Insect rearing

The Spodoptera litura population was gotten from School of Life Sciences, Sun Yat-sen University. And they were reared on an artificial diet (Chen et al., Reference Chen, Li and Pang2000) at 25 ± 1°C in a 14L:10D photoperiod and 70–80% relative humidity in intelligent light incubator from 2013. The newly emerged adults were transferred to a one-end open cylindrical plastic cage (Φ = 12 cm, H = 25 cm) covered with filter paper in inner around and a cotton cloth at the open end, honey added as a diet supplement.

Gene cloning

Total RNA was isolated from about 100 mg fat body from 6th larvae using the Trizol reagent according to the manufacturer's specifications (Invitrogen, USA). First-strand complementary DNA was synthesized from 2 μg total RNA using a first strand synthesis kit (PrimeScript™ II 1st Strand cDNA Synthesis Kit, TaKaRa, Japan). The intermediate fragment of AKHR was amplified by a pair of degenerate primers which were designed based on the conserved amino acid sequences of the reported insect AKHRs in NCBI database (table 1). The PCR was carried out with the following conditions: initial preheating for 5 min at 94 °C, 35 cycles at 94 °C for 30 s, 48 °C for 30 s and 72 °C for 1 min, and with a final extension at 72 °C for 10 min using the primer pair SlAKHR-F1and SlAKHR-R1.

Table 1. Primers used in this study

For the full-length cDNA cloning, A Rapid Amplification of cDNA Ends (RACE) Kit (Clontech, Japan) was used. Specific primers for the 5′-and 3′-Rapid RACE were designed based on partial SlAKHR cDNA sequence amplified by the degenerate primers SlAKHR-F1 and SlAKHR-R1. The specific primers GSP1 and NGSP1 were used for 5′-RACE, while GSP2 and NGSP2 used for 3′-RACE (table 1).

Expression profiles of SlAKHR

The AKHR transcript levels were detected by quantitative real-time PCR (qRT-PCR) using an iCycler iQ (BIO-RAD, Hercules, CA) and SYBR Premix Ex Taq (Takara, Japan). Briefly, each qRT-PCR mixture contained 10 μl total volume: 5 μl TB Green Premix Ex Taq II (Tli RNaseH Plus) (Takara), 0.4 μl forward and 0.4 μl reverse primers (10 μM), 3.2 μl MilliQ water and 1 μl cDNA. The target gene primer pair SlAKHR-qF1 and SlAKHR-qR1 was used with a housekeeping gene (Ribosomal protein L10, RPL10, GenBank Acc. No. KC866373) primers SlRPL10-qF1 and SlRPL10-qR1. The qRT-PCR was performed in a CFX Connect Real-Time System (BIO-RAD) under the following conditions: one cycle for 30 s at 95°C, followed by 40 cycles of 10 s at 95°C, 30 s at 60°C and 30 s at 72°C. The data were normalized to the reference gene (RPL10) expression. The relative expression levels were calculated by 2^−ΔΔCT method (Livak and Schmittgen, Reference Livak and Schmittgen2001).

To investigate the expression pattern of different developmental phases and tissues, we got the 1st to 6th larvae, pupae, newly female adults. And the head, ovaries, midgut, fat body of newly female adults were carefully separated and collected. The specimen or tissues were rinsed in PBS buffer (0.01 M, pH = 7.4) several times, and each tissue was pooled from 8–10 individuals. Total RNA was isolated from all samples and obtained the first-strand cDNA as above.

Gene characterizationand phylogenetic analysis

The signal peptide of the AKHR was predicted with the SignalP server (http://www.cbs.dtu.dk/services/SignalP). And the transmembrane domain predicting was executed under the the TMHMM server (http://www.cbs.dtu.dk/services/TMHMM). The alignment of all sequences were generated using the MultiAlin website server (http://multalin.toulouse.inra.fr/multalin/multalin.html). The neighbor-joining (NJ) tree was produced in MEGA 6.0 software (Tamura et al., Reference Tamura, Stecher, Peterson, Filipski and Kumar2013) with Maximum-likelihood analysis using the Jones-Taylor-Thornton model (1000 bootstrap replicates). AKHR amino acid sequences used for phylogenetic analysis derived from other reported sequences.

RNA interference

According to the manufacturer recommendations of T7 RiboMAX™ Express RNAi System(Promega), two pairs of primers (SlAKHR ds-F1,SlAKHR ds-R1, T7 SlAKHR ds-F and T7 SlAKHR ds-R) (table 1) were designed to synthesize the 544-bp (734–1278 bp) region of the SlAKHR gene that included a T7 promoter region in both the sense and antisense strands, The SlAKHR cDNAs from fat body was used as a template, The amplification reactions protocol comprised 36 cycles of 95 °C for 40 s, 55 °C for 45 s and 72 °C for 60 s, with a final extension step of 72 °C for 10 min. The sequence was verified by sequencing (Huada gene company, Shenzhen, China). The EGFP gene (DQ768212.1) was used as a control dsRNA. The PCR primers EGFP dsRNA-F1 and EGFP dsRNA-R1 were used to amplify the EGFP fragment (547 bp) (126–672 bp) (table 1), and the dsRNA was synthesized by T7 RiboMAX™ Express RNAi System as above. The final dsRNA production corresponding to SlAKHR and EGFP genes were eluted into sterilized DEPC ddH2O, The quality and concentration of dsRNAs were determined by Nano-Drop Spectrophotometer (Implen, München, Germany) and their integrity were confirmed by a 1% agarose gel electrophoresis. Then they were stored at −80 °C and used up within 1 week.

For RNAi bioassays, newly 6th larvae were anesthetized on ice for 1 min before injection. dsRNAs were prepared the final concentrate 1 μg μl⁻¹. 5 μl dsRNA per larva was injected into the body cavity between the 3rd and 4th abdominal segment using a 10 μl micro-syringe syringe (Hamilton) and the injection point was sealed immediately with wax (Dong et al., Reference Dong, Zhong, Hu, Yi, Zhao and Wang2013). The injected larvae were then returned to the artificial diet under the conditions described above. The efficiency of SlAKHR gene knowdown was calculated using qRT-PCR at 12, 24, 36 and 48 h as described above. Larvae injected with EGFP dsRNA were used as controls.

Determination of triacylglycerol (TAG)

For TAG contents quantification, the TAG assay kit (Solarbio Biotech, Beijing, China) was used. Briefly, About 100 mg fat body was separated. After 1 ml n-heptane & isopropanol (1 : 1) was added, the mixture was homogenized in on ice for 5 min. Then the sample was centrifuged at 8000g for 10 min at 4°C. 40 μl supernatant was transferred to a new 200 μl eppendorf tube. After added 125 μl reagent I and 25 μl reagent II, vortex shock 30 s. Then 15 μl supernatant was transferred to another new 200 μl eppendorf tube, 50 μl reagent III, 15 μl reagent IV, 50 μl reagent V and 50 μl reagent VI was added inturn. After incubated 15 min at 65 °C, 250μl compound was transferred to a 96-well plate, and the OD value was measured at 420 nm on a HIDEX Sense 425-301 (Turku, Finland) on room temperature. The ultrapure water was used for blank controls.

Measurement of free fatty acid (FFA)

The contents of FFA measurement was guided by Li and Yuan (Reference Li and Yuan2013). Simplely, 300 μl hemolymph sample from the 6th instar larvae were collected with 15 ml centrifuge tubes respectively, Then 1 ml 1/30 M PBS buffer (pH = 8.0) and 6 ml chloroform were added. After shook for 30 s, 2 ml copper reagent (triethanolamine solution: acetum: 6.45% copper nitrate solution = 9:1:10) was added. Another shaking for 15 min, stayed 10 min at room temperature. After centrifuged for 5 min at 3000g, 4 ml subnatant was tansfered to a new 15 ml centrifuge tubes. Then 0.5 ml developer (100 mg sodium diethyl dithiocarbamate trihydrate dissolved in 100 ml n-butyl alcohol) was added. 5 min later, the OD value were measured at 440 nm on a spectrophotometer UV-5500 (PC) (Metash instrument, Shanghai, China). Ultrapure water was used for blank controls.

Lipid droplet staining and microscopy

The dissected fat bodies were fixed with 4% paraformaldehyde on a glass slide for 2 h at room temperature and then washed with chilled PBS (0.01 M, pH = 7.4) three times (5 min × 3). Then these fat bodies were submerged in Nile red solution (5 μl Nile red (1 mg ml⁻¹) in 495 μl PBS) for overnight at 4°C (Wang et al., Reference Wang, Hou, Saha, Pei, Raikhel and Zou2017). After washing for 5 min with PBS for three times, the fat bodies were re-stained in DAPI (2 ng μl⁻¹) for 10 min, next 5 min washing with PBS for three times (Zhao and Huang, Reference Zhao and Huang2019). The fat body were mounted on glass slides in 80% glycerol and visualized under a fluorescence microscope (Nikon, Japan) at 510–560 nm excitation wavelength combined with a 580 nm emission filter.

Statistical analysis

Results were presented as means ± SD (standard deviation) based on three independent biological replications. Differences between two groups were analyzed by Student's t-test (*P < 0.05; **P < 0.01). One-way ANOVA followed by a Fisher's protected LSD multiple comparison was used for the comparison among more than two different conditions. Statistical analyses were performed using SPSS 20.0 (Chicago, USA).