supporting information). There were 67 genes coding for hypothetical proteins with unknown functions. Those (131) that shared homology with genes of known function in the database were categorized according to biological processes and molecular function (Figure 4c,d). Significantly enriched GO categories for genes with higher expression in the Pisum host race compared to the Medicago host race included biological regulation, cellular component organization or biogenesis, cellular process, metabolic processes, and the regulation of biological process response to stimulus, signaling, single-organism process, binding, catalytic activity, structural molecule activity, and transporter activity (Table S5, Supporting information). For the genes with lower expression in the Pisum host race compared to the Medicago host race, enriched GO categories included cellular component organization or biogenesis, cellular process, metabolic process, response to stimulus, single-organism process, binding, catalytic activity, and structural molecule activity (Table S6, Supporting information). The KEGG metabolic pathway analyses indicated that the very abundant categories for the differential expression of genes between the two host races on M. sativa were amino acid metabolism, carbohydrate metabolism, lipid metabolism, xenobiotics biodegradation and metabolism and nucleotide metabolism (Figure 4b).    Among the differentially expressed genes between the two host races of A. pisum on M. sativa, we identified six genes associated with detoxification (Table 2), which included UDP-glucuronosyltransferase 2B2 (LOC 100166729), UDP-glucuronosyltransferase 2B17 (LOC 100169601), UDP-glucuronosyltransferase 1-7C-like (LOC 100159691), glutathione-S-transferase (LOC100570856), cytochrome P450 6a13 (LOC100572007) and cytochrome P450 family 6 (LOC100569567). These genes showed higher expression in the Pisum host race samples relative to the Medicago host race samples with a probability ≥ 0.8 and a fold change ≥ 2. Consistent with the transcriptomic data, further qPCR experiments also confirmed that these six genes were all up-regulated in the Pisum host race when compared with the Medicago host race ( Figure 5).

Discussion
Divergent natural selection from host plant [33] or facultative symbionts [34] is generally regarded as the driving force of host race formation in insects. Thus, deciphering the unique traits under divergent selection is an essential step towards understanding host race formation [35]. We have shown that, since the Medicago host race of A. pisum down-regulated while the Pisum host race up-regulated the content of genistein, the Medicago host race had a higher population abundance and feeding efficiency on M. sativa than the Pisum host race. Furthermore, the up-regulation of six genes related to detoxification was observed in the Pisum host race of A. pisum, which suggests a physiological cost in the life history of the Pisum host race on M. sativa. This study provides a revolutionary insight into the interspecific interactions between the two host races of A. Pisum and their Fabaceae hosts.
The Medicago host races of A. pisum seem to be capable of colonizing a range of Fabaceae hosts with optimal fitness on their own host M. sativa, as well as other hosts, such as P. sativum. By contrast, the Trifolium host races and Pisum host races of A. pisum do not establish well on M. sativa. Further experiments on phytohormone-dependent resistance suggested that the Medicago host races impaired the JA signaling pathway of M. sativa by reducing the formation of 12-oxophytodienoic acid (OPDA), while the Pisum host races and Trifolium host races did not [15]. Moreover, the unique pattern of the aphid host races in manipulating the host defenses may result from the differentially expressed salivary proteins of aphids, which has important consequences for modifying the cross-talk between SA and JA signaling pathways [36]. A recent study showed that Armet, a salivary protein from A. pisum, can suppress the effective JA pathway through the modification of the SA pathway to benefit the feeding activity of A. pisum [37]. Mp10, a salivary protein from M. persicae, could activate both the JA and SA signaling pathways, which led to the relatively low fecundity upon Nicotiana benthamiana [36]. It was suggested that the failure of suppression in efficient host defenses may result in a lower

Discussion
Divergent natural selection from host plant [33] or facultative symbionts [34] is generally regarded as the driving force of host race formation in insects. Thus, deciphering the unique traits under divergent selection is an essential step towards understanding host race formation [35]. We have shown that, since the Medicago host race of A. pisum down-regulated while the Pisum host race up-regulated the content of genistein, the Medicago host race had a higher population abundance and feeding efficiency on M. sativa than the Pisum host race. Furthermore, the up-regulation of six genes related to detoxification was observed in the Pisum host race of A. pisum, which suggests a physiological cost in the life history of the Pisum host race on M. sativa. This study provides a revolutionary insight into the interspecific interactions between the two host races of A. Pisum and their Fabaceae hosts.
The Medicago host races of A. pisum seem to be capable of colonizing a range of Fabaceae hosts with optimal fitness on their own host M. sativa, as well as other hosts, such as P. sativum. By contrast, the Trifolium host races and Pisum host races of A. pisum do not establish well on M. sativa. Further experiments on phytohormone-dependent resistance suggested that the Medicago host races impaired the JA signaling pathway of M. sativa by reducing the formation of 12-oxophytodienoic acid (OPDA), while the Pisum host races and Trifolium host races did not [15]. Moreover, the unique pattern of the aphid host races in manipulating the host defenses may result from the differentially expressed salivary proteins of aphids, which has important consequences for modifying the cross-talk between SA and JA signaling pathways [36]. A recent study showed that Armet, a salivary protein from A. pisum, can suppress the effective JA pathway through the modification of the SA pathway to benefit the feeding activity of A. pisum [37]. Mp10, a salivary protein from M. persicae, could activate both the JA and SA signaling pathways, which led to the relatively low fecundity upon Nicotiana benthamiana [36]. It was suggested that the failure of suppression in efficient host defenses may result in a lower population fitness of the Pisum host race on M. sativa. Additionally, there are strong indications that some facultative endosymbionts of A. pisum contribute to host plant colonization. For example, most of the Trifolium host race of the A. pisum carried Regiella insecticola [38][39][40][41][42]. Once R. insecticola was removed, the fitness of the Trifolium host race of A. pisum was remarkably decreased when fed on T. repens. Nevertheless, inconsistent results also revealed that the acquisition of R. insecticola had little effect on improving the performance of some lineages of the Trifolium host race of A. pisum on T. pratense [43][44][45].
Plant phenolics include flavonoid glycosides, chlorogenic acid, and caffeic acid, which act as antifeedants or exhibit toxicity activity against aphid feeding, which leads to oxidative stress in the aphid tissues and attenuates aphid digestion and metabolism [46][47][48][49]. A previous study found that the application of genistein in an artificial diet prolonged the period of probing and shortened the passive ingestion duration of A. pisum, which suggested that genistein decreased the feeding efficiency of A. pisum [50]. Similar detrimental effects of genistein were also shown in other aphid species, i.e., Aphis glycines and Aphis craccivora [51,52]. Our result showed that the infestation of the Pisum host race induced the accumulation of genistein in M. sativa, which, in turn, reduced the survival rate of aphids and suggested that genistein is one of the components that are responsible for decreased fitness on M. sativa. Furthermore, the higher content of foliar genistein may result from longer penetration and probing durations of the Pisum host race, which causes stronger induced defenses in M. sativa. The antibiosis effects of rutoside and ferulic acid against phloem-sucking insects have been reported in soybean and barley [53,54]. Although these compounds were detected in our study, our data showed that there was little difference in the concentration of rutoside and ferulic acid between the two host races, suggesting these phenolics are likely not associated with resistance to the Pisum host race in M. sativa.
The strategies of phenolic metabolism in aphids include the avoidance absorption by the gut, elimination from the body cavity, and degradation by detoxifying enzymes [18]. A previous study showed that the genistein content in A. pisum would increase with the rise of genistein content in M. truncatula, which lead to the low performance of A. pisum on M. truncatula [21]. It is indicated that decreasing the accumulation of phytotoxins in the body cavity is an efficient way for aphids to adapt to plant secondary metabolites. Our study found that the Pisum host races had shorter phloem ingestion duration on M. sativa than those of the Medicago host races, which suggested that reduced feeding in M. sativa could effectively function to reduce the consumption and absorption of genistein by the Pisum host race.
Recent transcriptome data showed that a subset of chemosensory and salivary proteins may have an important role in the host-race formation of A. pisum [7]. Our transcriptome data found that the detoxification genes of aphids may participate in their host transfer and colonization. The GSTs and P450s of aphids are involved in the detoxification of toxic host plant allelochemicals [55][56][57]. For example, aphid GSTs have been reported to detoxify glucosinolates in Arabidopsis, nicotine in tobacco and the hydroxamic acid in cereal plants [23,58,59]. The detoxification-related genes were highly up-regulated in the Pisum host race, suggesting that a higher expression of detoxification enzymes is required for the Pisum host race to cope with M. sativa. This may cause a physiological cost, which reduces the fitness of the Pisum host race on M. sativa. A more detailed understanding of the molecular mechanisms of genistein degradation in aphids are needed to refine the utilization of the gene silencing approach for the future control of aphid infestation.
Supplementary Materials: The following are available online at http://www.mdpi.com/2075-4450/10/4/97/s1. Table S1: Primer sequences for quantitative PCR; Table S2: Summary of transcriptome parameters of Pisum host race samples and Medicago host race samples; Table S3: Genes with higher expression in the Pisum host race samples when compared to the Medicago host race samples; Table S4: Genes with lower expression in the Pisum host race samples when compared to the Medicago host race samples; Table S5: Significantly enriched Gene Ontology (GO) categories for genes with higher expression in the Pisum host race samples relative to the Medicago host race samples (FDP corrected p < 0.01); Table S6: Significantly enriched Gene Ontology (GO) categories for genes with lower expression in the Pisum host race samples relative to the Medicago host race samples (FDP corrected p < 0.01).