Assessment of Beauveria bassiana for the biological control of corn borer, Ostrinia furnacalis, in sweet maize by irrigation application

Ostrinia furnacalis egg masses were obtained from a laboratory colony maintained at the Institute of Plant Protection, Jilin Academy of Agricultural Sciences, Jilin, China (JAAS). Colony larvae were fed artificial diet and incubated at 26 ± 1 °C, 60–70% RH with a L:D 18:8 photoperiod) as described previously (Song et al. 1999). Moths were kept at constant temperature 26 °C with RH of 60–80% RH and a L:D 14:10 photoperiod, and egg masses laid on wax paper. Egg masses used in this study were laid by females the first day after caging. Furthermore, only egg masses with 60 eggs each were selected, allowed to develop to blackhead stage, and transported to the greenhouse in 2.0 ml air-permeable centrifuge tubes for infestations.

The B. bassiana strain GZ01 (preservation number 12471; China General Microbiological Culture Collection Center, Beijing, China) was maintained by JAAS as described in Online Resource (Supplementary material 1a). GZ01 was previously applied to control O. furnacalis on a large scale in maize production fields (Li 2015). Strain GZ01 was prepared as (1) pore suspensions at 1 × 10⁸ conidia ml⁻¹ (Online Resource Supplementary material 1b) or (2) conidia on ground maize stover granules at 1 × 10⁸ conidia g⁻¹ (Online Resource Supplementary material 1c). (2019).

Sweet maize seeds were sown in 30 cm diameter × 37 cm high pots with 20 kg of a 1:1 mix of local nutrient soil and placed in a greenhouse at JAAS (25 °C ± 2 °C during the day, 20 °C ± 2 °C during the night, RH 50–60%, L:D 12:12 photoperiod). Blastospore suspensions at 1 × 10⁸ conidia ml⁻¹ were prepared as described in Online Resource Supplementary material 1d. Fourteen plants were assigned to each inoculation of 20 ml of B. bassiana aerial conidia suspensions at 1 × 10⁸ conidia ml⁻¹ (I1); 20 ml of B. bassiana blastospore suspensions at 1 × 10⁸ conidia ml⁻¹ (I2); or 10 ml of aerial conidia suspensions and 10 ml of blastospore suspensions (I3). A 20 ml application of 0.05% Tween 80 was used as a control. For each treatment group, B. bassiana was applied to soil as seeds that were sown, and then poured onto soil every three days until the ear stage. Leaves were collected at Bundesanstalt, Bundessortenamt und Chemical Industrie (BBCH) defined growth stage 15 (five leaves unfolded) (Bleiholder et al. 2001) and surface sterilized, and transferred into potato dextrose agar (PDA) medium containing streptomycin sulphate (100 mg⁻¹) and incubated at 26 °C in the dark for seven days. Fungal growth was recorded daily for 15 days (Online Resource Supplementary material 1e). At BBCH growth stage 15 two 2nd instar O. furnacalis larvae were placed into the whorl leaves of each plant across all treatment groups using feather-tipped forceps. The leaf feeding ratings were recorded seven days after infestation.

Sweet maize seeds were germinated (Online Resource Supplementary material 1f) and sown in pots as described above. Eighty plants were distributed across 20 groups with four plants in each group, and a distance of 30 cm was maintained between plants within groups such that the leaves did not contact adjacent plants. Plants were grown in a greenhouse at JAAS (25 ℃ ± 2 ℃ during the day, 20 °C  ± 2 °C during the night, RH 50–60%, and a L:D 12:12 photoperiod). To avoid cross-contamination by splashing of soil during watering, an automatic dripping irrigation system was used for 1 h once every two days to replicate dry area conditions.

Each of the plants within groups was subjected to a different B. bassiana application and O. furnacalis infestation regime. Infestations consisted of pinning two black headed O. furnacalis egg masses on wax paper substrate to each plant, at one or two separate times to simulate O. furnacalis first-generation oviposition by placing the two egg masses into whorls, and second-generation oviposition by sticking the two eggs on the back side of leaves above the ears. Two treatments with five grams of B. bassiana granules with 1 × 10⁸ conidia g⁻¹ were applied five days post-O. furnacalis infestation: Treatment 1 (T1) a single application to the whorl of each plant at BBCH growth stage 15 (after first-generation O. furnacalis infestation); or Treatment 2 (T2) to whorls and on the ear at BBCH growth stages 15 and 65, respectively. Uninoculated controls infested at whorl (C1) or ear stage (C2) were included. Leaf feeding was rated seven days after egg infestation on whorl stage maize according to a Chinese national grading standard NY/T 1248.5–2006 (Supplementary Table S1; Wang et al. 2006). In the autumn, the entire stalk of the sweet maize from all treatments were dissected, stem internodes marked, then the number of living O. furnacalis larvae, the number of damaged plants, quantity location of corn borer entry holes per plant, and the length of tunneling were recorded.

Maize was grown in a greenhouse in the same replicated design as described above, except that five plants were included per group across 20 groups. Also, 20 ml of B. bassiana conidial suspension at 1 × 10⁸ conidia ml⁻¹ was poured onto soil at time of sowing, followed by three additional inoculations to plants at 3rd leaf stage, early whorl stage and early ear stage as described previously (Li 2015), and corresponding to BBCH growth stages 13, 39, and 65, respectively. Plants were infested with O. furnacalis egg masses at whorl and ear stages (Treatment 3; T3), whorl stage (Treatment 4; T4) or ear stage (Treatment 5; T5). Controls C1 and C2 were included as described above. Plants were infested with egg masses and rating of O. furnacalis damage was recorded as described in our methods above.

Differences in the efficacy of B. bassiana treatments were made independently within and between granule and suspension experiments for all measures: leaf feeding ratings, number boreholes, tunnel length, and number of dead and surviving O. furnacalis larvae. Significance in variation was assessed by one-way ANOVA. Due to uneven variance of empirical data, a square root transformation was used before ANOVA for tunnel length and average number of boreholes in respective plant nodes among the granule treatments. Post-hoc Tukey’s Honest Significant Difference (HSD) tests were then performed on leaf feeding ratings, number boreholes, tunnel length, and number of dead and surviving O. furnacalis larvae within and between granule and suspension experiments. All statistical analyses used the multcomp package (http://​multcomp.​r-forge.​r-project.​org; Bretz et al. 2011) in R 4.4.2 (R Core Team 2022) via the integrated development environment, Rstudio 2022. 07.2 + 576 (RStudio Team, 2019).

We detected B. bassiana in maize leaves treated with B. bassiana spore suspensions (Fig. S1), with colonization rates for blastospores and aerial conidia treatment (50%), blastospores treatment (50%) and aerial conidia suspensions treatment (57.14%). No B. bassiana colonies were formed by samples from un-inoculated controls (Supplementary Fig. S1). The leaf feeding ratings for first-generation of O. furnacalis damage (Table 1) were significantly different (F_3,52 = 5.141, p = 0.0035), with subsequent Tukey’s HSD tests showing significance only between control (C) and aerial conidia & blastospore treatment (I3; p = 0.0019; Table 1).

Number of surviving larvae and measures of damage to maize among controls (C1 and C2) and treatments (T1 and T2: Table 2) showed that O. furnacalis can be controlled when B. bassiana granules were applied to maize whorl based on measurements taken seven days after O. furnacalis infestation. Specifically, significant variation was detected among C1, C2, T1 and T2 for all measures (F_3,76 ≥ 3.873, p ≤ 0.0124, Supplementary Table S2a). Significantly lower levels of O. furnacalis damage in maize treated with granules at whorl stage and those infested at whorl and ear stages (T1) compared to controls infested at whorl stage (C1), as detected by Tukey’s HSD tests for leaf feeding ratings (Q_k=4,v=76 = 11.260, p = 0.0010, Supplementary Table S2a), and borehole number (Q_4,76 = 4.174, p = 0.0215, Supplementary Table S2b). Significant differences were also detected between T1 and C2 (infested at ear stage) for leaf feeding rating (Q_4,76 = 6.878, p = 0.0010, Supplementary Table S2a), the borehole number (Q_4,76 = 6.061, p = 0.0010, Supplementary Table S2b), the tunnel lengths (Q_4,76 = 4.977, p = 0.0040, Supplementary Table S2c) and the number of surviving larvae (Q_4,76 = 4.276, p = 0.0193, Supplementary Table S2d), wherein all rating were lower for treatments compared to control groups. Compared to uninoculated C1 (infested at whorl stage), T2 (granular B. bassiana applications and O. furnacalis infestations at both whorl and ear stages) showed significantly lower leaf feeding ratings (Q_4,76 = 7.987, p = 0.0010, Supplementary Table S2a), and borehole number (Q_4,76 = 4.968, p < 0.0041, Supplementary Table S2b). Analogously, T2 was significantly lower than C2 plants in the number of boreholes (Q_4,76 = 6.856, p = 0.0010, Supplementary Table S2b), tunnel lengths (Q_4,76 = 4.602, p = 0.0090, Supplementary Table S2c), and the number of alive larvae (Q_4,76 = 3.842, p = 0.0399, Supplementary Table S2d). C1 and C2 showed significant differences only in leaf feeding ratings (Q_4,76 = 4.282, p = 0.0142, Supplementary Table S2; Fig. 1a). No differences in levels of damage were observed between T1 and T2. These results revealed the relative equivalence of B. bassiana granule treatments at whorl stage and at both whorl and ear stages for reducing O. furnacalis leaf feeding ratings (Fig. 1a, Table 2) as well as decreasing borehole number, tunnel length, and number of surviving larvae (Fig. 1b, Table 2).

The spatial distribution of O. furnacalis damage was biased towards the middle part of the plant at internodes around the ear. Within treatments and controls there were significant differences in the number of boreholes and tunnel length between upper, middle and lower internodes (Fig. 2; p < 0.05; remaining data not shown).

The second B. bassiana application method used suspensions that were sprayed on soil and vegetative tissues to simulate repeated overhead field irrigations. These resulted in significant differences in 7-day post-infestation damage ratings between all treatments and control plants across all measures (F_4,95 ≥ 3.290, p ≤ 0.0143; Supplementary Table S2a). Specifically, for infestations at whorl stage the ratings were significant lower in T4 compared to C1 for leaf feeding (Q_5,96 = 6.081, p = 0.0010, Supplementary Table S2a), and borehole number (Q_5,96 = 5.183, p = 0.0037, Table S2b). Plants treated with Beauveria in aqueous suspension and infested in ear stage in T5 showed significantly lower number of boreholes (Q_5,96 = 6.201, p = 0.0010, Supplementary Table S2b), tunnel lengths (Q_5,96 = 4.707, p = 0.0107, Supplementary Table S2c) and the number of surviving larvae (Q_5,96 = 4.010, p = 0.0434, Supplementary Table S2d) compared to its corresponding C2. In contrast, borehole number and tunnel lengths of plants infested in whorl and ear stages (T3) did not differ significantly from either of the two controls, C1 or C2. These measures were significantly higher in T3 compared to T4 (infestation at whorl stage) (Q_5,96 = 7.556, p < 0.0010, Supplementary Table S2b; Q_5,96 = 4.935, p = 0.0065, Supplementary Table S2c). Only borehole number was different between T3 and T5 (infestation at ear stage) (Q_5,96 = 6.612, p < 0.0001, Supplementary Table S2b). The number of dead larvae was not significantly different among the treatments or when compared to their controls (Fig. 1d).

Boreholes on maize treated with B. bassiana suspension were predominantly documented in the internodes around the ear node, whereas internodes above the ear had fewer than those below the ear. This was similarly shown for tunnel length. There were significant differences among the upper, middle and lower internodes of stalks in the same treatment for borehole number and the tunnel length (Fig. 2; p < 0.05; remaining data not shown).

Significant variation was detected among a combination of granular and suspension treatments for leaf feeding ratings (F_4,95 = 2.779, p = 0.0312), borehole number (F_4,95 = 9.407, p < 0.0001), and tunnel lengths (F_4,95 = 3.642, p = 0.0083) (Supplementary Table S2), but not for number of surviving larvae (F_4,95 = 1.493, p = 0.2105). Results of subsequent Tukey’s HSD tests for leaf feeding ratings, borehole number, and tunnel length data indicated a total of four significant differences between treatments from granular (T1 and T2) and suspension treatments (T3, T4, and T5). Specifically, three of these significance estimates were a consequence of higher readings for T3 compared to T1 (Q_5,96 ≥ 4.089, p ≤ 0.0374) (Supplementary Table S2).