Experimental material and chemicals

Inulin (extracted from Jerusalem artichoke tubers) was purchased from the Qinghai Weide Biotechnology Co., Ltd.

The total sugar content was determined using the phenol–sulphuric acid method. The purity of inulin was determined by subtracting the reducing sugar content from the total sugar content (3-amino-5-nitrosalicylic acid method)^{(Reference Cuesta, Suarez and Bessio21,Reference Waes, Baert and Carlier22)} . The purity of inulin was 90·1 %.

Metformin HCl (1,1-dimethyl metformin HCl, C₁₄H₁₁N₅.HCl, molecular weight 165·63 g/mol) tablets were purchased from Sino-American Shanghai Squibb Pharmaceuticals Ltd. Metformin HCl is a biguanide antihyperglycaemic drug administered orally alone or in combination with other hypoglycaemics in treating type 2 diabetes mellitus^{(Reference Stepensky, Friedman and Raz23–Reference Nayaka and Pal26)}. STZ (C₈H₁₅N₃O₇, molecular weight 265·22 g/mol) was purchased from the Biosharp Co., Ltd).

Ethics statement of animal experiments

All of the procedures involving mice were carried out in accordance with the Guidelines for the Care and Use of Laboratory Animals prepared by the Institutional Animal Care and Use Committee of Nanjing Agricultural University, Nanjing, China (SYXK(SU)2017-0007). The experimentation was performed in the laboratory animal centre of Nanjing Agricultural University. The method of euthanasia was cervical dislocation.

Experimental animals and diets

The feeding method of Yu et al. ^{(Reference Yu, Zhao and Xu27)} was followed. Sixty male 6-week-old C57BL/6J mice were provided by the Yangzhou University Medical Center; each weighed about 20 g (the experimental animal production license: SCXK (Su) 201605253). All animals had free access to drinking water and were fed a standard diet for 7 d and then followed by feeding them with the standard (control) diet or HFD MD1203 (45 % energy from fat) purchased from Medicience Ltd. (Yangzhou, China). The high-fat with a high-sucrose diet is an effective method to induce insulin resistance. The detailed composition of the diet is shown in Table 1. Mice were housed in plastic cages (five per cage) under standard conditions (20–26°C, 40–70 % relative humidity, 12 h light–12 h dark cycle). The standard (control) diet was provided by the Animal Experimental Center of Nanjing Agricultural University, and its formula is formulated according to the ‘Experimental Animal Compound Feed Nutritional Component (GB14924.3-2010)’ in the National Standard for Experimental Animal Environment and Facilities (GB14925-2010). The comparison of nutrients between the standard (control) diet and HFD is shown in online Supplementary Table S1.

Table 1. Composition of the high-fat diet

Development of high-fat-diet-fed and streptozotocin-treated type 2 diabetic mice

In order to investigate the alleviation effect of inulin on the type 2 diabetes, mice were fed the HFD and treated with STZ (Table 2). According to a power calculation to determine sample size, the sixty C57BL/6J mice were randomly divided into two groups: the normal control group (n 10) and the experimental group (n 50); the normal control group was fed the standard (control) diet, and the experimental group was fed the HFD for 4 weeks. Then the experimental group was injected intraperitoneally with low-dose STZ (50 mg/kg, in citrate buffer, pH 4·4) for 1 week, whereas the control group mice were given just the same volume of citrate buffer preparation. After another 2 weeks of feeding, all the mice were fasted for 12 h, and the FBG test was carried out by ACCU-CHEK Active (Roche Diagnostics GmbH). FBG ≥ 11·1 mmol/l is the diagnostic criterion for diabetes. All mice had unlimited access to drinking water.

Table 2. Construction of experimental mouse model*

STZ, streptozotocin.

* All mice had unlimited access to drinking water.

Experimental design

The experimental setup consisted of six different groups. Type 2 diabetic mice were randomly divided into five groups (ten mice per group) and treated daily with intra-gastric administration (0·2 ml/10 g) of each test compound (as described in the previous section) for 4 weeks. The solvent was made with distilled water. Then we fed group CK mice (blank control, standard diet + 5 g/kg physiological saline per d) and group H mice (experimental control group with induced diabetes, standard diet + 5 g/kg physiological saline per d) the standard diet, and they received intra-gastric administration of 5 g/kg physiological saline (0·9 % NaCl w/v) per d for 4 weeks. Group CP mice (positive control group, standard diet + metformin HCl tablets 125 mg/kg per d) were fed the standard diet and treated with 125 mg/kg per d metformin HCl tablets. Mice in groups LJ (standard diet + inulin 2·5 g/kg per d), MJ (standard diet + inulin 5 g/kg per d) and HJ (standard diet + inulin 10 g/kg per d) were fed the standard diet and treated with, respectively, 2·5, 5 and 10 g inulin/kg per d (the inulin irrigation amounts were, respectively, 5, 10 and 20 times the recommended daily intake for people)⁽²⁸⁾.

Determination of weekly body weight and relative liver weight

The Yu’s^{(Reference Yu, Zhao and Xu27)} feeding method was followed. Body weight of each mouse was measured weekly. At the end of the experiment, the relative liver weight per 100 g of total weight of each mouse was calculated:

$${\rm{Relative}}\;{\rm{liver}}\;{\rm{weight}}\quad {\rm{ =}}\frac{{{\rm{weight}}\;{\rm{of}}\;{\rm{mice}}\;{\rm{liver}}\;({\rm{g}})}}{{{\rm{body}}\;{\rm{weight}}\;{\rm{on}}\;{\rm{the}}\;{\rm{final}}\;{\rm{experimental}}\;{\rm{day}}\;({\rm{g}})}} \times {\rm{100}}$$

Blood collection and biochemical assays

At the end of the 4-week treatment, all the mice were fasted for 12 h and the FBG test was carried out by ACCU-CHEK Active. The blood samples were collected from the orbital sinus of mice using a 2-ml heparinised syringe and placed on ice for transfer and then centrifuged at 3500 g at 4°C for 15 min to separate the plasma. The concentrations of total cholesterol, TAG, HDL-cholesterol and LDL-cholesterol in plasma were measured using a Roche MODULAR automatic biochemical analyser at the Integrated Traditional Chinese and Western Medicine Hospital of Nanjing University of Chinese Medicine (Nanjing, China).

Liver collection, total RNA extraction, reverse transcription and real-time PCR

The liver was taken out, fat cleaned and the liver flushed by physiological saline to remove the surface blood at 4°C. The related gene expression of liver was performed at Shanghai Wcgene Biotech Co. Ltd.

Briefly, to isolate the total RNA, approximately 30 mg of the main lobe from each liver was placed into RNAiso Plus (Takara Co. Ltd), according to the manufacturer’s instructions and then resuspended in diethyl pyrocarbonate-treated water. The quality of RNA was assessed by electrophoresis in 1·0 % (w/v) formaldehyde denaturing agarose gel. Real-time PCR was used to determine mRNA levels based on the Roche FS Universal SYBR Master: 04913914001 instructions in an ABI ViiA7 Real-Time PCR System. A 20-μl reaction system contained 5 μl Roche FS Universal SYBR Master (ROX), 3 μl ddH₂O, 0·75 μl Primer F, 0·75 μl Primer R, 0·5 μl DNA sample and 10 μl total volume. The cycling parameters were as follows: 10 min at 95°C followed by one cycle, 30 s at 95°C followed by forty cycles, 30 s at 60°C followed by forty cycles and 10 min at 72°C followed by one cycle.

DNA extraction and intestinal micro-organism communities

Three replicate mice were randomly selected from each experimental group. Total bacterial DNA from 0·25 g of colon segment of the large intestine was extracted using a PowerFecal^TM DNA Isolation kit (MO BIO Laboratories Inc), according to the manufacturer’s instructions and was stored at −80°C for further analysis^{(Reference Rodrigues, Pellizari and Mueller29)}. Amplicon pyrosequencing was performed on an Illumina MiSeq platform at Allwegene Technology Inc.

Briefly, DNA was amplified using the 338F/806R primer set (338F: 5′-ACTCCTACGGGAGGCAGCAG-3′, 806R: 5′-GGACTACHVGGGTWTCTAAT-3′) that targets the regions (V3–V4) of the 16S rRNA gene because sequences in those regions provided the greatest diversity at the domain and phylum levels. The PCR was performed in 25-μl volume containing 30 ng of DNA template. The cycling parameters were as follows: 5 min of denaturation at 95°C followed by twenty-five cycles of 30 s at 95°C, 30 s for annealing at 56°C and 40 s at 72°C (elongation), with a final extension at 72°C for 10 min. PCR products were processed with an AxyPrep™ Mag PCR Normaliser kit (Axygen, Inc.) for normalisation.

Quantitative Insights Into Microbial Ecology (https://qiime.org/tutorials/processing_illumina_data.html) quality filters were used to filter the reads^{(Reference Schloss, Gevers and Westcott30)}. We used the Cluster Database at High Identity with Tolerance (CD-HIT) pipeline for picking operational taxonomic units (OTU) and making OTU table. The sequences with similarity of 97 % were assigned to OTU. A representative sequence was selected for each OTU, and the classification data were assigned to each of the representative sequences using the Ribosome Database Project (RDP) classifier^{(Reference Caporaso, Gordon and Walters31)}.

To estimate α diversity, the OTU table was rarefied, and four indicators were calculated: Chao 1 estimating richness, the observed OTU as the only OTU counting sample, and Shannon index estimating diversity^{(Reference Kuffner, Hai and Rattei32,Reference Vishnivetskaya, Mosher and Palumbo33)} . Each sample was classified and statistically analysed using RDP, Greengene and Silva three database comparison^{(Reference Cole, Wang and Cardenas34–Reference Quast, Pruesse and Yilmaz36)}. The sequences obtained were distributed in eight bacterial phyla by RDP (V14 https://rdp.cme.msu.edu/).

Linear discriminant analysis (LDA) and effect size measurement (LEfSe) are common methods for the discovery of macrogenomic biomarkers. We performed LEfSe calculations for the non-parametric Wilcoxon sum-rank test followed by LDA using online software (https://huttenhower.sph.harvard.edu/galaxy/) to assess the effect size of each taxon with differential abundance^{(Reference Segata, Izard and Waldron37)}.

The complete datasets were deposited in the National Center for Biotechnology Information. The Sequence Read Archive accession number is SRP108873.

Statistical analysis

Data were analysed by one-way ANOVA using SPSS 19.0 (SPSS Inc.). All data were tested for homogeneity of variance by Levene’s test. Tukey’s test was then used to compare the differences among the treatments. The level of significance was set at P ≤ 0·05. All data were expressed as means with their standard errors.