Brown planthopper population used in the experiments were originally collected from rice fields in Hangzhou (E120°12, N30°16), China. Successive generations were maintained on the susceptible rice variety TN1 in a climatic chamber under constant conditions of 26 ± 1°C, 70–80% relative humidity and a 16 h light/8 h dark photoperiod. The TN1 seedlings were cultured in 14 cm diameter plastic pots and used for BPH mass rearing at the tillering stage (height: 14–16 cm).

The fungicide 50% propiconazole ME was provided from Qingdao Hengyuanxiang Chemical Co., Ltd., Propiconazole was diluted with 0.01 mol/L phosphate buffer solution (PBS) to 0.17 ng/nL. The final concentration for microinjection was determined by the preliminary gradient experiments. Thirty BPH nymphs in the 5th instar or 1-day-old female adults were used for microinjection for each treatment with five replications. The BPH individuals were anesthetized using CO₂ for 30 s and fixed on 4% agarose plate with their abdomen facing up. Propiconazole at 17 ng (100 nL) was injected into each BPH thorax using the FemtoJet 4i microinjection device (Eppendorf, Germany), and the injection sites were located on the conjunction between prothorax and mesothorax (Lu et al., 2015). The treatments with 0.01 mol/L PBS and without microinjection were used as the negative and the blank controls, respectively. BPH samples were collected at day 1, day 2, and day 4 after injection to investigate the number of YLS and H. chrysospermus. The mortality and fecundity of BPH were investigated and calculated correspondingly.

Foliar spraying with propiconazole was carried out at the rice tillering stage using a mini-sprayer. Propiconazole was used at the recommended concentration (0.5 mg/mL) in the field trial. Three stems of sprayed rice plants were placed in a test tube (2.5 cm in diameter and 30 cm in height) filled with 20 ml rice nutrient solution (Wilkinson and Ishikawa, 2001; Shentu et al., 2016). Thirty fifth-instar nymphs or 1-day-old female adults were released into the test tube, which was covered with two pieces of gauze. These were then kept in a constant temperature room at 26 ± 1°C with 16 h light/8 h dark photoperiod. Five replications were performed in each treatment. The treatment sprayed with water only was used as the negative control. The mortality and fecundity of BPH were calculated. The number of YLS and H. chrysospermus in the BPH body was investigated at day 1, day 2, and day 4 after BPH release.

Brown planthopper samples were sterilized by immersion in 75% ethanol for 3 min and then washed quickly with 0.01 mol/L PBS for 90 s. The fat bodies in the BPH abdomen and the hemolymph in the BPH thorax were collected by dissection and homogenized in 0.01 mol/L ice-cold PBS at pH 7.4 Percoll (Pharmacia, Sweden), respectively (Shentu et al., 2016). The total number of YLS in the fat body and the hemolymph were counted on a hemocytometer under a binocular microscope (400 ×). Each sample was observed in triplicate.

Total DNA of YLS in the hemolymph and fat body was extracted using a Yeast DNA Mini Kit (Tiangen Biotech Co., Ltd., Beijing, China). The DNA concentration was measured using a spectrophotometer (Nanodrop). To estimate the abundance of H. chrysospermus, the copy number of the 18S rDNA (Genbank: AF267233.1) fragment was measured by qPCR (Applied Biosystems) using a FastStart Universal SYBR Green Master(ROX) (Roche Biotechnology Co., Ltd.), and the two primers used for qPCR amplification were F: 5′-CGTAGGAGAGCAGCAAAC-3′ and R: 5′-CGATGCCAGAGCCAAGA G-3′. The actin (Genbank: KU365929.1) was used as the reference gene. The primers were F:5′-GATGAGGCGCAGTCAAAGAG-3′ and R:5′-GTCATCTTCTCACGGTTGG C-3′. The primers were designed by Primer Premier 5.0 with DNA sequence and cDNA sequence. The resulting PCR products were cloned into a pMD18-T vector (TaKaRa Biotechnology (Dalian) Co., Ltd.). The inserted gene fragments were sequenced and were proven to correspond to a part of the target gene. The qPCR was performed in a 20 μL total reaction volume containing 10 μL of FastStart Universal SYBR Green Master(ROX), 2 μL of template DNA, 0.8 μL of forward primer (10 μM), 0.8 μL of reverse primer (10 μM), and 6.4 μL of ddH₂O. The qPCR reactions were pre-denatured at 95°C for 10 min, followed by 40 cycles of 95°C for 15 s and 60°C for 1 min. Each DNA template was analyzed in triplicate. The acceptable qPCR standard curve (0.9 ≤E ≤ 1.0, R² ≥ 0.99) for each gene was optimized by altering the annealing temperature and time. The normalized fold changes of the target gene DNA copy number were expressed as 2^-ΔΔCT (Schmittgen and Livak, 2008).

Propiconazole standard sample was purchased from Aladdin–Holdings Group. Fifteen BPH individuals in group were dissected, and their hemolymph and gut were collected and homogenized in 0.01 mol/L PBS at pH 7.4 Percoll (Pharmacia, Sweden), respectively (Shentu et al., 2016). Then, the PBS extraction solution was subjected to centrifugation (12,000 r/min, 5 min) to obtain the supernatant. The 500 μL supernatant was filtrated with 0.22 μm filter membrane. The residue of propiconazole was analyzed using a Waters e2695 HPLC (2998 PDA Detector, Waters Workstation, United States) (Mu et al., 2005). The mobile phase was methanol and water (85:15, v/v). The detection wavelength was 225 nm, and the flow speed was 1.0 mL/min. The column (RP-C18 column) temperature was maintained at 30°C (250 mm × 4.6 mm, 5 μm, XBridgeTM, Waters, United States).

Values were expressed as mean ± SE. All data were analyzed with SPSS, version 24.0. Comparisons of the means were conducted based on Least Significant Difference (LSD) test following a one-way analysis of variance (ANOVA). Differences between means was deemed significant and highly significant when P < 0.05 and P < 0.01, respectively.

Effect of propiconazole on the YLS in hemolymph and fat body of BPH was indicated in Figure 1A–D. The total number of all YLS in BPH generally increased with the growth of host BPH (Figure 1A,B). One day after propiconazole microinjection, the total number of YLS in the hemolymph of nymph decreased as low as 33.6% of that in the negative control (PBS treatment). At days 2 and 4 after microinjection, the numbers of YLS in the treatment with propiconazole significantly declined to 48.7 and 50.6% as compared with that in the negative control, respectively (P < 0.05). Similar results were also obtained from the treatment of BPH female adults. The total number of YLS in the hemolymph of female adults obviously declined when treated with propiconazole. Especially at day 4 after microinjection, the number of the YLS dropped to 18.9 % of that in the negative control (PBS treatment) (Figure 1A).

The total number of YLS in the BPH fat body after propiconazole microinjection was significantly lower than that of untreated or PBS-treated controls (P < 0.05). For the 5th instar nymph and 1-day-old female adults, the growth and reproduction of YLS was effectively suppressed at day 1 (a drop of 43.3 and 21.2%), day 2 (a drop of 32.7 and 53.8%), and day 4 (a drop of 35.2 and 42.6%) after propiconazole microinjection as compared with PBS microinjection, respectively (Figure 1B).

The number of H. chrysospermus was analyzed after microinjection (Figure 1C,D). In the 5th instar BPH nymph, the number of H. chrysospermus increased with BPH growth. However, the number of H. chrysospermus in the BPH hemolymph treated with propiconazole was significantly decreased compared with that of the PBS-control (P < 0.05). On 1-day-old female adults, the number of H. chrysospermus had rapid declined at day 1 (a decline of 90%), day 2 (a decline of 65%), and day 4 (a decline of 76%) after propiconazole microinjection as compared with PBS microinjection (Figure 1C). Meanwhile, a big decline in the number of H. chrysospermus was observed after propiconazole microinjection in BPH fat body (Figure 1D).

The survival rates of BPH by hemolymph microinjection were indicated in Figure 2A,B. During days 1 and 3 after microinjection, there was a significant difference in the survival rates of the 5th instar nymph between BPH treated with propiconazole and PBS (P < 0.05) (Figure 2A). Furthermore, from days 4 to 8 after propiconazole microinjection, the survival rate of 5th instar nymph was highly significantly lower than that of the control treated with PBS (P < 0.01). The BPH survival rate was 40% after microinjection at day 8, which was lower by half of the BPH survival rate after treatment with PBS microinjection (Figure 2A). During days 5 and 8, the survival rates of 1-day-old female adults treated with propiconazole were significantly different from those treated with PBS (P < 0.05) (Figure 2B).

The fecundity of BPH females significantly decreased after propiconazole microinjection (P < 0.05) (Figure 3). Female adults (1-day-old) laid 229 eggs per female after propiconazole microinjection, which was 20% lower than the control treated with PBS. For BPH treated in the 5th instar nymph, the oviposition of BPH treated with propiconazole was 195 eggs per female, which was only 75% of the PBS treatment.

The effect of fungicide on YLS after foliar spraying was shown in Figure 4A,B. From day 1 to day 3 after spraying, the number of YLS in the BPH hemolymph in 5th instar nymph was similar to that of water-treated BPH. However, the numbers of YLS in 1-day-old female adults significantly declined to 32, 29, and 22% of the negative control at day 1, day 2, and day 4 after foliar spraying, respectively (Figure 4A).

In the fat body of the 5th instar nymph, the number of YLS reduced significantly at day 1 and day 4 after foliar spraying with propiconazole compared with the water-treated control (P < 0.05). Meanwhile the growth and reproduction of YLS in 1-day-old female adults was also significantly inhibited at day 2 and day 4 after foliar spraying with propiconazole (P < 0.05) (Figure 4B).

The number of the dominant YLS species, H. chrysospermus, decreased after foliar spraying with propiconazole in the 5th instar nymphs and 1-day-old female adults (Figure 4C,D). Particularly, the number of H. chrysospermus in 1-day-old female adults significantly decreased at day 1 (a drop of 86%), day 2 (a drop of 81%), and day 4 (a drop of 81%) after foliar spraying with propiconazole compared with the negative control (P < 0.05) (Figure 4C). In the BPH fat body, an obvious reduction in the number of H. chrysospermus at day 2 and day 4 was observed after foliar spraying with propiconazole (Figure 4D).

From day 1 to day 5 after foliar spraying with propiconazole, there was no significant difference between the treatment and negative control in both the 5th instar nymph and 1-day-old female adults (P < 0.05) (Figure 5A,B). Furthermore, from day 6 to day 8 after foliar spraying, the survival rates of the 5th nymph and 1-day-old female adults of BPH showed significant differences between propiconazole and water treatments (P < 0.05).

The fecundity of BPH significantly decreased after foliar spraying with propiconazole (Figure 6). The BPH treated with fungicide at the 5th nymph and 1-day-old female adults laid 199 and 214 eggs per female, respectively, which were 27 and 31% drops compared with the water-treated BPH.

In the foliar spraying test, the residue of propiconazole in the hemolymph and gut was detected at day 1 after BPH release and the result was shown in Figure 7. According to the retention time and ultraviolet absorption spectrum of propiconazole by HPLC, there were propiconazole residues in the hemolymph and gut of BPH, respectively. The concentration of propiconazole residue in the gut was higher than in the hemolymph.