Plants and aphids

To measure the toxicity effects and aphid behaviour in relation to MPR, climate-controlled experiments were performed. In addition, two climate-controlled experiments were performed to compare timing and intensity of MPR between different genotypes of sugar beet. All indoor climate-controlled experiments were conducted at the Dutch Institute for Sugar Beet Research (IRS, Dinteloord, the Netherlands). Trial conditions were at a 16 h:8 h light:dark period (LED 119 mmol m⁻² s⁻¹, RAZRx PLUS, Fluence Bioengineering, Austin, Texas, USA) with 23°C during the day and 16°C during the night. Unless mentioned otherwise, 6-week-old sugar beet plants (8th–10th leaf stage) of a commercial variety of Strube (D&S GmbH, Söllingen, Germany) were used. Seeds were sown on sterilized river sand to which Dolokal (0.3% (v/v)) and Osmocote Exact Mini (ICL speciality fertilizer; 0.1% (v/v)) were added. Dolokal contains calcium carbonate, magnesium carbonate and magnesium oxide, preventing a low pH. Osmocote is a controlled release fertilizer, consisting of a resin-coated nutrient core containing nitrogen, phosphorus and potassium. After one week, plants were transferred to 700 ml pots containing 50:50 river sand:potting soil (Primasta, zaai-en stekgrond, Primasta, Asten, The Netherlands). For all experiments, the oldest fully expanded leaf without symptoms of senescence was used. In practice, this was always a leaf from the second-oldest leaf pair as during the experiments the two oldest leaves started to display senescence symptoms such as yellowing.

In all experiments, apterous nymphs of the green peach aphid (M. persicae) were used and reared on 6–10 weeks old sugar beet plants. For infestation of plants in the climate-controlled experiments, aphids were synchronized by placing fully grown apterous aphids on 6-week-old sugar beet plants. After 2–3 days the adults were removed and 3 days after removal, the 5–6 days old nymphs were used for infestation. For climate-controlled and field experiments, onset and intensity of MPR was monitored by visually assessing the presence of the black deposit in the stomach in individual aphids. If aphids died without a black deposit, these aphids were not included in the analysis, because no distinction could be made with aphids which died from other causes (e.g. not feeding or broken stylet).

Toxicity effects of MPR in young plants on aphids

To compare the toxicity effects of young and old sugar beet leaves on M. persicae, climate-controlled experiments were performed, in which mortality, number of black deposits and fecundity were investigated. Aphid development on old and young leaves was compared by counting the aphid numbers and appearance of the black deposit in the stomach after 3, 7, 10 and 14 days. For each replicate, ten aphids were confined on the inner leaf of the plant by a small tube made of a fine mesh (250 μ) (fig. S1A), or on the oldest fully expanded leaf (without clear senescence symptoms, such as yellowing) by a self-made box, made of a Petri dish, with a rectangular cut-out of 8 × 8 cm, covered with a fine mesh. Around the plant stem, foam was placed to close the hole and prevent aphids from escaping (fig. S1B).

Aphid preference assay

To explore the effects of MPR on aphid behaviour, the aphid preference for older or younger sugar beet leaves was investigated under climate-controlled conditions by placing 30 nymphs (5–6 days old) on a 6 × 3 cm paper on top of a 6-week-old sugar beet plant. The paper was positioned in such a way that it was in contact with the youngest and oldest leaves, allowing the aphids to move freely over the plants. Five days post infestation (DPI), the locations of the aphids were monitored.

Electrical Penetration Graph recording

To further explore the effects of MPR on aphid behaviour, Electrical Penetration Graph (EPG) recordings (McLean and Kinsey, Reference McLean and Kinsey1964; Tjallingii, Reference Tjallingii1988) were performed, according to an adapted methodology by ten Broeke et al. (Reference ten Broeke, Dicke and van Loon2013). In short, an 18 μm-thin gold wire with a length of 2 ± 0.5 cm was gently attached to the back of the aphid using water-based silver glue. Subsequently, aphids were either placed on the adaxial side of a young heart leaf, or on the adaxial side of an oldest fully expanded leaf (without clear senescence symptoms such as yellowing) of a 6-week-old sugar beet plant. Aphid behaviour was monitored with a Direct Current Giga-8 system (http://www.epgsystems.eu) for a total duration of 8 h with the program EPG Stylet + d. Annotation of the waveforms was done in EPG Stylet + a (www.epgsystems.eu). During each recording, a total of ten aphids could be monitored; one per plant. During each recording, five aphids were placed on young leaves and five on old leaves in an alternating position within a Faraday cage. In total, seven EPG recordings, of each ten aphids, were performed. For the analysis, 29 EPG annotation files from aphids on young heart leaves, were compared to 34 EPG annotation files from aphids on older leaves and further processed in R (R-Core-Team, 2020). Aphid feeding behaviour was compared for 22 feeding characteristics (table S1) by performing Mann–Whitney U tests (sometimes with continuity correction), and in case of proportional variables, Pearson's χ² tests with Yates' continuity correction. Waveforms that did not occur were considered as missing data for total duration, mean duration and latency variables. Feeding events that were interrupted by the end of the recording, and thus continued after the 8 h of recording, were included in all calculations.

Variation in mature plant resistance between plant genotypes

To investigate the variation in the intensity and timing in MPR, two climate-controlled experiments and one field experiment were performed. For this, two hybrids and three recombinant inbred parent genotypes were used, provided by SESVanderHave (Tienen, Belgium) (table 1). One commercial variety originally obtained from Strube (see above) was used as a control. The seeds were treated with standard amounts of the fungicide hymexazol (g ai/unit) for Aphanomyces and the pyrethroid contact insecticide tefluthrin, except for genotype 2 which was only treated with hymexazol. Tefluthrin is a soil pesticide with no systemic activity that might affect aphids. The seeds from the cultivar from Strube were also treated with the fungicides sedaxane, fludioxonyl and metalaxyl-M (fig. S2).

Table 1. Specifications of the sugar beet genotypes provided by SESVanderHave and Strube used in the experiments

To test for differences in MPR under climate-controlled conditions, two climate room experiments were performed in which the six sugar beet genotypes were compared in a randomized block design with ten replicates. Ten aphids were confined on the second oldest leaf pair of 6-week-old plants and 3, 7, 10 and 14 DPI aphid numbers (alive and dead) and the presence of the black deposit were registered.

In addition, to compare climate-controlled conditions with outdoor trials, a field experiment was performed at Oude Molen (Noord-Brabant, The Netherlands). Seeds from the six different sugar beet genotypes were sown in a complete randomized block design with four blocks. The seeds were sown to final stand with a specialised seed drill on 27 March 2020. Tillage, seed bed preparation and applications of fertilizers and pesticides (except for insecticides) were done according to the best local practice. Over the growing season, plants were infested with M. persicae at four different time points after sowing. For the confinement, ten aphids were placed on a leaf surrounded by a bag made of an aphid proof mesh (Polyester, 250 μ). Foam was used to properly and non-intrusively close the bag around the stem. After placing the aphids in the bag, the bag was closed at the top with a fine wire. For all infestations, bags of one size were used (20 × 39 cm) (fig. S1C). The dates of the infestations were: 7 May (6 weeks), 25 May (9 weeks), 22 June (13 weeks) and 13 July (16 weeks). During the infestations, plants were in their 4th, 8th–10th, 16th–22nd and 24th–30th leaf stage, respectively. In total, 40 plants per sugar beet genotype (without VY symptoms) were selected for infestation, ten plants for each time point of infestation. At 4 DPI, the bags with the leaves were collected from 20 plants per genotype and taken to the laboratory, where aphid numbers were counted and the presence of the black deposit was noted. The infested leaves from the remaining 20 plants were collected and counted 8 DPI.

Statistical analysis

To model the probability that a single aphid will accumulate a black deposit in its stomach, generalized linear models with a log link function were used to ensure positive fitted values.

To determine the effect of leaf age on the probability that an aphid will become black in the climate-controlled experiment, the following model was applied:

(1)$$\eqalignno{& \left. {\displaystyle{{\,p_{{\rm blac}{\rm k}_i}} \over {1-p_{{\rm blac}{\rm k}_i}}}} \right\vert u = \exp ( {\rm \mu }_0 + {\rm \beta }_1{\rm Age}\;{\rm Lea}{\rm f}_i + {\rm \beta }_2{\rm DP}{\rm I}_i + u\,{\rm Plan}{\rm t}_i + {\rm \varepsilon }_i) \cr & \quad \quad \quad \quad \,\,\,{\rm \varepsilon }_i\sim N( 0, \;\,\sigma ^2) & ( 1)} $$

Here, $p_{{\rm black}_i}}$ is the probability that aphid i will become black. By rewriting the probability into odds ${\frac{p_{{\rm blac}{\rm k}_i}}{ 1-p_{{\rm blac}{\rm k}_i}}$, it was possible to apply a linear regression model as per definition of the logit model. In equation 1, β₁ and β₂ represent the estimated coefficients of the parameters Age Leaf and DPI (days post infestation), respectively. Age Leaf is a binary independent variable which represents (1) the young inner heart leaves, or (2) the oldest leaves (without clear senescence symptoms such as yellowing). The factor DPI has four levels, as measurements were taken at 3, 7, 10 and 14 DPI. In this experiment, groups of aphids were confined for an extended time on separate plants. As a result, the observed aphids with black deposits on each plant for a separate time interval were not an independent measurement. Aphids that were observed to have a black deposit on a specific plant (Plant_i) would also be observed to have a black deposit in sequential time steps, creating a pooled dataset. This dependence was corrected for by using a random effects model in which the probability $p_{{\rm black}_i}}$ was modelled, given the estimated random effect (u) of each plant. ε _i represents the error term.

For the climate chamber experiment in which multiple sugar beet genotypes were compared, the following model was applied:

(2)$$\eqalignno{& \left. {\displaystyle{{\,p_{{\rm blac}{\rm k}_i}} \over {1-p_{{\rm blac}{\rm k}_i}}}} \right\vert u = \exp ( {{\rm \mu }_0 + {\rm \beta }_1{\rm Genotyp}{\rm e}_i + {\rm \beta }_2{\rm DP}{\rm I}_i + u\,{\rm Plan}{\rm t}_i + {\rm \varepsilon }_i} ) \cr & \quad \quad \quad \quad \quad {\rm \varepsilon }_i\sim N( 0, \;\,\sigma ^2) & (2)} $$

Here, Genotype represents the six sugar beet genotypes. The factor DPI and the random effect u for each Plant represent the same as in equation 1.

For the field trial, the model was as follows:

(3)$$\fleqalignno{\left. {\displaystyle{{\,p_{{\rm blac}{\rm k}_i}} \over {1-p_{{\rm blac}{\rm k}_i}}}} \right\vert u &= {\rm exp}( {{\rm \mu }_0 + {\rm \beta }_1{\rm Genotyp}{\rm e}_i + {\rm \beta }_2{\rm DP}{\rm I}_i + {\rm \beta }_3{\rm Dat}{\rm e}_i} \cr &{ + {\rm \beta }_{1 \times 2}{\rm Genotyp}{\rm e}_i \times {\rm DP}{\rm I}_i + {\rm \beta }_{1 \times 3}\;{\rm Genotyp}{\rm e}_i \times {\rm Dat}{\rm e}_i }\cr&+ {u\,{\rm Plan}{\rm t}_i + {\rm \varepsilon }_i} ) \cr&{\rm \varepsilon }_i\sim N( 0, \;\,{\rm \sigma }_{\rm \varepsilon }^2 ) \hskip5.3pc& \hskip1.2pc ( 3)} $$

Here, Genotype represents the individual sugar beet genotypes. The factor Date represents the four infestation times. In this experiment, DPI is a binary variable and modelled whether aphids were confined for 4 or 8 days on the leaf. In this experiment, ten aphids were confined on the same leaf of an individual plant. As a result, the number of observed aphids with black deposits on each plant is not an independent measurement and the random effect u for each Plant had to be included. For both Date and DPI, we investigated if there was a different impact for each genotype on the probability of aphids turning black by adding the interaction terms Genotype × Date and Genotype × DPI. Other interactions did not have significant effects on the formation of black deposits and were therefore taken out of the model.

For the analysis, the function glmer of the R package ‘stats’ (R-Core-Team, 2020) was used to fit the model (equations 1–3). The package ggplot2 (Wickham, Reference Wickham2016) was used to make graphs. The dataset met all requirements for a logit regression. Overdispersion was not an issue with a binary response variable. Statistical analyses of the EPG data are described in the paragraph ‘Electrical Penetration Graph recording’.