Bifidobacterium infantisstrains with and without a combination of Oligofructose and Inulin (OFI) attenuate inflammation in DSS-induced colitis in rats

Sprague-Dawley rats (200 g) (Möllegård, Viby, Denmark) were used and divided into six groups (6 animals each), colitis control and five treatment groups. One group was treated with a commercially available preparation of oligofructose and inulin (OFI) (Raftilose Synergy 1, Orafti Active Food ingredients, Tienen, Belgium). This contains inulin with selected chain lengths from chicory that has been enriched by a specific fraction of oligofructose produced by partial enzymatic hydrolysis of chicory inulin. Four groups were treated with Bifidobacterium infantis (B. infantis DSM 15158 [= CURE19] or B. infantis DSM 15159 [= CURE21], Probi AB, Lund, Sweden) alone or together with OFI. The two B. infantis strains have been isolated from infant feces, and have been selected for their colonization capabilities and abilities to produce amino acids from inorganic nitrogen. The animals were kept at room temperature (22°C) with a controlled 12 hr light/dark cycle and free access to a standard rat chow (R3; Lactamin, Stockholm). The experimental solutions were administered orally by oro-gastric tube twice daily for 7 days before starting DSS and continued for 7 days after DSS induction (probiotics 3 ml; 3 × 10⁶ CFU per animal, prebiotics 3 ml; 0.5 g per animal, synbiotics 3 ml; 3 × 10⁶ CFU + 0.5 g per animal). Normal saline (3 ml) was administered in the colitis control group. Colitis was induced by 5% (w/v) DSS (MW = 36,000–50,000; ICN Biomedicals Inc., Aurora, OH) dissolved in drinking water for 7 days. Severity of colitis was assessed daily using a disease activity index (DAI). After the seventh day of induction of colitis, animals were anesthetized with a subcutaneous injection of a mixture (1:1:2) of Hypnorm (Division of Janssen-Cilag Ltd., Janssen Pharmaceutica, Beerse, Belgium) + Dormicum (F. Hoffmann-La Roche AG, Basel, Switzerland) + dH₂O at a dose of 0.15 ml/100 g. Under aseptic technique a laparotomy was performed through a midline incision and samples were collected for bacterial microflora (cecum), bacterial translocation (arterial and portal blood, mesenteric lymph nodes, and liver), SCFAs (cecal contents), Myeloperoxidase (MPO), cytokines (IL-1β, TNF-α, IL-10 and TGF-β) and Malondialdehyde (MDA) (colon tissues). Bacterial microflora samples were placed immediately in sterile tubes containing, 3 ml of transport medium, whereas bacterial translocation samples were placed in sterile tubes containing, 2 ml for blood, and, 6 m1 for segments [12]. Samples for cytokines, MPO, MDA, and SCFAs were immediately frozen at -70°C. The experimental design was approved by the Animal Ethics Committee of Lund University and the experiments adhered to the guiding principles in the care and use of animals.

The severity of colitis was assessed daily using a Disease Activity Index (DAI) based on the scoring system of Murthy et al. [13, 14], which scores body weight loss, stool consistency, and rectal bleeding. Occult blood in feces was evaluated by means of test slides, Hemoccult II (SmithKline Diagnostic, USA). The DAI clinical parameters used here are comprehensive functional measures that are somewhat analogous to clinical symptoms observed in human IBD and the scoring method has been validated by repeated studies [15].

The samples from the cecum were placed in an ultrasonic bath and swirled on Chiltern as above. A conventional dilution procedure was done. Viable counts were obtained from BHI agar that was incubated aerobically and anaerobically at 37°C for 72 h (aerobic and anaerobic bacterial count, respectively), Rogosa agar (Oxoid) that was incubated anaerobically at 37°C for 72 h (lactobacilli count), from VRBG agar (Oxoid) that was incubated aerobically at 37°C for 24 h (Enterobacteriaceae count), and from the selective media, Modified Wilkins-Chalgren agar (MW; Oxoid), Modified Trypticase phytone-yeast extract agar (MTPY; ACSA, Spain) [16] and non-strictly selective Basic nutrient-poor media [17], which was modified according to the following composition per liter, (sodium acetate 10 g: ascorbic acid 10 g: (NH₄)₂SO₄ 5 g: K₂HPO₄ 3 g: (KH)₂PO₄ 3 g: tween 80 1 ml: yeast extract 0.5 g: glucose 20 g: agar 15 g and 5 ml of the mineral salt solution which composed per 250 ml of(MgSO₄·7H₂O 16 g: FeSO₄·7H₂O 0.5 g: MnSO₄·H₂O 0.35 g: NaCl 0.5 g) pH 6.18–6.24. They were incubated under anaerobic conditions at 37°C for 72 h (bifidobacteria count).

Samples of colon were weighed and homogenized for 1 min in phosphate buffer. The homogenates were centrifuged at 10 000 g at 4°C for 5 min. TNF-α, IL-1β, IL-10 and TGF-β concentration in the supernatants were determined by ELISA using the commercially available Quantikine kit (R&D Systems, Minneapolis, MN 55413, USA). Optical densities were measured on an ELISA reader at a wavelength of 450 nm. Data were analyzed against the linear portion of the generated standard curve.

Colonic tissues were collected, weighed prior to storage at -70°C until time of assay for MPO activity. The colonic segments were homogenized in 1 ml potassium phosphate buffer (20 mM, pH 7.4) for 60 sec. Subsequently, the homogenate was centrifuged (14000 rpm, 10 min) and the pellet was resuspended in 1 ml potassium phosphate buffer (50 mM, pH 6.0) containing 0.5% hexadecyl-trimethyl-ammonium bromide. The sample was then freeze thawed once, sonicated (90 sec) and kept in water bath for 120 min (60°C). Next, the sample was centrifuged (14000 rpm, 10 min) and the MPO activity of the supernatant (20 μl) assessed in 96-well plates (Nunc, Invitrogen A/S, Taastrup, Denmark). The enzyme activity was determined spectrophotometrically at 450 nm. MPO (Sigma Chemical Co., St. Louis, MO, USA) was used as standard and values are expressed as MPO units g^-1 tissue.

Malondialdehyde (MDA) were determined as index of lipid peroxidation, using MDA 586™ (R&D, Europe Ltd, Abingdon, Oxon, UK). Colonic segments were collected, rinsed in ice cold Dulbecco's PBS, weighed and then frozen immediately at -70°C for later evaluation. Lipid peroxidation was estimated by adding 1 ml Dulbecco's PBS with 5 mM butylated-hydroxyltoluene to the samples and then homogenized. After homogenization the samples were centrifuged at 4000 × g for 10 minutes (min) at 4°C. An aliquot (200 μl) of the standard and/or the supernatant was added to a reaction mixture containing 640 μl of N-methyl-2-phelindole, 10 μl probucol and 150 μl of 12 M hydrochloric acid. The samples were then incubated in a water bath for 60 min at 45°C and centrifuged at 10000 × g for 10 min at 4°C. The absorbance of the standard and supernatant was measured by Spectrophotometry at 586 nm. The results were expressed as nmol MDA/g tissue.

SCFAs and organic acids (lactic, and succinic, acid) were measured by a modification of the capillary GC method by Richardson et al. [18] as described by Jensen et al. [19]. Sample preparation was done by diluting 10 times the cecal content samples with a working solution containing water and internal standard (IS) (100 mmol/l 2-Ethylbutyric acid). The diluted sample was homogenized and a 1 ml sub-sample was taken for extraction. This sample was extracted by adding 0.1 ml H₂O, 500 μl hydrochloric acid (HCl) and 2000 μl ether followed by mixing for 30 seconds on a Vibrax at 1400 rpm, and centrifugation for 10 min at 3000 g. For every 8 samples, 2 standard mixtures were prepared by adding 0.1 ml H₂O, 0.5 ml HCl, 100 μl working solution and 2000 μl ether to a 1 ml standard mixture. To the GC microvial was added 50 μl sample and/or standard from the ether-phase together with 10 μl N-tert-butyldimethylsilyl-N-trifluoroacetamid, to derivatize the samples and get volatile and thermal constant derivatives that are suitable for GC run. The vial with Crimp-Caps were closed and mixed once and placed on the 80°C heating block for 20 minutes. To complete the derivatisation, the samples were allowed to stand 48 hours before injection. The analysis was performed using a gas chromatograph provided with capillary column (DB-5, J&W Scientific, USA). The following temperature-program were used (70°C (3 min), 70–110°C (10°C/min), 110–270°C (20°C/min). Detector and injector temperature were 275 and 300°C, respectively, and the carrier gas was helium (1.9 ml/min). 2 μl sample volume was injected.

There was no mortality among the experimental groups. DAI decreased significantly on day 4 & 5 (data not shown) and day 6 & 7 in all groups compared to colitis control group (Figure 1).

Bacterial translocation to the liver decreased significantly in all the groups compared to colitis control and OFI + B. infantis DSM 15158 groups (Table 1). Bacterial translocation to the mesenteric lymph nods decreased significantly in all the groups compared to colitis control (Table 1).

The bifidobacterial counts in cecum (using 2 selective media) increased significantly in the OFI groups with and without added B. infants compared to colitis control (8.74 ± 0.07, 8.89 ± 0.16, 8.32 ± 0.50 versus 6.82 ± 0.37 for the modified Wilkins-Chalgren agar) and (8.73 ± 0.07, 8.60 ± 0.19, 8.23 ± 0.48 versus 6.57 ± 0.37 for the modified Trypticase phytone-yeast extract agar). For the not strictly selective media it increased significantly in all groups compared to colitis control (Data not shown). There were no differences in the cecum Enterobacteriaceae count. The cecal count of lactobacilli increased significantly in B. infantis DSM 15159 groups with and without OFI (8.85 ± 0.24 and 9.56 ± 0.05 respectively) compared to colitis control (7.82 ± 0.47).

Colonic myeloperoxidase activity decreased significantly in all groups compared to the colitis control group (Figure 2).

Colonic tissue IL-1β decreased significantly in all treated groups except B. infantis DSM 15158 (Figure 3), while levels of TGF-β and IL-10 were maintained in all groups without significant difference (data not shown). There was no detection of TNF-α in any of the groups.

MDA decreased significantly in the B. infantis DSM 15159 groups with and without OFI compared to colitis control (Figure 4).

Succinic acid increased significantly in the OFI groups with and without DSM 15159 compared to the control and other groups (Table 2). Sum values of propionic and butyric acid increased significantly in all treated groups [5.9 (3.9–7.3), 6.1(4.1–8.6), 4.7(3.3–6.5), 5.7(4.5–6.4), 6.4(4.6–10.1)] compare to the colitis control group [3.2(2.3–3.8)]. Sum values of succinic, propionic and butyric acids also increased significantly in all treated groups [5.4 (3.6–7.0), 4.1(0.0–6.6), 3.3(1.6–5.2), 4.9(3.0–5.8), 6.0(4.0–10.0)] compare to the colitis control group [2.6(0.0–3.3)], but the OFI + B. infantis DSM 15159 was significantly higher [6.0(4.0–10.0)] than in all other groups.