Orally ingested bovine lactoferrin (bLF) has been shown to provide a wide range of benefits in various animal models with inflamed and damaged tissues, such as the large intestine( Reference Togawa, Nagase and Tanaka 1 ), liver( Reference Tsubota, Yoshikawa and Nariai 2 ), oesophagus and lung( Reference Ushida, Sekine and Kuhara 3 , Reference Kuhara, Iigo and Itoh 4 ), oocytes( Reference Horiuchi, Higuchi and Tatsumi 5 ) and bone( Reference Guo, Jiang and Ibrahim 6 ). Clinical use of bLF has also produced several promising outcomes, such as the suppression of colorectal adenomas( Reference Kozu, Iinuma and Ohashi 7 ), the inhibition of hepatic inflammation in chronic hepatitis C patients( Reference Tanaka, Ikeda and Nozaki 8 ) and the prevention of sepsis in very low-birth-weight neonates( Reference Manzoni, Rinaldi and Cattani 9 ). Lactoferrin has physical and chemical properties that protect against oxidative damage( Reference Ye, Wang and Liu 10 ) and suppress inflammatory cytokine production by interfering with the NF-κB signalling pathway( Reference Inubushi, Kawazoe and Miyauchi 11 ). Furthermore, lactoferrin specifically binds to the hepatitis C virus (HCV), preventing HCV infection( Reference Nozaki, Ikeda and Naganuma 12 ). However, it has been reported that the pathway and mode of administration of bLF and its manufacturing process influence the physiological functions of bLF( Reference Sferi, Dubany and Boyaka 13 ). Despite all clinical uses of bLF being oral, most primary studies on the anti-inflammatory effect of bLF have been conducted using other routes of administration( Reference Yin, Cheng and Holt 14 ). In the present study, we first ascertained the anti-inflammatory activity of orally administered bLF using several mouse models of hepatitis. The underlying mechanisms in hepatitis induced by d-galactosamine (GalN), carbon tetrachloride (CCl4) and lipopolysaccharide (LPS) plus zymosan involve the cessation of macromolecular biosynthesis in hepatocytes( Reference Lehmann, Freudenberg and Galanos 15 ), the accumulation of lipid peroxidation and intracellular Ca ions by trichloromethyl radicals( Reference Nakatsuka, Taniguchi and Hirata 16 ) and the production of pro-inflammatory cytokines from activated Kupffer cells( Reference Yamaguchi, Matsuura and Kobayashi 17 ), respectively. We hypothesised that these various mouse models would be useful to determine the most effective properties and mechanisms of orally administered bLF in hepatitis.
Given that only barely detectable amounts of bLF and its large fragments are absorbed by the intestines( Reference Kuwata, Yamauchi and Teraguchi 18 ), it has been assumed that orally ingested bLF cannot exert a biological response through the direct interaction with target organs, but probably affects digestive tract functions. Previously, we demonstrated that orally ingested bLF enhances IL-18 production in the intestinal epithelium and type I interferon production in Peyer's patches, enhancing peripheral natural killer (NK) cell activity in mice( Reference Kuhara, Yamauchi and Tamura 19 ) and inhibiting tumour metastasis( Reference Kuhara, Iigo and Itoh 4 ). Our previous study demonstrating the immunomodulatory activity of orally ingested bLF was conducted under inflamed conditions( Reference Kuhara, Yamauchi and Tamura 19 ), because only minor changes in physiological function can be observed under normal conditions due to oral bLF administration. In rats with colitis induced by 2,4,6-trinitrobenzene sulfonic acid, oral bLF administration has been shown to reduce inflammation by correcting the cytokine imbalance( Reference Togawa, Nagase and Tanaka 1 ); however, inflammation of the intestine made it difficult to analyse the activity of bLF in the intestine. Therefore, in the present study, we analysed the mechanism underlying the anti-inflammatory activity of bLF using a mouse model of hepatitis induced by intravenous (i.v.) injection of zymosan plus LPS to minimise the direct effects of the agent on the intestine( Reference Yamaguchi, Matsuura and Kobayashi 17 ).
Previously, we demonstrated that bLF passes through the epithelium and directly stimulates IL-11 production in human myofibroblasts, and that IL-11 produced by myofibroblasts exerts protective activity towards epithelial cells( Reference Kuhara, Yamauchi and Iwatsuki 20 ). IL-11, a pleiotropic cytokine, has a variety of haematopoietic and non-haematopoietic activities( Reference Du and Williams 21 ). The i.v. injection of recombinant human IL-11 prevents CCl4-induced hepatotoxicity( Reference Kawakami, Takahashi and Shimizu 22 ). IL-11 suppresses the production of inflammatory mediators such as TNF-α, IL-1β and NO in activated macrophages via the inhibition of NF-κB( Reference Trepicchio, Wang and Bozza 23 ). Using the zymosan plus LPS-induced hepatitis model, we investigated the effects of orally administered bLF on the expression of inflammatory and anti-inflammatory factors in the small intestine, including IL-11. Furthermore, to clarify the role of IL-11 in the anti-hepatitis activity of bLF, we used IL-11 receptor α (IL-11Rα)-deficient mice. It has been demonstrated that in the absence of IL-11Rα, bone remodelling is impaired through the suppression of osteoblast differentiation( Reference Sims, Jenkins and Nakamura 24 ), and females are infertile due to abnormal development of the placenta( Reference Bao, Devi and Bowen-Shauver 25 ), due to the loss of IL-11 bioactivity.
Experimental methods
Mouse models of hepatitis
All animal studies were approved by the Committee for Animal Care and Oversight of Morinaga Milk Industry in accordance with its guidelines for the care and use of laboratory animals. We used four mouse models of hepatitis induced by GalN, CCl4, GalN plus LPS and zymosan plus LPS, respectively, to examine the anti-hepatitis activity of orally administered bLF. Mice were housed under constant conditions (21–25°C; humidity, 40–60 %; 12 h light–12 h dark cycle), fed a non-purified diet (Labo MR Stock; Nihon Nosan Kogyo) containing 18·7 % protein, 4·1 % fat, 5·7 % fibre, 6·7 % mineral mixtures and 0·2 % vitamin mixture, and allowed free access to tap water.
Expt 1 involved GalN-induced hepatitis mouse model. In Expt 1A, male CD1 mice (7–8 weeks old; Charles River) were intraperitoneally (i.p.) injected with GalN (Wako Pure Chemical Industries) at a dose of 500 mg/kg body weight. Mice were then orally administered bLF (Morinaga Milk Industry) at doses of 30, 100 and 300 mg/kg body weight as a suspension in water at a dose of 10 ml/kg for 14 d via a gastric tube (bLF-treated group). Bovine serum albumin (BSA, 300 mg/kg body weight; Sigma-Aldrich) was administered to the BSA-treated control group. On day 14, mice were administered a second i.p. injection of GalN at the same dose. At 18 h later, mice were anaesthetised using diethyl ether, their blood was harvested and their serum alanine aminotransferase (ALT) and aspartate aminotransferase (AST) concentrations were measured using a colorimetric diagnostic kit (Transaminase CII Test Kit; Wako Pure Chemical Industries). To evaluate the specificity of bLF (Expt 1B), other milk whey proteins (α-lactalbumin, β-lactoglobulin (Sigma-Aldrich) and BSA) were compared with bLF in the above model. These experiments were repeated twice with eight or nine mice per group. The untreated controls receiving no i.p. injections or oral administrations were also sampled during the experiment.
Expt 2, the CCl4-induced liver injury mouse model, included both acute (Expt 2A) and chronic (Expt 2B) treatments. In Expt 2A, male CD1 mice were orally pre-administered bLF or BSA daily at a dose of 300 mg/kg body weight for 14 d. On day 14, 0·4 ml/kg body weight of CCl4 (Kanto Chemical) dissolved in olive oil were injected i.p. at a concentration of 20 %. After 18 h, blood samples were collected under anaesthesia. The treated group included ten mice and the untreated group comprised six mice. In Expt 2B, chronic liver injury was induced by i.p. injection of CCl4 for 24 weeks. Mice were administered bLF or BSA once daily. On day 5 and then twice weekly, 0·08 ml/kg body weight of CCl4 dissolved in olive oil were injected i.p. at a concentration of 5 %. Mice were killed under anaesthesia at 72 h after the final injection of CCl4, and blood and liver samples were collected. After fixation in 20 % neutral-buffered formalin (Sakura Finetek), the number and sizes of fibrotic nodules on the surface of the entire liver were macroscopically measured. In the chronic liver injury experiment, serum IL-6 and TNF-α concentrations were also measured using an ELISA kit (DuoSet ELISA Development System; R&D Systems). The bLF-treated group included twelve mice, the BSA-treated group eleven and the untreated group six.
Expt 3 was a LPS plus GalN-induced lethality mouse model. GalN was used to increase the sensitivity of mice to the hepatotoxic effects of endotoxin( Reference Lehmann, Freudenberg and Galanos 15 ). Male CD1 mice were orally administered bLF or BSA at a dose of 300 mg/kg body weight for 14 d. On day 14, mice were administered LPS (5 mg/kg body weight, Escherichia coli 0111:B4; Sigma-Aldrich) and GalN (1 g/kg body weight) i.p. Survival of mice over the following 12, 24, 36 and 72 h was recorded. This experiment was repeated twice, with twenty-four mice in the bLF-treated group and twenty-two mice in the BSA group.
Expt 4 was a zymosan plus LPS-induced hepatitis mouse model. In Expt 4A, male BALB/c mice (7–8 weeks old; Charles River) were injected with zymosan (Sigma-Aldrich) into the tail vein at a dose of 25 mg/kg body weight on day 0. BSA or bLF was orally administered on days 1–7 at a dose of 300 mg/kg body weight once daily. At 3 h after the final oral administration, 15 μg/kg body weight of LPS was injected intravenously and blood was harvested 18 h later. This experiment was repeated twice, with twelve mice in each treatment group and six in the untreated group.
Effects of bovine lactoferrin on small-intestinal tissue (Expt 4B)
Direct effects of bLF on small-intestinal tissue under inflammatory conditions were determined using the i.v. zymosan plus LPS-induced hepatitis model, as described for Expt 4. On days 1, 3 and 6, and 18 h after LPS injection on day 8, a mucosal tissue sample excised from the middle section of the small intestine and a portion of the liver were frozen immediately and held at − 80°C until further analysis. Several anti-inflammatory factors, inflammatory factors and some related factors were analysed using real-time RT-PCR, as described previously( Reference Kuhara, Yamauchi and Iwatsuki 20 ). Based on the results from the real-time RT-PCR analysis, IL-11 and bone morphogenetic protein 2 (BMP2) production in the mucosal tissue of the small intestine were analysed by immunoblotting, as described previously( Reference Kuhara, Yamauchi and Iwatsuki 20 ). Chemiluminescent signals were detected using ECL Plus Western blotting detection reagents and film (GE Healthcare) and quantified using the imaging software cellSens (Olympus). Signal intensity was normalised to that of β-actin. This experiment was repeated three times, with six mice at each time point.
IL-11 receptor α-null mice (Expt 5)
Fertilised ova targeted at the IL-11 Rα locus( Reference Nandurkar, Robb and Tarlinton 26 ) were obtained from The Jackson Laboratory and IL-11Rα-null mice were then generated and obtained from Charles River. Heterozygous offspring were inbred to yield wild-type and IL-11Rα-null mice. Mouse genotyping was performed by Southern blot analysis as described previously( Reference Nandurkar, Robb and Tarlinton 26 ). First, male IL-11Rα-null mice and wild-type littermates (8–12 weeks old) were used in a zymosan plus LPS-induced hepatitis experiment to evaluate the effects of endogenous IL-11 (Expt 5A). A portion of each liver and the middle section of the small intestine were fixed in 20 % neutral-buffered formalin. Another portion of the small intestine was used for immunoblot analyses. Sections of paraffin-embedded liver and intestinal tissues were stained with haematoxylin and eosin (Muto Pure Chemicals) for histological analyses. Histological assessment of liver damage was microscopically conducted by an observer blinded to the treatment. Scores of grades 0–4 were assigned based on fibrosis, swelling cells, disarrangement and hyalinisation. Among the wild-type mice, none was categorised as grade 4. To measure IL-11 and BMP2 production, sections of intestinal tissue were stained using anti-IL-11 or anti-BMP2 antibody (Bioworld Technology) as the primary antibody, Simple Stain Mouse (anti-rabbit; Nichirei Biosciences) as the secondary antibody and a 3,3′-diaminobenzidine substrate (Nichirei Biosciences) according to the standard immunohistochemistry procedures. The sections were examined using light microscopy at 200 × magnification without knowledge of the treatment group. The intensity of immunostaining was semi-quantitatively graded from 0 to 3: grade 0, no staining; grade 1, focal or weak staining; grade 2, diffuse, moderate staining; grade 3, strong staining. This experiment was repeated three times, with nine mice in each of the treatment groups and six in the untreated group. Moreover, to investigate whether the endogenous IL-11 induced by bLF exerted anti-inflammatory activity against other forms of hepatitis, GalN- and acute CCl4-induced hepatitis models were also generated using IL-11Rα-null mice and wild-type littermates (8–12 weeks old, n 6; two pooled experiments). These experiments were designated as Expt 5B and 5C, respectively.
Statistical analyses
Data are expressed as means and standard deviations. Statistical analyses were performed using StatView 5.0 software (SAS Institute). For single variables, differences among groups were compared using ANOVA followed by the Tukey–Kramer test (ALT and AST concentrations in Expt 1, 2 and 4; TNF-α and IL-6 concentrations in Expt 2; BMP2 contents in Expt 5A). For two variables, we performed a two-way ANOVA followed by the Tukey–Kramer test and Student's unpaired t test (relative expression of mRNA and IL-11 and BMP2 concentrations in Expt 4; ALT concentrations in Expt 5). Variables with unequal variances were log-transformed. Significant differences in final survival (Expt 3) and the incidence of granulomas (Expt 2B) were determined using the χ2 test. The number of granulomas (Expt 2B) was evaluated using the Mann–Whitney U test. To assess the relationships between the degree of inflammation in the liver and IL-11 and BMP2 expression in the small intestine, Spearman's correlation coefficient was calculated for the histological data (Expt 5A). Differences were considered significant at P< 0·05.
Results
Oral bovine lactoferrin administration prevents the progression of hepatic failure in all hepatitis mouse models
In Expt 1A, i.p. injection of GalN at 2-week intervals significantly elevated serum AST concentrations in the BSA-treated control group compared with the untreated group 18 h after the last injection of GalN (Fig. 1(B)). Compared with the BSA control treatment, serum AST concentrations decreased in a dose-dependent manner up to 300 mg/kg body weight via oral administration of bLF for fourteen successive days. Serum ALT levels were significantly different between the BSA-treated controls and mice administered bLF at the dose of 300 mg/kg (P< 0·05). In Expt 1B, oral administration of bLF inhibited the elevation of AST concentrations compared with the BSA control treatment, but other milk whey proteins did not (Fig. 1(D)).
In Expt 2A, serum ALT and AST concentrations in the BSA-pre-treated control and bLF-pre-administered groups were significantly higher than that of the untreated control group at 18 h after i.p. injection of CCl4 (P< 0·05; Fig. 1(E) and (F)). However, serum ALT and AST concentrations were significantly lower in the bLF-pre-administered group than in the BSA-pre-treated control group (P< 0·05). In the chronic hepatitis experiment (Expt 2B), serum ALT concentrations were also elevated in the BSA-treated control group at 72 h after the final injection of CCl4 (P< 0·05; Fig. 1(G)). Oral bLF administration for 24 weeks suppressed the increase in serum ALT concentrations to levels that did not significantly differ from that of the untreated control group. Oral administration of bLF also significantly improved serum TNF-α and IL-6 levels compared with the levels of the BSA-treated control group (P< 0·05, Fig. 1(I) and (J)). Fibrotic nodules were produced on the surface of the liver after i.p. injection of CCl4 for 24 weeks. The incidence of nodules >5 mm in diameter was 58·3 % for the BSA-treated control and 16·7 % for the bLF-treated group (P< 0·05). The numbers of nodules < 5 mm in diameter were 5·17 (sd 2·29) and 2·64 (sd 1·96), respectively (P< 0·05).
In Expt 3, i.p. injection of GalN plus LPS following pre-administration of BSA for 14 d induced a high incidence of mortality in mice; 12 h after i.p. injection, the survival rate was only 18·2 %. However, pre-administration of bLF improved the survival rate to 45·8 % (P< 0·05). Both the survival rates were unchanged throughout the experiment (72 h).
In Expt 4A, i.v. injection of LPS at 7 d after zymosan treatment induced a significant elevation of serum ALT and AST concentrations 18 h after LPS injection in the BSA-treated control group compared with the untreated group (P< 0·05; Fig. 2(A) and (B)). Administration of bLF significantly inhibited the increase in serum AST concentrations compared with the BSA-treated control group (P< 0·05), and suppressed the increase in serum ALT levels to levels that did not significantly differ from that of the untreated group.
In Expt 4B, which was designed to avoid inflammation in the intestine, oral administration of bLF enhanced IL-11 and BMP2 expression in the small intestine. In a zymosan plus LPS-induced hepatitis model, profiling of changes in the expression of inflammatory and anti-inflammatory factors in the small intestine revealed a gradual increase in the mRNA expression of IL-11 during bLF administration (Table 1). On day 6, the mRNA expression of IL-11 was significantly higher in the bLF-treated group than in the BSA-treated control group (P< 0·05). The mRNA expression of BMP2 was also elevated in the bLF-treated group after LPS injection compared with the basal level before LPS injection (P< 0·05). Expression of the other factors tested, including IL-1β, TNF-α and transforming growth factor-β, did not change in the small intestine (data not shown). Thus, neither of the inflammation-inducing agents directly influenced small-intestinal tissue in this model. Immunoblot analyses also revealed an increase in IL-11 production in the small intestine following bLF administration after zymosan injection (Fig. 2(C) and (D)). IL-11 levels in the small intestine were higher in the bLF-treated group than in the BSA-treated control group (P< 0·05). Oral administration of bLF induced an increase in BMP2 production in the small intestine after i.v. injection of LPS (P< 0·05; Fig. 2(E) and (F)). In the small intestine, mRNA expression of suppressor of cytokine signal 3 (SOCS3), a suppressor of cytokine signalling via gp130, was markedly elevated after LPS injection, mirroring IL-11 production. In addition, mRNA expression of a negative regulatory molecule in BMP2 signalling, Smad6, was reduced by bLF, but not BSA, at days 3 and 8 (P< 0·05; Table 1).
BSA, bovine serum albumin; T, treatment; D, time.
a,bMean values within a row with unlike superscript letters were significantly different (P< 0·05).
* Mean value was significantly different from that of the BSA-treated control group (P< 0·05; unpaired t test).
† Fold of the mean of the untreated group, n 6 at each time point (three pooled experiments).
‡ mRNA obtained from the untreated control group were isolated at the same time as the other group or at the beginning or end of the experiment, as the case may be.
§ SOCS3 values were log-transformed before ANOVA calculations to adjust for unequal variances.
We also examined the mRNA expression of IL-11, BMP2 and the inflammatory cytokines IL-1β and TNF-α in the liver. Expression of IL-1β and TNF-α mRNA gradually increased after injection of zymosan, and LPS treatment strongly enhanced the levels of these mRNA, presumably reflecting inflammation (Table 2). Oral administration of bLF suppressed the expression of IL-1β at days 6 and 8 and the expression of TNF-α at day 6 compared with the BSA-treated control group (P< 0·05). After LPS treatment, mRNA expression of IL-11 in the BSA-treated control group increased relative to the basal mRNA levels of IL-11 (P< 0·05). In the bLF-treated group, mRNA expression of IL-11 was significantly lower (P< 0·05) than that in the BSA-treated control group before LPS injection. Unlike IL-11, mRNA expression of BMP2 in the liver was not affected in these mice.
BSA, bovine serum albumin; T, treatment; D, time.
a,b,c,dMean values within a row with unlike superscript letters were significantly different (P< 0·05).
* Mean value was significantly different from that of the BSA-treated control group (P< 0·05; unpaired t test).
† Fold of the mean of the untreated group, n 6 at each time point (three pooled experiments).
‡ IL-1β, TNF-α and IL-11 values were log-transformed before ANOVA calculations to adjust for unequal variances.
§ mRNA obtained from the untreated control group were isolated at the same time as the other group or at the beginning or end of the experiment, as the case may be.
Anti-inflammatory activity of bovine lactoferrin is abolished in IL-11 receptor α-null mice (Expt 5)
IL-11Rα-null mice and wild-type littermates were used to evaluate the effect of endogenous IL-11. Zymosan plus LPS injected intravenously induced a similar degree of hepatic failure in both wild-type and IL-11Rα-null mice (Fig. 3(A)). In wild-type mice, oral administration of bLF lowered serum ALT concentrations compared with that in the BSA-treated control group 18 h after LPS injection (P< 0·05). However, in IL-11Rα-null mice, administration of bLF did not suppress the increase in the levels of this indicator.
Immunohistochemical staining revealed the expression of IL-11 in the epithelium and in mesenchymal cells underlying the epithelium. In wild-type mice, the intensity of staining for IL-11 in the bLF-treated group (Fig. 3(D)) was greater than that in the BSA-treated control group 18 h after LPS injection (Fig. 3(E)), and similar results were obtained for IL-11Rα-null mice (Fig. 3(F)). The expression of BMP2 was mainly detected in the epithelium. For wild-type mice, administration of bLF, but not BSA, increased the intensity of BMP2 staining (Fig. 3(G) and (H)). BMP2 expression was also not observed in either treatment of IL-11Rα-null mice (Fig. 3(I)). Immunoblot analyses revealed that after i.v. injection of LPS, the production of intestinal BMP2 induced by bLF administration was suppressed in IL-11Rα-null mice (P< 0·05; Fig. 3(B) and (C)). Histochemical analyses showed no inflammation in the small intestine (data not shown), in accordance with our experimental design.
The anti-inflammatory activity of orally administered bLF was also examined in the GalN- and acute CCl4-induced hepatitis models using IL-11Rα-null mice. Similar to that in CD1 mice in Expt 1, oral administration of bLF for 14 d suppressed the increase in serum ALT levels in the B6-background wild-type mice (P= 0·066); however, in IL-11Rα-null mice, bLF administration did not reduce serum ALT levels (Expt 5B; Fig. 3(J)). Furthermore, pre-treatment with bLF for 14 d significantly inhibited the CCl4-induced increase in serum ALT levels in wild-type mice (P< 0·05), although this treatment was not efficacious in IL-11Rα-null mice in Expt 5C (Fig. 3(K)).
Finally, correlations between the hepatic inflammation score and the expression of IL-11 and BMP2 in the small intestine were calculated based on the histochemical results (Fig. 4). The inflammation scores generally paralleled serum ALT and AST levels. In wild-type mice, the expression score for IL-11 in the bLF-treated group was negatively correlated with the hepatic inflammation score (P< 0·05; Fig. 4(A)); however, no negative correlation was observed with BMP2 expression (Fig. 4(C)). In IL-11Rα-null mice, there was no correlation between the inflammation score and the expression of IL-11 (Fig. 4(B)) or BMP2 (Fig. 4(D)).
Discussion
In the present study, we demonstrated that oral administration of bLF exerts anti-inflammatory activity in several mouse models of hepatitis designed to correspond to clinical disorders, such as chronic biliary disease, GalN-induced hepatitis( Reference Jonker, Dijkhuis and Hardonk 27 ), hypoplastic liver injury, CCl4-induced hepatitis( Reference Nakatsuka, Taniguchi and Hirata 16 ) and hepatitis virus infection, using LPS( Reference Lehmann, Freudenberg and Galanos 15 ). A few small clinical studies have suggested that bLF ingestion decreases serum ALT and HCV RNA concentrations( Reference Tanaka, Ikeda and Nozaki 8 , Reference Iwasa, Kaito and Ikoma 28 ); however, a randomised, double-blind, placebo-controlled, large-scale trial of bLF in patients with chronic hepatitis C did not demonstrate significant efficacy( Reference Ueno, Sato and Yamamoto 29 ). Furthermore, in a clinical study of ninety patients with chronic hepatitis C, oral administration of bLF inhibited lipid peroxidation and the elevation of serum ALT concentrations, but did not alter serum HCV RNA levels( Reference Konishi, Iwasa and Yamauchi 30 ). These clinical data imply limited antiviral activity and effective anti-inflammatory activity of bLF in hepatitis patients.
Given the observation that oral bLF administration before the occurrence of inflammation suppressed serum AST levels (Expt 2A) and the mortality rate (Expt 3), and that ingested bLF was not detected in the portal vein( Reference Yamaguchi, Matsuura and Kobayashi 17 ), we hypothesise that bLF acts as a modulator on an intestinal function and, subsequently, anti-inflammatory and restorative factors are produced and propagated. In the zymosan plus LPS-induced hepatitis model of the present study, we searched for such factors and identified IL-11 and BMP2. In the reported experimental models, IL-11 has exhibited effectiveness in rats with colitis( Reference Qui, Pfeiffer and Keith 31 ) and in mice with hepatitis( Reference Bozza, Bliss and Maylor 32 ), as with bLF. Some clinical effects of IL-11 treatment are also similar to those of bLF. In patients undergoing chemotherapy, IL-11 prevents gastrointestinal epithelial disintegrity and gut-associated infections( Reference Ellis, Zwaan and Hedstrom 33 ). bLF supplementation prevents sepsis in neonates( Reference Manzoni, Rinaldi and Cattani 9 ). In patients with psoriasis, IL-11 reduced cutaneous inflammation( Reference Trepicchio, Ozawa and Walters 34 ). Oral administration of bLF improved dermatological inflammatory symptoms in patients with tinea pedis( Reference Yamauchi, Hiruma and Yamazaki 35 ). In addition, a clinical study of HCV patients has suggested that IL-11 has beneficial anti-inflammatory effects( Reference Lawitz, Hepburn and Casey 36 ). In the zymosan plus LPS-induced hepatitis model, we attempted to measure serum IL-11 concentrations in the portal vein following the administration of bLF; however, its concentration was undetectable in many samples. Serum IL-11 concentrations were detected only in a few oral bLF-treated mice, but not in the BSA group (data not shown). However, induction of IL-11 production in the intestine supports the beneficial effect of orally administered bLF, because the anti-inflammatory effect of orally administered bLF completely disappeared in IL-11Rα-null mice. These observations in IL-11Rα-impaired mice suggest that bLF activity is mediated by IL-11.
In the present study, we also observed that oral administration of bLF significantly increased BMP2 expression. BMP2 performs a variety of functions, including embryonic development, bone morphogenetic differentiation and regulation of systemic Fe balance( Reference Babitt, Huang and Xia 37 , Reference Chen, Zhao and Mundy 38 ). Additionally, it has been suggested that BMP2 regulates bone homeostasis in concert with IL-11( Reference Takeuchi, Watanabe and Ishii 39 ), i.e. IL-11 enhances BMP2–Smad1 signalling via formation of the Smad1–STAT3 (signal transducer and activator of transcription 3) complex( Reference Nakashima, Yanagisawa and Arakawa 40 ), leading to osteoblastogenesis. BMP2 has been shown to play an important role in the wound-healing response in rats with CCl4-induced hepatitis( Reference Nakatsuka, Taniguchi and Hirata 16 ). In the present study, mRNA expression of IL-11 in the small intestine was elevated before LPS injection (Table 1), but an increase in the mRNA expression of BMP2 was not noted until after LPS injection. We previously demonstrated that bLF did not directly stimulate the expression of BMP2 in cultured intestinal epithelial cells, myofibroblasts or monocytes( Reference Kuhara, Yamauchi and Iwatsuki 20 ). In the present study, bLF-induced enhancement of BMP2 production was reduced in IL-11Rα-null mice (Fig. 3(B) and (C)). In addition, expression of Smad6, a suppressor of BMP2 signalling, was suppressed by bLF administration (Table 1). Collectively, these results suggest that bLF regulates BMP2 production and activity in the intestinal epithelium via induction of IL-11, as in osteoblastogenesis( Reference Takeuchi, Watanabe and Ishii 39 ). In the present study, BMP2 expression in the small intestine was not correlated with the anti-inflammatory activity of orally administered bLF (Fig. 4). BMP2 expression in the liver did not increase in mice with hepatitis, suggesting that the anti-inflammatory activity of BMP2 is limited in mouse models.
In clinical trials, bLF ingestion significantly retarded the growth of adenomatous colorectal polyps( Reference Kozu, Iinuma and Ohashi 7 ). In the same trials, bLF administration significantly enhanced NK cell activity throughout the therapeutic period. BMP2 has been shown to act as a tumour suppressor, promoting apoptosis in colonic epithelial cells( Reference Hardwick, Van Den Brink and Bleuming 41 ). BMP2 expression was absent in the microadenomas of patients with familial adenomatous polyposis( Reference Hardwick, Van Den Brink and Bleuming 41 ). Furthermore, BMP2 has been shown to stimulate the production of IL-18( Reference Hori, Sawai and Tsuji 42 ). Previously, we reported that oral administration of bLF increased the production of IL-18 in the intestinal epithelium, thereby increasing NK cell activity in mice( Reference Kuhara, Yamauchi and Tamura 19 ). It has also been reported that IL-11 signalling is essential for the differentiation of NK cells in certain organs( Reference Ain, Trinh and Soares 43 ). We propose that the immunomodulatory activity of bLF, particularly the enhancement of NK cell activity, is associated with these factors.
In conclusion, oral administration of bLF protected against inflammation in mice with hepatitis. Orally ingested bLF enhanced the expression of IL-11 and BMP2 in the small intestine. In IL-11Rα-null mice, the anti-inflammatory and BMP2-inducing activities of orally administered bLF were abolished. The anti-inflammatory effect of orally administered bLF may arise from its promotion of IL-11 production in the small intestine.
Acknowledgements
The authors thank Mr Hirokazu Hamano for assistance with the statistical analysis.
The present study received no specific grant from any funding agency from commercial or not-for-profit sectors.
The authors' contributions are as follows: T. K. designed and conducted the study, analysed the data and wrote the manuscript; A. T. conducted the research and analysed the data; K. Y. and K. I. revised the manuscript; T. K. had primary responsibility for the final content. All the authors read and approved the final manuscript.
There are no conflicts of interest.