1. Introduction
In China, the largest pig-raising country in the world, feed resources are gradually scarce, and the imports of some grain crops including corns are increasing. During the last decade, the pattern of the feed industry has changed dramatically in price and accessibility of animal feed raw materials [
1]. Therefore, it is an urgent problem to find alternatives to grain feed materials. The supply of milling by-products, which is a rich source of dietary fiber (DF), has increased. It is essential to understand the effects of these new and potential DF sources on gut health in pigs. A lot was already known about the impact of DF on swine nutrition [
2,
3,
4,
5,
6]. In addition, people are increasingly interested in adding dietary fiber to pig diets because DF has been found to modulate gut microbiota and improve gut health [
7].
Defatted rice bran (DFRB), an abundant and underutilized agricultural coproduct of the brown rice refining process, is rich in energy and DF [
8,
9]. The concentration of soluble dietary fiber and insoluble dietary fiber were 1.4% and 26.1% in DFRB, respectively (measured value of the present study). Ingredients of DFRB usually increase beneficial bacteria, reduce potentially pathogenic bacteria populations, and improve gut barrier function [
10,
11,
12,
13]. Some studies have indicated that addition of rice bran in diets may have a prebiotic effect. Addition of 10% and 20% full fatted rice bran (FFRB) in mice diets significantly reduced the enteric burden of
Salmonella infection and increased
Lactobacillus [
13]. Adding 10% rice bran to mice diets increased
Lactobacillus [
10]. Addition of 10% rice bran improved feed utilization efficiency and tended to increase intestinal
Bifidobacteria in weaning pigs [
14]. Arabinoxylan (insoluble dietary fiber) reduced colonic mucosa permeability of healthy humans [
11].
However, the high level of DFRB may have a negative effect on growth performance, intestinal bacteria, and gut barrier function because of the high concentration of DF. Warren et al. [
15] found addition of 10% or 20% DFRB to growing pigs’ diets had no effect on growth performance, but addition of 30% reduced gain to feed ratio (G:F). Gloria et al. [
16] found that average daily feed intake (ADFI) increased linearly and G:F decreased linearly as DFRB increased from 0% to 30% in the diets of finishing pigs. The high mixed-linked β-glucan (soluble dietary fiber) in diets fed to piglets significantly reduced numbers of
Lactobacilli in the small intestine and decreased the microbial diversity in the colon [
17]. Addition of 10% guar gum which is rich in soluble dietary fiber increased colonization of enterotoxigenic
E. coli and reduced body weight gain in pigs infected with enterotoxigenic
E. coli [
18].
Our previous study has shown that the growth performance of Suhuai finishing pigs were not affected by 28% DFRB [
19]. Intestinal barrier function and bacteria are very important to porcine health, whereas effects of increasing levels of DFRB on intestinal barrier function and bacteria was not clear. We hypothesized that moderate levels of DF may improve intestinal barrier function and beneficial bacteria, but excessive levels of DF may have a negative effect on them, and there is an optimal replacement of DFRB for porcine intestinal health.
Therefore, the aims of this study were to assess the effects of increasing levels of DFRB as a replacement for corns on intestinal physical barrier function and bacteria and determine the optimal substitution level of DFRB in finishing pigs.
2. Materials and Methods
2.1. Experimental Design and Animal Management
A total of 35 Suhuai castrated finishing pigs (age: 158.5 ± 2.0 d, initial body weight: 62.9 ± 0.8 kg) were blocked by initial body weight and randomly divided into one of five experimental diets using a complete randomized block design. Suhuai pig is a new breed that is bred by Chinese Huai pig (25%) and Western Large white pig (75%). The five treatments included a control group and four experimental groups in which maize was separately replaced by 7%, 14%, 21%, and 28% DFRB. All pigs were fed by the Osborne Testing Stations System (OTSS) and it can accurately record daily intake, daily weight gain for each pig. Therefore, each pig was identified as a replicate and there were seven replicates in each treatment. The size of each pen was 5.25 × 2.50 m. The pre-feeding period of the trial was 10 days and all pigs were fed with the same control diet during this period. The feeding experiment lasted 28 d. The finishing body weight of control group, 7%, 14%, 21%, and 28% DFRB group were 82.7 ± 2.1, 82.2 ± 2.0, 84.8 ± 2.1, 83.9 ± 3.0, and 84.8 ± 2.9 kg, respectively. All the pigs were held in the same pigsty with a half seam floor, air-source heat pumps, and a fan system. The temperature inside the piggery varied from 15.5 to 19.6 °C for the whole experimental period. Pigs had ad libitum access to feed by OTSS and water by water-saving type stainless-steel drinker. Pigs were healthy and no mortality or diarrhea was observed throughout the experiment. The experimental protocol and procedures were approved by the Animal Care and Use Committee of Nanjing Agricultural University, China (with protocol SYXK (Su) 2017-0007).
2.2. Diet Design
The basal diet used for pigs was formulated according to the Feeding Standard of Swine 60–90 kg Standard of Meat-fat Type Growing-finishing Pig (NY/T 65-2004). It was mainly maize that was replaced by 7%, 14%, 21%, and 28% DFRB in four experimental diets. In addition to maize, the other raw materials including wheat bran, soybean oil, lysine also made a small change in four experimental diets to balance metabolic energy and amino acids among five groups. The feed was produced by Huaian Zhengchang Feed Co., Ltd. (Jiangsu, China). Crude protein (CP), crude fiber (CF), ether extract (EE), acid detergent fiber (ADF), neutral detergent fiber (NDF), and hemicellulose contents of corn and DFRB are summarized in
Table 1. The chemical characteristics of five diets were analyzed as previously described [
20] and presented in
Table 2.
2.3. Sample Collection
After the 28-d trial, blood samples were collected from jugular vein and centrifuged at 3000×
g at 4 °C for 10 min to collect serum [
21]. The serum was stored at −80 °C until further analyses of endotoxin, diamine oxidase (DAO), and D-lactate. All pigs were stunned by electric shock and slaughtered. The abdomen of each pig was immediately opened, and the jejunum, cecum, and colon were removed. The middle sections (1 cm) of the colon and cecum were collected and then fixed in 4% paraformaldehyde for histological analysis. Mucosal scrapings from the jejunum, ileum, and colon were prepared and stored at −80 °C for measuring 16S rRNA gene copy numbers in bacteria and the mRNA levels of
Caspase 3,
Bax, and
Bcl-2L1.
2.4. Histological Measurements
Since fibers are mainly fermented in the large intestine and may have an impact on morphology of the large intestine, we only measured caecal and colonic mucosal morphology. Crypt depth and thickness of the intestinal wall were determined as described by Shen et al. [
22]. Fixed intestinal segments were dehydrated with alcohol and encapsulated with paraffin. Consecutive sections at 5 μm thickness were stained with hematoxylin-eosin for histology morphological measurements. The crypt depth was determined on well oriented crypts as distance from the crypt mouth to the crypt base at the basement membrane. Thickness of the intestinal wall was determined as vertical distance from the lateral side of the intestinal wall to the crypt mouth. Crypt depth and thickness of the intestinal wall was measured with a Nikon Eclipse 80i microscope (Nikon Company, Tokyo, Japan).
2.5. Blood Sample Analysis
According to the manufacturer’s instructions, the levels of endotoxin, D-lactate, and DAO in the serum were measured by a reagent kit (Jiancheng Bioengineering Institute of Nanjing, Nanjing, Jiangsu, China). The range of the detection of endotoxin, D-lactate, and DAO was 0–1600 EU/L, 0–4.8 μg/L, and 0–80 ng/mL, respectively. Serum was diluted 10 times when D-lactate was measured.
2.6. DNA Isolation, Design, and Validation of Primers for Total Bacteria Escherichia coli, Clostridium perfringens, Bifidobacterium and Lactobacillus
Bacterial DNA of the intestinal mucosal scrapings was extracted by FastDNA
® Spin Kit for Soil (MP Biomedicals, Irvine, CA, USA). All the primers (
Table 3) were commercially synthesized by Beijing Tsingke Biotech Co., Ltd. DNA quality and concentration of were measured using UL-1000 (Shanghai Meixi Instrument Co., Ltd., Shanghai, China). For the quantification of bacteria in samples, standard curves were made by constructing standard plasmids, as described by Han et al. [
23]. The specific PCR product of target bacteria was purified by the Cycle Pure Kit PCR (OMEGA Bio-tek, Norcross, GA, USA), and inserted into a Versatile Simple Vector (TsingKe, Nanjing, China). The plasmid DNA was extracted using the AxyPrep
TM Plasmid Miniprep Kit (AXYGEN, Fremont, CA, USA) and standard plasmids were constructed successfully. The copies were calculated by the following formula: (6.0233 × 10
23copies/mol × DNA concentration (μg/mL))/(660 × 10
9 × DNA size (bp)). A 10-fold serial dilution series of plasmid DNA was used to construct the standard curves for total bacteria,
E. coli,
C. perfringens,
Lactobacillus, and
Bifidobacterium. Each standard curve was constructed by linear regression of the plotted points, and cycle threshold (CT) values were plotted against the logarithm of template copy numbers. Quantitative analysis of PCR was performed with TB Green
® Premix Ex Taq ™ II (TaRaKa Biotechnology, Shiga, Japan) by an ABI QuantStudio 3 Real-Time PCR System (Applied Biosystems, Foster City, CA, USA).
2.7. Real-Time Quantitative PCR
Caspase-3 is considered to be the most important apoptotic executor, and its activation is a marker of irreversible apoptosis. Bcl-2L1 protein family plays an important role in regulating apoptosis, in which Bcl2 is an anti-apoptotic gene and Bax is a pro-apoptotic gene. All of them play an important role in the process of apoptosis. To evaluate the effects of increasing levels of DFRB as a replacement for corns on intestinal cell proliferation and apoptosis of finishing pigs, the mRNA levels of Caspase 3, Bax, and Bcl-2L1 were detected by real-time quantitative PCR.
According to the manufacturer’s guidelines, total RNA of intestinal mucosa was extracted using TRIZOL (Shanghai Yuanye Biotechnology Co., Ltd., Shanghai, China). The RNA concentration and quality were measured using UL-1000 (Shanghai Meixi Instrument Co., Ltd., Shanghai, China). The RNA samples were reverse transcribed into complementary DNA using 5X All-In-One RT MasterMix (Applied Biological Materials, Richmond, B.C., Canada). Quantitative analysis of PCR was performed with TB Green ® Premix Ex Taq ™ II (TaRaKa, Shiga, Japan) by an ABI QuantStudio 3 Real-Time PCR System (Applied Biosystems, Foster City, CA, USA).
The reaction was performed using the following cycle program: a hold stage at 95 °C for 10 min; 35 cycles for PCR stage at 95 °C for 15 s and at 60 °C for 60 s; a melt curve stage at 95 °C for 15 s, at 60 °C for 60 s, and at 95 °C for 1 s. All samples were analyzed for three repetitions. The relative expression of the
Caspase 3,
Bax, and
Bcl-2L1 mRNA was calculated using the 2
−ΔΔCt method [
31].
2.8. Statistical Analysis
Bacterial 16S rRNA gene copy numbers were transformed (log 10) before statistical analysis. Linear and quadratic effects of dietary treatments on all indices were determined by curve estimation and some indices including serum endotoxins, DAO and
Escherichia coli in the jejunum in
Appendix A Table A1 were also analyzed by one-way ANOVA (SPSS 25.0) (SPSS Inc., Chicago, IL, USA). DFRB was the main effect. Each pig was considered as the experimental unit for all analyses. The α-level was set as 0.05 for significance determination. Data are presented as means with their pooled standard errors. The linear effects was determined by equation:
where y is dependent variable, and x is the content of DFRB.
The optimal substitution level of corn by DFRB was predicted by quadratic regression equation as described by Souza et al. [
32]. Quadratic regression equation:
where y is dependent variable, and x is the content of DFRB.
4. Discussion
Integrated intestinal mucosal barrier is important for the defense of pathogenic bacteria [
33,
34]. The intestinal permeability can be increased by the injured intestinal mucosal barrier. The intestinal barrier function has to do with many factors, including endotoxins, D-lactate concentration, and DAO activity in serum [
35,
36,
37,
38]. They have been considered as markers for evaluating the extent of intestinal mucosal damage and repair [
39]. As one of the secretions of
Escherichia coli, serum endotoxins activity increased with increased intestinal permeability or injury to intestinal barrier integrity [
40]. D-Lactate is the end product of intestinal bacteria. Mammals produced neither D-lactate nor D-lactate dehydrogenase. Hence, they maintain a lower level of D-Lactate in healthy conditions [
41]. When intestinal mucosal integrity is impaired, almost all D-lactate will release into the blood. Thus, this indicates that serum D-Lactate reflects the integrity and maturity of intestinal mucosa [
42]. DAO is one of the DAO catalyzed by deaminases, only exists in the villi of the upper small intestine, and its increasing concentrations indicate increased intestinal epithelial permeability or damage to intestinal barrier function [
43,
44]. Serum endotoxins concentration and DAO activity were both increased with the DFRB level. There was a quadratic response in serum D-lactate concentration to the increased DFRB. However, compared with control group, serum endotoxins concentration and DAO activity were not different in pigs fed with 7% DFRB in the diet. Therefore, 7% DFRB had had no adverse effect on intestinal permeability.
On the other hand, integral morphological structure is important for the intestinal tract to maintain the ability to secret, digest, and absorb nutrients. As fibers are mainly fermented in the large intestine and may have an impact on morphology of the large intestine, we only measured cecal and colonic mucosal morphology. The present study showed that colonic morphology was not influenced by the increased DFRB. However, in the cecum, thickness of the intestinal wall significantly increased with increasing level of DFRB in the diets while crypt depth/thickness of the intestinal wall ratio decreased with the increasing level of DFRB in the diets. One possible explanation for this result is that muscle thickness increased but crypt depth remained unchanged with the increasing level of DFRB in the diets. Additionally, increased muscle thickness may increase the mixing of intestinal contents to increase digestibility of the DF.
The intestinal microflora is very important to intestinal health, not only because the imbalance of the microflora may lead to an inflammation response, but also may compete with the host for nutrients [
45]. The microflora enhances the intestinal mucosa barrier function and reduces the adhesion of pathogenic microorganisms to the mucosa, thus reducing the chance of pathogenic microorganisms entering enterocytes.
Lactobacillus and
Bifidobacteria are the main beneficial bacteria in the intestinal tract of mammals. They play a resistant role against intestinal pathogens through a variety of mechanisms.
Lactobacillus is considered to be a reflection of changes in the population structure of beneficial bacteria because a large number of intestinal bacteria cannot be cultured [
46]. It is controversial to consider
E. coli as a marker of pathogenic bacteria; however, the number of
E. coli increased in the intestinal tract of diarrhea pigs [
47]. Therefore, the reduction of
E. coli caused by dietary intervention is considered to be beneficial by many people to a certain extent [
48,
49,
50]. Many studies have shown that DF is beneficial to the proliferation of beneficial bacteria and inhibits harmful bacteria. Drew et al. [
51] found that wheat-based diets increased
Bifidobacterium and reduced total aerobes and
Clostridium. Similarly, Nielsen et al. [
52] reported that addition of arabinoxylan (AX) in pig diets increased
Bifidobacterium and
Lactobacillus in the feces. In line with the previous findings, this study shows that there were declined
Escherichia coli and increased
Bifidobacterium as DFRB increased from 0% to 7%.
Escherichia coli increased and
Bifidobacterium declined when 14% DFRB was fed. One possible explanation might be that high-fiber diets have a negative effect on intestinal barrier function and is not conducive to the growth of beneficial bacteria. The high level of DFRB have a negative effect on the intestinal barrier function, which may be mediated by the changes of microbial composition and the accompanying changes of intestinal permeability.
This study shows the mRNA levels of
Caspase 3,
Bax, and
Bcl-2L1 were not influenced by the level of DFRB in the diets in jejunum, ileum, and colon. The results showed that the addition of defatted rice bran in the diet did not affect the apoptotic process of intestinal cells. This is consistent with the previous study made by Gregoire et al. [
53]. They reported that a short-term increase in dietary fiber does not result in a significant difference in cell proliferation [
53]. However, Jin et al. [
54] found that the number of epithelial cells exhibiting DNA fragmentation (indicating programmed cell death) was greater in growing pigs consuming the high-fiber diet than in the low-fiber diet group for jejunum and ileum. The difference in the results may be due to the different types of fibers and the different stages of animal growth.