Animal treatments

This study was conducted in accordance with the principles and guidelines for international animal care and approved by the Animal Experimental Committee of the University of Tsukuba (approval number 21-1007).

Thirty 5-week-old female Sprague-Dawley (sd) rats (Japan CLEA Co., Ltd.) were used in this experiment. After acclimatisation to the environment for 1 week, the animals were divided into four groups: no exercise and ad libitum food intake (Con, n 7), exercise and ad libitum food intake (Ex, n 7), no exercise and 50–60 % food restriction (FR, n 8) and exercise and 50–60 % food restriction group (FAT, n 8). The minimum sample size was estimated and determined from our unpublished data. The experimental period was 4 weeks. During the study period, the FR and FAT groups were fed 50 % of the food intake of the Ex group for the first week. However, because of the rapid weight loss observed during the first week (approximately 20 % weight loss in the FAT group), the FR and FAT groups were fed 60 % of the food intake of the Ex group from the second week. Since FAT is primarily attributed to reduced available energy, this study limited only energy sources, not vitamins and minerals. The composition of the diet is listed in Table 1. During the experiment, the rats had free access to the rotating wheel and exercised spontaneously. The rats were kept in a stainless-steel wire case (13 × 13 × 22 cm) for the Con and FR groups and in a cage with a rotary wheel (1 m per lap, cage size: 35 cm high–27 cm wide–35 cm deep) for the Ex and FAT groups to perform the exercise. The room temperature and humidity were maintained at 25 ± 1°C and 80 ± 10 % under a constant 12:12 h light–dark cycle (light 6:00–18:00).

Table 1.

Composition of daily diet of rats used in the study

* Casein contained 45 mg Ca/100 g and 127 mg P/100 g.

† Components of the water-soluble vitamin mixture (%): thiamine, 0·5; riboflavin, 0·5; pyridoxine, 0·5; calcium pantothenate, 2·8; nicotinamide, 2·0; inositol, 20·0; folic acid, 0·02; vitamin B₁₂, 0·002; biotin, 0·01 and glucose monohydrate, 73·7.

‡ The rats received a supplement of the following oil-soluble vitamins in cottonseed oil/week: β-carotene, 70 µg; 2-methyl-1·4-naphthoquinone, 105 µg; α-tocopherol, 875 µg and vitamin D₃, 525 mg.

§ Ca- and P-free salt mixture (%): KCl, 57·7; NaCl, 20·9; MgSO₄, 17·9; FeSO₄ · 7H₂O, 3·22; CuSO₄ · 5H₂O, 0·078; NaF, 0·133; CoCl₂ · 6H₂O, 0·004; KI, 0·01; MnSO₄ · 5H₂O, 0·06; ZnSO₄ · 7H₂O, 0·44; and (NH₄)₆Mo₇O₂₄ · 4H₂O, 0·005.

Daily data and sample collection

The body weight, food intake and running distance were recorded daily. The rats were made to fast for 2 h prior to autopsy and isoflurane (Mylan Inc.) was inhaled. After confirming the disappearance of the rise reflex, whole blood was quickly drawn from the abdominal aorta and the rats were killed. The blood was kept on ice for 30 min and then centrifuged (2500 rpm, 4°C, 15 min) to obtain serum. After killing, the femur and lumbar spine were collected, and the lumbar spines were preserved in 70 % ethanol. The femurs were collected, and the wet weight was measured. The jejunum was collected as previously described^{(Reference Aoki, Yanazawa and Tokinoya12)}. Briefly, the small intestine was cut in half and the duodenum side was used as the jejunum. The central parts of the jejunum (approximately 1 cm) were used for haematoxylin and eosin staining. The remaining sample was cut open longitudinally, the muscle layer was removed and the mucosa was collected. Femurs were stored at 4°C until biomechanical testing.

Measurement of bone strength

The fracture force and fracture energy were measured using a bone fracture characteristic-measuring device (DYN-1255, Iio Electric Co.) using the femurs. The conditions were as follows: distance between fulcrums, 1 cm; plunger speed, 100 m/min; full scale, 50 kg and chart speed, 120 cm/min.

Measurement of bone mineral content and bone mineral density

Bone mineral content and BMD of the L3–L6 lumbar spine were measured using dual-energy X-ray absorptiometry (DXA; QDR-4500A, Hologic Inc.). All scans were performed using small animal mode and high regional resolution.

Haematoxylin and eosin staining and measurements

Jejunum samples were stained with haematoxylin and eosin according to protocols from previous studies^{(Reference Aoki, Yanazawa and Tokinoya12,Reference Aoki, Suzuki and Hui16)} . Mucosal thickness, villus height, crypt depth and villus width were measured in at least five villi/rat as previously described^{(Reference Todorov, Kollar and Bayer17)}. Briefly, crypt depth was measured from the lowest layer of the mucosa excluding the muscular layer to the sub-basal portion of the villus, and villus height was measured from the sub-basal to apical portion of the villus, and the sum of these two was used as the mucosa thickness. Villus width was measured at the thickest part of the villus.

All images were captured using a microscope (BZ-X710; Keyence).

Immunoblotting

All immunoblotting procedures were performed according to a previous study^{(Reference Aoki, Yanazawa and Tokinoya12)}. Briefly, total protein was extracted from jejunal mucosa samples using a lysis buffer (1 % NP-40, 50 mM Tris, 150 mM NaCl, 1 mM EDTA including proteinase inhibitor tablets (cOmpleteTM mini, Roche)). Protein concentration was measured using a Takara BCA Assay kit (T9300A, Takara Bio) and microplate reader (Varioskan LUX, Thermo Fisher Scientific). Finally, the protein samples were adjusted to a concentration of 1 μg/μl. The total protein (15 μg/lane) was used for gel electrophoresis. For western blotting, primary antibodies against liver-type fatty acid-binding protein (1:1000, sc-374537, Santa Cruz Biotechnology), intestinal-type fatty acid-binding protein (1:1000, sc-374482, Santa Cruz Biotechnology), APOA1 (1:500, sc-58230, Santa Cruz Biotechnology), alanyl aminopeptidase (1:1000, sc-13536, Santa Cruz Biotechnology), SLC15A1 (1:1000, sc-373742, Santa Cruz Biotechnology), SGLT1 (1:1000, A11976, ABclonal Technology), GLUT2 (1:1000, 20436-1-AP, Proteintech Group Inc.) and sucrase-isomaltase (1:1000, sc-393470, Santa Cruz Biotechnology) were used. Horseradish peroxidase-conjugated anti-rabbit IgG (Cell Signaling Technology, #7074) and anti-mouse IgG (Cell Signaling Technology, #7076) were used as secondary antibodies. Signals were detected using chemiluminescence reagent (EzWestLumi One or EzWestLumi plus, ATTO). Blots were scanned using a chemiluminescence imaging system (FUSION FX7.EDGE; Vilber Lourmat).

Quantitative PCR

All quantitative PCR (qPCR) procedures were performed as previously described^{(Reference Aoki, Yanazawa and Tokinoya12)}. Briefly, total RNA was extracted from the jejunal mucosa using Sepasol ®-RNA I Super G (Nacalai Tesque). Concentration and quality of RNA were measured using a spectrophotometer (NanoDrop OneC, Thermo Fisher Scientific). RNA quality was assessed with the 260/280 nm and 260/230 nm absorbance ratios (>1·8). Total RNA samples were adjusted to 400 ng/tube, and reverse transcription was performed using 5 × PrimeScript RT Master Mix (RR 036 A, Takara Bio) in a thermal cycler (TP 350, Takara Bio). After reverse transcription, TB Green ® Premix Ex Taq ™ II (Takara Bio) was used to perform qPCR using QuantStudio® 5 (Thermo Fisher Scientific). qPCR was performed with the following conditions: Hold stage: 95°C for 20 s, PCR stage: 95°C for 1 s, 60°C for 20 s, 40 cycles and Melt curve stage: 95°C for 1 s, 60°C for 20 s, 95°C for 1 s. The 28S ribosomal RNA was used as the housekeeping gene. The primer sequences were adopted from a previous study^{(Reference Aoki, Suzuki and Hui16)}. The primer sequences for the 28S ribosomal RNA were as follows: forward 5′-CCCAGAAAAGGTGTTGGTTGA-3′ and reverse 5′-TGATTCGGCAGGTGAGTTGTT-3′. The primer sequences for sucrase-isomaltase (Si) were as follows: Forward 5′-GCAGAAGGCTACATGGA-3′ and Reverse 5′--3′ and Reverse 5′-CCTTGCGACTGTCTCA-3′. The quantification cycle (Cq) value of the target gene was normalised to that of the housekeeping gene. The results were analysed using the 2^−ΔΔCt method adapted from Livak and Schmittgen^{(Reference Livak and Schmittgen18)} and expressed relative to the levels in the Con group.

Sucrase activity assay

Sucrase activity assay was conducted as previously described^{(Reference Suzuki, Mayanagi and Keta19,Reference Dahlqvist20)} . Each jejunal mucosa sample was homogenised in buffer containing 10 mM KH₂PO₄ and 10 mM K₂HPO₄ (pH 7·0). Mixtures of the homogenate and sucrose were incubated at 37°C for 20 min. After incubation, the reaction temperature was increased to 100°C for 2 min to inactivate the sucrase. To detect the hydrolysed glucose from sucrose, Tris-HCl-glucose oxidase reagent (3:7 ratio of 0·5 M Tris-HCl, pH 7·0 to Glu CII test Wako was added to each well and subsequently incubated at 37°C for 30 min. Then, 200 µl of the reaction solution was transferred to a new plate, and the absorbance was measured at 505 nm. The total protein concentration of each homogenate was determined using a bicinchoninic acid (BCA) protein assay kit (Takara Bio). One unit of sucrase activity corresponds to 1 mmol of glucose produced/min. It was also standardised by protein concentration of the homogenate.

Chromatin immunoprecipitation quantitative PCR

Chromatin immunoprecipitation (ChIP) qPCR was performed as previously described with minor modifications^{(Reference Inoue, Honma and Mochizuki21,Reference Inoue, Mochizuki and Goda22)} . The mucosa removed from the jejunum was fixed in formaldehyde solution (1 % formaldehyde, 4·5 mM HEPES (pH 8·0), 9 mM NaCl, 0·09 mM EDTA, 0·04 mM ethylene glycol tetraacetic acid) in PBS for 30 min at 37°C. The reaction was terminated with 2 M glycine (final concentration, 150 mM). After washing in fluorescence-activated cell sorter solution (1 × PBS(-), 2 % bovine serum, 0·05 % NaN3), the samples were sonicated in sodium dodecyl sulfate lysis buffer (50 mM Tris-hydrochloride (pH 8·0), 10 mM EDTA (pH 8·0), 1 % sodium dodecyl sulfate) and ChIP dilution buffer (50 mM Tris–HCl (pH 8·0), 167 mM NaCl, 1·1 % Triton X-100, 0·11 % sodium deoxycholate) (ratio 1:4) with a protease inhibitor cocktail (Wako) to obtain 200- to 500-bp DNA fragments. The ChIP assay was performed using the following antibodies: anti-trimethyl-histone H3K4 (1:160, A2357, ABclonal) or 1 mg of control rabbit (Ig)G. The precipitated DNA was analysed by real-time PCR. ChIP results were expressed as a percentage of the PCR signal for input DNA using the delta–delta method^{(Reference Livak and Schmittgen18)}, The Cq value was calculated by raising 2 to the power of Cq_{immunoprecipitated (IP) DNA}-Cq_{input DNA} (100 × [2^{(Cq of Input-Cq of IP sample})]). PCR equipment and conditions used were the same as in the qPCR section. Optimised PCR primer sequences and gene regions were obtained as previously described^{(Reference Inoue, Mochizuki and Goda22)}.

Statistical analysis

Data are shown as mean ± sem. Two-way ANOVA was conducted. If interaction was observed, followed by Tukey’s post hoc test was used to compare each group (independent variables: exercise (Ex) and food restriction (FR)). In qPCR, data were not normally distributed; therefore, the Kruskal–Wallis H test, followed by a two-stage Benjamini, Krieger and Yekutieli false discovery rate procedure as a post hoc test, was used. An unpaired t-test was used for comparison between the two groups. Statistical significance was set at P < 0·05 and significance tendency was set at P < 0·1. Statistical analyses were performed using the GraphPad Prism 8.4.3 software for Mac.