Background
Clostridium difficile is the most common known cause of nosocomial diarrhea. Recently, the incidence and the frequency of morbidity and mortality from
C. difficile infection (CDI) have increased [
1,
2]. These have been attributed to the BI/NAP1/III/027 strain which is fluoroquinolone resistant, carries an 18 bp deletion in the
tcdC gene (a possible negative regulator of toxin gene production), produces binary toxin and displays hypertoxigenic properties [
3]. Current treatment consists of antibiotics that suppress normal flora. While transiently effective, these treatments result in a 20-30% relapse rate, prolonged shedding and reacquisition of
C. difficile [
4]. Moreover, CDI secondary to the emerging strain has already been reported to be less responsive to metronidazole and is associated with more relapses compared with the historical strains [
5]. There are now more patients requiring colectomies and ICU care. New non-antimicrobial approaches to treatment are urgently needed for CDI.
Several clinical studies have shown that glutamine and its stable derivative, alanyl-glutamine, improve gastrointestinal mucosal structure and function following injury from chemotherapy, radiotherapy or prolonged parenteral nutrition [
6]. In addition to its role as an important building block for protein synthesis, glutamine also is a regulator of intracellular kinases [
7], redox status [
6], cell proliferation [
8], apoptosis [
9] and heat shock protein expression [
10].
C. difficile toxin A induces activation of caspases 6, 8, 9 and 3 in intestinal epithelial cells [
11]. Glutamine and alanylglutamine have been shown to inhibit caspase 8 and decrease toxin A-induced apoptosis [
12]. Activation of adenosine A
2A receptors attenuates inflammation in many tissues. A
2A receptor activation in neutrophils decreases production of reactive oxygen species. In macrophages A
2A receptor activation decreases secretion of inflammatory cytokines (e.g. IL-2, IL-12, IL-6, TNFα) and increases IL-10 [
13,
14]. In mouse ileal tissues, ATL 313, another adenosine A
2A receptor agonist, reduced
C. difficile toxin A-induced mucosal injury, neutrophillic infiltration and cell death [
15].
In this study we examined the effect of combining alanyl-glutamine and ATL 370 on secretion and mucosal structural damage in C. difficile toxin A-induced enteritis in rabbits and cecitis in mice. We also evaluated apoptosis by immunohistologic staining in the rabbit ileum and the secretion of inflammatory (keratinocyte-derived chemokine, KC) and anti-inflammatory (IL-10) cytokines in the mouse cecum.
Methods
Rabbit ileal loop model
Animal protocols were approved by the University of Virginia Animal Care and Use Committee. New Zealand White rabbits weighing approximately 2 kg were fasted overnight. The rabbits were anesthetized with ketamine (60-80 mg/kg) and xylazine (5-10 mg/kg), administered intramuscularly or by inhalational isoflurane. A midline abdominal incision was made to expose the small bowel. After the ileum was flushed with 5-10 ml of PBS, 8-10 loops were created by ligation using double ties and a 1-cm interval was left between the loops. Control loops were injected with either PBS (1 ml/loop) alone or C. difficile toxin A (TechLab, Blacksburg VA) (10-20 μg/loop dissolved in 1 ml of PBS). Treated animals received alanyl-glutamine (Sigma-Aldrich) at a final concentration of 3, 10, 30 or 100 mM injected into the intestinal lumen just prior to toxin A injection. The ligated loops were then returned to the abdomen and the abdominal wall sutured closed. Treated animals also received either the adenosine A2A receptor agonist, ATL 370 (Dogwood Therapeutics), at 0, 1.5 ng, 15 ng or 150 ng dissolved in 250 uL PBS by intravenous route immediately after administration of toxin A (time 0) and 2 h after the addition of toxin A. A separate experiment was performed using equimolar concentrations (3.5 ng, 34.5 ng, or 345 ng) of adenosine A2A receptor antagonist, SCH 58261 (Tocris Bioscience), given intravenously 5 min after the administration of ATL 370 (at time 0 and 2 h later) to investigate the specificity of the agonist effect.
Mouse cecal loop model
To confirm results from the rabbit experiments and determine the effects of treatment on cytokine production, mouse cecal loop experiments were also performed. C57BL/6 male mice, weighing 23-25 g each, were fasted overnight. The mice were anesthetized with ketamine (60-80 mg/kg) and xylazine (5-10 mg/kg), administered intramuscularly. A midline abdominal incision was made to expose the cecum. After flushing with PBS, a ligature was placed each at the ileal and colonic openings of the cecum, while avoiding ligation of the vascular supply. Control loops were injected with either PBS (200 μL/loop) alone or C. difficile toxin A (20 μg/loop dissolved in 200 μL of PBS). Treated animals received alanyl-glutamine at a final concentration of 100 mM injected into the cecal lumen just prior to toxin A injection. The ligated cecal loops were then returned to the abdomen and the abdominal wall sutured closed. Treated animals also received either the adenosine A2A receptor agonist, ATL 370, at a dose of 3 ng/g by subcutaneous route, immediately after administration of toxin A (time 0).
Secretion and histopathology
After 4-5 h of incubation, the animals were euthanized and the abdomen incised. The intestines were exposed and the lengths of each ligated ileal loop were measured. Intestinal fluid was extracted from the loop and quantified. The volume:length ratio (V:L) was calculated in milliliters per centimeter per loop. The gross description (clear, serous, purulent, or bloody) of the collected fluid was also noted. One set of tissues was fixed with 10% formalin and stained with hematoxylin-eosin for histopathology. Each slide was read blindly by at least 2 investigators (CAW, SWP, GC). A grading scale for histopathology of intestinal tissues, previously formulated and published [
16‐
18], was used to grade each slide according to mucosal disruption, cellularity, and vascular congestion. The final histopathologic score is the mean of the scores of all graders. Samples of intestinal tissue from control and treated loops were placed in liquid nitrogen for subsequent protein and RNA extraction.
In situapoptotic staining
Paraffin-embedded tissues were analyzed for apoptotic cells using ApopTag® Peroxidase In Situ Apoptosis Detection Kit. All steps were performed according to the manufacturer's instructions. Crystal Violet free Methyl Green was used as the counterstain. Images were obtained by Olympus BX41TF with Digital Camera and MIcrosuite Pathology provided by the University of Virginia Biorepository and Tissue Research Facility. Apoptosis was quantified by counting peroxidase-stained cells in 3 randomly chosen high power fields (hpf) per tissue section quadrant. The total number of cells was then divided by 12 (3 hpfs × 4 quadrants) and the reading reported as number of apoptotic cells per hpf.
KC, IL-10 enzyme-linked immunosorbent assays (ELISA)
Detection and quantification of KC and IL-10 proteins present in mouse cecal samples were determined by using Mouse CXCL1/KC and IL-10 Quantikine ELISA kits (R&D Systems), respectively. Cecal tissues, harvested from the mouse cecal loop model described above, were minced, bead beat for 1 min twice (with 2 min interval on ice in between bead beating) and lysed in NP-40 lysis buffer for 20 min on ice, followed by spinning at 14,000 rpm at 4
°C for 30 min. Protein concentration in a 1:10 dilution of the supernatant was measured using bicinchoninic acid assay (BCA) following the manufacturer's instructions (Pierce Thermo-Fisher Kit) [
19]. ELISA on the mouse cecal lysates was performed according to manufacturer's instructions [
20,
21]. Both sample sets were analyzed in triplicate. Of note, antibodies to rabbit IL-10 and IL-8 are not readily available and homologous to human sequences by only 80% and 78%, respectively. Thus, we opted to use mouse tissues to detect cytokine production.
KC and IL-10 gene expression assay
RNA was extracted from mouse cecal tissues using Qiagen RNeasy mini Kit according to manufacturer's instructions. RNA concentration was quantified and checked for purity (A260:280 ratio) by standard spectrophotometry (Biophotometer, Eppendorf, Hamburg, Germany). Synthesis of cDNA by Reverse Transcriptase PCR was performed using SuperScript III First-Strand Synthesis System SuperMix (Invitrogen) with the use of oligo (dT) as primers. cDNA was used in quantitative PCR for measuring KC and IL-10 expression compared to hypoxanthine guanine phosphoribosyl (HPRT) expression. The primers used were: murine HPRT (forward: 5'-TCC CTG GTT AAG CAG TAC AGC CCC-3; reverse: 5'-CCA ACA AAG TCT GGC CTG TAT CCA A-3') (GenBank no. NM_013556.2), IL-10 (forward: 5'-GGC GCT GTC ATC GAT TTC TCC CC-3'; reverse: 5'-GGC CCT GTA GAC ACC TTG GTC TTGG-3') (GenBank no. NM_010548.2) and Cxcl1/KC (forward: 5'-CGC ACG TGT TGA CGC TTC CCT-3'; reverse: 5'-GTC CCG AGC GAG ACG AGA CCA-3') (GenBank no. NM_008176.3). The reaction was performed in a Bio-Rad iCycler iQ multicolor PCR Detection System using iCycler software (version 3.0). The relative gene expression was determined using the 2
-ΔΔCt (Livak) method using HRPT as the housekeeping gene [
22].
Statistical analysis
Continuous variables, such as V:L, histopathologic score, protein levels, were expressed as means ± standard error of the mean (SEM). For statistical comparison of the magnitude of secretion, the amount of inflammation, and protein levels, a one-way analysis of variance (ANOVA) with Bonferroni post-hoc test to compare multiple selected pairs was performed. To compare 2 groups of treatment only, a 2-tailed Student's unpaired t test with Welch's correction was applied.
Discussion
C. difficile toxin A has repeatedly been shown in numerous
in vitro and
in vivo studies to elicit an exuberant inflammatory response causing recruitment of inflammatory cells (neutrophils, macrophages and mast cells), secretion of inflammatory cytokines (IL-8, IL1B, TNFα), cell death, mucosal damage and intestinal secretion [
23‐
25]. Although both
C. difficile toxins A and B glucosylate Rho GTPases [
25] and are important in pathogenesis during infection [
26,
27], most animal models of intoxication--rabbits, mouse, rats and hamsters, are more responsive to the enterotoxic effects of toxin A than toxin B [
23,
28]. This study has shown that adenosine A
2A receptor agonist, ATL 370, ameliorates
C. difficile toxin A-induced intestinal epithelial disruption, inflammation and secretion in the ligated loop model of enteritis in rabbits. These effects were augmented by co-administration of the dipeptide, alanyl-glutamine. Significant decreases in IL-8 and IL-10 in mouse cecal tissues were also mostly noted with the co-administration of ATL370 and alanyl-glutamine.
Adenosine is a naturally occurring purine nucleoside that is produced in many tissues in response to inflammatory or hypoxic stimuli. There are 4 known G-protein coupled adenosine receptors- A
1, A
2A, A
2B and A
3. Adenosine produces anti-inflammatory activity via A
2A receptors found in immune cells including neutrophils, macrophages, dendritic cells and platelets. In the presence of tissue injury or hypoxia, generation of adenosine is increased and adenosine receptors are upregulated [
29]. Activation of the A
2A receptor with adenosine or a specific A
2A receptor agonists inhibits recruitment of inflammatory cells and expression of inflammatory cytokines [
30]. Adenosine inhibits expression of adhesion molecules (E-selectin and vascular cell adhesion molecule-1, VCAM-1) and secretion of IL-6 and IL-8 in human endothelial cells [
31]. Indeed, it has previously been reported that intraluminal administration of A
2A agonist, ATL 313, in
C. difficile toxin A-challenged murine ileal loops decreased neutrophil infiltration as measured by myeloperoxidase activity and tissue TNFα secretion [
15].
C. difficile toxin A-induced intestinal mucosal injury, intraluminal secretion and apoptosis were all improved in ileal tissues treated with ATL 313. Our study using two different animal models (rabbit ileal and murine cecal loops) and a different adenosine A
2A receptor agonist (ATL 370) corroborated these previous findings. Interestingly, the high doses of ATL 370 (150 ng) used in this study did not offer additional improvement in histopathologic scores indicating that lower doses may be sufficient for an optimal effect. The observed effects of ATL 370 on intestinal secretion were dose-dependent and reversed by highly specific A
2A antagonist, SCH 58261, also in a dose-dependent manner suggesting the specificity of the observations to the adenosine A
2A receptor. In addition, our study showed that the anti-inflammatory, anti-secretory and anti-apoptotic effects from treatment with A
2A agonist may be enhanced by the addition of alanyl-glutamine.
The exact mechanism as to how glutamine and alanyl-glutamine (a highly soluble and stable derivative of glutamine) protect enterocytes from injury and modulate inflammatory response is unclear. Alanyl-glutamine is hydrolyzed to alanine and glutamine in the gut. Glutamine is the major oxidative energy source for enterocytes, being the building block for purine and pyrimidine nucleotide synthesis and precursor of glutathione in the gut [
32]. Under pathologic or catabolically stressful conditions, i.e. infection or injury, glutamine is observed to be depleted and thus, it is considered as a conditionally essential amino acid [
33]. Moreover, glutamine deprivation has been known to induce apoptosis in intestinal epithelial cells [
34]. The protective effect of glutamine against mucosal injury and inflammation is thought to be partly mediated by heat shock proteins [
10,
35]. More recently, glutamine has also been considered to be an agonist of peroxisome proliferator-activated receptor gamma, which belongs to the family of nuclear receptor proteins which regulates expression of inflammatory cytokines [
36]. It has also been previously shown that
C. difficile toxin A induces apoptosis by activation of caspases 3, 6, 8, and 9 and Bid, mitochondrial damage and release of cytochrome c in T84 cells [
11]. Glutamine and alanyl-glutamine inhibited activation of caspase 8 and reduced apoptosis in T84 cells and improved intestinal secretion and mucosal disruption in rabbit ileal loops challenged with
C. difficile toxin A [
12]. These findings are consistent with what we have observed where the presence of alanyl-glutamine enhanced reduction of apoptosis, inflammation, secretion and epithelial injury in ATL 370-treated,
C. difficile toxin A-stimulated ileal tissues.
The beneficial effect of combination therapy for toxin A-induced enteritis is less explored in the literature. In this study we attempted to control both epithelial disruption and inflammatory response with an adenosine A
2A receptor, ATL 370, and alanyl-glutamine. ATL 370 was delivered parenterally and glutamine intraluminally. Given the short incubation time (4-5 h) of the experiments, it is conceivable that systemically administered A
2A agonist may have acted mostly on the immune cells, specifically neutrophils, and endothelial cells, which are known to express more of the A
2A receptors than on the enterocytes, which express more of A
2B receptors [
37‐
39]. Indeed, other A
2A agonists have been shown to decrease inflammatory responses and improved survival in mouse models of endotoxemia and sepsis [
40,
41]. Several experimental studies have shown that alanyl-glutamine is at least as effective as glutamine in improving electrolyte absorption and preserving mucosal integrity against enterotoxin or chemical insult [
42‐
46]. Alanyl-glutamine enters enterocytes through PepT1 proton-coupled peptide transporters and release L-glutamine by the action of cytosolic peptidases [
47,
48]. Although glutamine may affect leukocyte-dependent inflammatory events, such as migration and release of inflammatory cytokines, in this particular study, glutamine may have caused more of the protective effect on mucosal architecture and prevention of enterocyte apoptosis than prevented recruitment of inflammatory cells. However, release of cytokines from disrupted epithelial cells contributes to recruitment of immune cells and inflammatory mediators from the later also contribute significantly to mucosal injury [
49]. These joint epithelial and immune responses to a biologic insult such as an enterotoxin, possibly explains the additive amelioration of mucosal injury, secretion, and apoptosis or even the synergistic effects on the expression of cytokines with combined treatment in this study. Whether these observations will hold true in the mouse model of
C. difficile infection remain to be seen but these preliminary findings raise the potential use of combination therapy with enteral alanyl-glutamine and systemic low-dose A
2A adenosine agonist in the management of
C. difficile-induced diarrhea.
Competing interests
CAW, GMC, YL and SWP have no competing interests. RAF is partially funded by Dogwood Pharmaceuticals, Inc. (formerly ATL, LLC). JR is employed by Dogwood Pharmaceuticals, Inc. PBE has collaboration on NIH grant with Dogwood Pharmaceuticals, Inc. JL is a consultant for Dogwood Pharmaceuticals, Inc. RLG co-founded AlGlutamine, LLC.
Authors' contributions
CAW conceptualized study design, performed animal experiments, collated and analyzed data, drafted manuscript. GMC participated in animal experiments, assisted in study design, performed protein and gene expression assays and immunohistochemistry. YL participated in animal experiments and assisted in mouse study design. SWP participated in rabbit experiments. RAF participated in reviewing data and manuscript. JR participated in reviewing data and manuscript. PBE critically reviewed data and manuscript. JML critically reviewed data and manuscript. RLG critically reviewed data and manuscript. All authors read and approved the final manuscript.