A total of 120 crossbred ([Yorkshire×Landrace]× Duroc) weaning pigs (28±3 d of age, 8.04±0.08 kg body weight [BW]) were assigned to one of five treatments considering sex and body weight in a randomized complete block design. Four pigs were reared in each pen of a weaning pigs’ house (concrete-slot floor, 0.90×2.15 m). The control treatment group was provided with corn-barley-soybean meal-based diet and the other groups were provided with diet containing 1.5%, 3.0%, 4.5%, or 6.0% of dried mealworm powder during 35 days after weaning. Feed and water were provided ad libitum through a feeder and a nipple during the whole experimental period. The temperature was kept at 30°C during the first 7 days and lowered 1°C every week. An experimental period consists of two phases (Phase I: from 0 day to 14 day, Phase II: from 14 day to 35 day), and body weight and feed intake were recorded at the end of each phase to calculate average daily gain (ADG), average daily feed intake (ADFI) and gain to feed ratio (G:F ratio). Corn-barley-soybean meal-based experimental diets were formulated to contain dried mealworm at levels of 0%, 1.5%, 3.0%, 4.5%, or 6.0%. Dried mealworm powder replaced soybean meal (SBM). and soy oil because of the high energy and protein content in dried tenebrio molitor larva powder (metabolizable energy 5,258 kcal/kg, crude protein [CP] 46.44%). All nutrients of experimental diets met or slightly exceeded the nutrient requirements as specified by NRC (2012). Mealworms were harvested until approximate 70 d of age and the air-dried Tenebrio molitor larvae were obtained from National Institute of Agricultural Sciences (Wanju, Korea). Dried mealworms were ground wholly by grinder for mealworm powder type before mixing the experimental feed. Dried mealworm (dry matter [DM] basis) contained approximately 5.84% of moisture, 43.27% of CP, 32.93% of crude fat, 4.86% of crude ash, respectively. Amino acid and fatty acid composition of dried mealworm are showed in Table 1. Formulas and chemical compositions of experimental diets are presented in Table 2 and 3.

A total of 20 crossbred pigs (10.05±0.98 kg BW) were assigned to individual metabolic crates and allotted to one of five treatments with 4 replicates in completely randomized design. Each pig was fed 200 g of phase II diet twice per day at 7:00 and 19:00, minimum level of feeding was 2% per body weight which was over 2 times the maintenance energy requirement (NRC, 1998). After 5 days adaptation period, a 5 day collection period was started with the addition of 1% chromium oxide in experimental diets as an initial marker. As a finishing marker, 1% ferric oxide was added in each experimental diet at 6th day of collection period. Collection of feces was started when the chromium oxide appeared in the feces and kept until the appearance of ferric oxide in the feces. Urine samples were collected during collection period in plastic containers containing 50 mL of 4 N H₂SO₄ to prevent evaporation of nitrogen prior to nitrogen retention analysis. Fecal and urinary samples were stored at −20°C until the end of collection period and the feces were dried in a drying oven at 60°C for 72 h and then ground to 1mm in a Wiley mill for chemical analysis including moisture, protein, fat, and ash contents by AOAC methods (1995).

In each treatment, 6 pigs with average body weight were bled through the anterior vena cava to analyze blood urea nitrogen (BUN), insulin-like growth factor (IGF-1) and immune response (IgA, IgG) at initial day and the ends of phases (phase I and phase II). Blood samples were collected in disposable culture tubes and centrifuged for 15 min by 3,000 rpm at 4°C (Eppendorf centrifuge 5810R, Hamburg, Germany). The serum was carefully transferred to 1.5 mL micro tubes and stored at −20°C until analysis. Total BUN concentration was analyzed using an analyzer (Ciba-Corning model, Express Plus, Ciba Corning diagnostics Co., Basel, Switzerland). The immunoglobulin G (IgG) and immunoglobulin A (IgA) concentration were analyzed by enzyme-linked immunosorbent assay (ELISA) assay by the manufacture’s protocols (ELISA Starter Accessory Package, Pig IgG ELISA Quantitation Kit, Pig IgA ELISA Quantitation Kit; Bethyl, Montgomery, TX, USA). The concentration of IGF-1 was analyzed by hormone analyzer (Immulite 2000, DPC, Malvern, PA, USA).

Diets and feces were ground by a Cyclotec 1093 Sample Mill (Foss Tecator, Hillerod, Denmark) and then analyzed. The contents of DM (procedure 967.03; AOAC, 1995), ash (procedure 923.03; AOAC, 1995). The nitrogen content was analyzed by using the Kjeldahl procedure with Kjeltec (KjeltecTM 2200, Foss Tecator, Höganäs, Sweden) and calculating the CP content (Nitrogen×6.25; procedure 981.10; AOAC, 1995).

Statistical analysis was carried out by least squares mean comparisons using PDIFF option of general linear model procedure (SAS, 2002; SAS Inst. Inc., Cary, NC, USA). Each pen was considered as experimental unit in measuring growth performance, while individual pig was used as experimental unit for analyzing nutrient digestibility, nitrogen retention and blood characteristics. Orthogonal polynomial contrasts were performed to determine linear and quadratic effects of inclusion levels of dried mealworm. Statistical differences were considered highly significant differ at p<0.01, significant differ at p<0.05, tendency between p≥0.05 and p≤0.10.