Open Access

Myrrh attenuates oxidative and inflammatory processes in acetic acid-induced ulcerative colitis

  • Authors:
    • Amal Jamil Fatani
    • Fatima Salih Alrojayee
    • Mihir Yogeshkumar Parmar
    • Hatem Mustafa Abuohashish
    • Mohammed Mahboobuddin Ahmed
    • Salim Salih Al‑Rejaie
  • View Affiliations

  • Published online on: May 26, 2016     https://doi.org/10.3892/etm.2016.3398
  • Pages: 730-738
  • Copyright: © Fatani et al. This is an open access article distributed under the terms of Creative Commons Attribution License.

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Abstract

The pathogenesis of ulcerative colitis (UC) has been associated with a weakened antioxidant capacity and increased inflammatory processes. Myrrh is traditionally used for the treatment of inflammatory diseases due to its antioxidant and anti‑inflammatory properties. The present study aimed to evaluate the effects of myrrh on an experimental rat model of UC. UC was induced in rats using acetic acid (AA) after pre‑treatment with myrrh (125, 250 or 500 mg/kg/day) or mesalazine (MES; 300 mg/kg/day) for 7 days. The levels of various inflammatory cytokines, prostaglandin E2 (PGE2) and nitric oxide (NO) in the rat colon tissues were assessed. In addition, the colonic levels of thiobarbituric acid reactive substances (TBARS) and non‑protein sulfhydryl groups (NP‑SH), as well as the activities of superoxide dismutase (SOD) and catalase (CAT), were estimated. Furthermore, total protein (TP) contents and the levels of DNA and RNA were measured, and histopathological changes in colonic tissues were analyzed. The results indicated that the levels of pro‑inflammatory cytokines, PGE2, NO and TBARS were markedly increased. By contrast, the levels of interleukin‑10, NP‑SH, TP and nucleic acids, and the enzymatic activities of SOD and CAT were significantly decreased in the AA model group. In addition, pretreatment with myrrh and MES was able to attenuate the impaired oxidative stress response and upregulation of inflammatory biomarkers. Furthermore, the enzymatic activities of SOD and CAT were near to normal in the myrrh and MES pretreated groups. The ability of myrrh to protect against UC was further confirmed by histopathological analysis, and the high dose of myrrh exerted an effect comparable to MES. In conclusion, the results of the present study suggested that myrrh has potent therapeutic value in the amelioration of experimental colitis in laboratory animals by downregulating the expression of proinflammatory mediators and improving endogenous antioxidative activities.

Introduction

Inflammatory bowel diseases (IBDs) comprise ulcerative colitis (UC) and Crohn's disease (1), both of which have a high incidence in developed countries and severely affect the quality of life of patients worldwide (2). IBDs, which are complex and multifactorial diseases caused by diverse pathophysiological mechanisms, have numerous clinical manifestations, including abdominal pain, diarrhea, blood in the stool and weight loss (1). Persistent UC has been associated with an increased risk of developing colorectal cancer by ~10-fold (3). UC is characterized by excessive inflammation and oxidative stress (4,5), which is considered a key factor in the pathogenesis and perpetuation of mucosal damage. Pro-inflammatory cytokines are secreted by macrophages and are responsible for the generation of reactive oxygen species (ROS), which activate the oxidative stress response and thus serve a vital role in the development and maintenance of IBD (6,7). It has been demonstrated that oxidative injury results from the overproduction of free radicals, which leads to the lipid peroxidation (LPO) of membranes and the impairment of cellular proteins and nucleic acids (8). In addition, the generation of ROS and subsequent LPO reduces the cellular antioxidant capacity, which may lead to colonic inflammation (5).

Nitric oxide (NO), an intracellular mediator released by inducible nitric oxide synthase, is able to interact with free radicals to precipitate tissue damage (9). Prostaglandin E2 (PGE2) is a pro-inflammatory mediator in the colon, and its upregulation has been associated with the inflammatory process (10). Various murine models of colitis have been developed over the past 20 years and are indispensable tools for elucidating the mechanisms underlying IBD pathogenesis, as well as for assaying potential therapeutics (11). The acetic acid (AA)-induced colitis model, which is similar to human UC in terms of its histological features, has been widely used to investigate the effects of various herbal therapies on experimental colitis (12,13).

The genus Commiphora (Burseraceae), which includes >150 plant species, is distributed in the tropical and subtropical regions, in particular within northeastern Africa, southern Arabia and India (14). Commiphora molmol Engl. is the main plant used in the production of myrrh, which is a oleo-gum-resin (OGR) made from dried tree sap that is traditionally used as a perfume, incense or embalming ointment (15). Previous studies have reported the beneficial effects of myrrh, which include anti-inflammatory, antispasmodic, antirheumatic, antipyretic, antiseptic and antihistaminic properties (1618). In addition, purified metabolites of myrrh crude extracts have been investigated for antiproliferative, antimicrobial, hepatoprotective and cardiovascular properties (19). Experimentally, myrrh has demonstrated antigastric ulcer (20), anti-oxidative, cytotoxic and non-mutagenic properties in various studies (21,22). Su et al (23) reported that myrrh significantly inhibited the production of PGE2 in carrageenan-induced paw edema in mice and exhibited potent anti-inflammatory effects. Therefore, the present study aimed to evaluate the ability of myrrh to protect against AA-induced UC in a rat model by measuring potential oxidative markers and inflammatory mediators known to damage the colonic tissues.

Materials and methods

Animals

The current study was performed using 36 male Wistar albino rats (age, 12 weeks; weight, 250–280 g) that were obtained from the Experimental Animal Care Center of King Saud University (Riyadh, Saudi Arabia). The rats were maintained at 25°C under a 12-h light/dark cycle with ad libitum access to Purina rat chow (Grain Silos and Flour Mills Organization, Riyadh, Saudi Arabia) and water. All experimental and euthanasia procedures were performed in accordance with the National Institute of Health Guide for the Care and Use of Laboratory Animals (NIH Publications No. 80–23; 1996), as well as the Ethical Guidelines of the Experimental Animal Care Center of King Saud University.

Plant material and phytochemical screening

Authenticated myrrh was purchased from the local market in Riyadh, Saudi Arabia. For the purpose of maintaining experimental institutional records, the voucher specimen of the myrrh OGR was housed in the Herbarium at the College of Pharmacy of King Saud University. Chemical tests to identify the constituents of myrrh were performed using the aqueous extract, according to a standard procedure (24,25). A yield of 9.72% essential oil was obtained by steam distillation (23.17%) from the volatile oil. The presence of terpenes, sesquiterpenes, ester, cuminic, aldehyde and eugenol was detected.

Chemicals

Mesalazine (MES) was obtained from Shire (Lexington, MA, USA). The thiobarbituric acid reactive substances (TBARS) assay kit (0801192) was purchased from ZeptoMetrix Corp. (Buffalo, NY, USA). Tumor necrosis factor-α (TNF-α; RTA00), interleukin (IL)-1β (RLB00), IL-6 (R6000B), IL-10 (M1000B), PGE2 (KGE004B) and NO (KGE001) ELISA kits were purchased from R&D Systems, Inc. (Minneapolis, MN, USA). All other chemicals used were of analytical reagent grade.

Experimental procedure

The rats were randomly allocated into five groups (6 rats per group), as follows: i) Control; ii) AA model; iii) myrrh (125 mg/kg/day) plus AA; iv) myrrh (250 mg/kg/day) plus AA; v) myrrh (500 mg/kg/day) plus AA; and vi) MES (300 mg/kg/day) plus AA. MES was used as a positive control against which to compare the effect of myrrh on UC. Pretreatment with myrrh or MES was conducted for 7 consecutive days by gavage. The doses used in the present study were selected based on an earlier study (20). At 24 h after the final treatment, UC was induced in all AA groups by administration of AA. After 1 day, the rats were sacrificed by decapitation under deep ether anesthesia (10 ml/l air), and 5–6-cm specimens of the rat colons were dissected, washed with saline solution and weighed. A small 5-µm-thick cross section of the colon tissue from each group was fixed in 10% formaldehyde solution for histopathological analysis. The remaining colonic tissues were maintained at −75°C for biochemical analysis.

Induction of UC

Experimental induction of UC in the rat colons was performed according to a previous study (26), with minor modifications. Briefly, the rats were transrectally administered 2 ml 4% AA solution (v/v; Merck Millipore, Darmstadt, Germany) under light ether anesthesia (5 ml/l air)using a 2.7-mm soft pediatric catheter. Following AA administration, the rats were held horizontally for 2 min to prevent AA leakage. The control rats underwent the same procedure using an equal volume of normal saline instead of AA solution.

Analysis of the adherent colonic mucus concentration

The concentration of colon adherent mucus was estimated according to a method described previously (27). Briefly, small 5-µm-thick sections of the rat colonic tissues were transferred immediately following weighing to a mixture of 1% Alcian blue and 0.16 mol/l sucrose solution (pH 5) for 24 h. The sucrose solution was used to rinse the excess dye, after which the dye bound to the colonic wall mucus was extracted using 0.5 mol/l MgCl2 and mixed with diethyl ether (1:1 ratio). The sample was then centrifuged at 1,800 × g for 15 min at room temperature and the absorbance of the aqueous layer was detected at 580 nm using a Pharmacia-LKB UV-M II spectrophotometer (GE Healthcare Life Sciences, Marlborough, MA, USA) and a standard curve. Subsequently, the quantity of Alcian blue extracted in µg/g of the wet colon was determined.

Determination of MDA levels in the rat colons

The levels of malondialdehyde (MDA), an LPO product, in the rat colon tissues were detected using the TBARS assay kit. Briefly, 100 µl colon tissue homogenate was mixed with 2.5 ml kit reaction buffer, followed by heating at 95°C for 1 h. The sample was left to cool, centrifuged at 1,800 × g for 15 min at room temperature, and then a Pharmacia-LKB UV-M II spectrophotometer was used to measure the absorbance of the supernatant at 532 nm using a standard curve. The MDA levels in the colonic tissue are expressed in terms of nm/mg protein.

Determination of non-protein sulfhydryl groups (NP-SH) concentration in the rat colons

The colonic concentration of NP-SH was determined according to the method described by Sedlak and Lindsay (28). Briefly, the homogenate was mixed with 1 ml 50% trichloroacetic acid (TCA), followed by intermittent shaking for 10–15 min and centrifugation at 1,350 × g for 15 min at room temperature. The supernatant was mixed with 0.4 mol/l Tris buffer (pH 8.9) in a ratio of 1:2, followed by the addition of 0.1 ml DTNB. The absorbance of the mixture was measured within 5 min at 412 nm using a Pharmacia-LKB UV-M II spectrophotometer and a standard curve.

Determination of superoxide dismutase (SOD) and catalase (CAT) activities in the rat colons

To obtain the post-mitochrondrial supernatant, 200 mg colon tissue was homogenized in 2.0 ml of 50 mM phosphate buffered saline (pH 7.4) using a Pyrex glass pestle tissue grinder. Homogenates were centrifuged at 1,000 × g for 10 min at 4°C to separate the nuclei and unbroken cells. Pellets were discarded and the supernatant was again centrifuged at 12,000 × g for 20 min at 4°C. The enzymatic activity of the antioxidant enzyme SOD was measured in the post-mitochondrial supernatant of the colon homogenate according to a previous study by Kono (29). Briefly, superoxide anions generated by hydroxylamine hydrochloride oxidation mediated the reduction of nitro-blue tetrazolium to a blue formazan, which was then measured at 560 nm under aerobic conditions. SOD is known to inhibit nitro-blue tetrazolium reduction, and thus the extent of inhibition was used as a measure of SOD activity, which is expressed as units/mg protein (30). The enzymatic activity of CAT was measured using a method described previously (31). Briefly, the post-mitochondrial supernatant of the colon homogenate was mixed with 50 mmol/l phosphate buffer (pH 7.0) and 20 mmol/l H2O2. The enzymatic activity of CAT was then determined according to the decrease in absorbance at 240 nm, and is expressed in terms of units/mg protein.

Determination of DNA, RNA and total protein (TP) levels in the rat colons

The DNA and RNA concentrations in the rat colon tissues were estimated according to a previously described method by Bregman (32). Briefly, the homogenized colon tissues were suspended in 5 ml of 10% ice-cold TCA, after which the samples were centrifuged at 450 × g for 3 min at room temperature and the resulting pellets were extracted twice using 95% ethanol. Next, the nucleic acid content was extracted using 5% TCA. For DNA quantification, diphenylamine reagent was added to the extracts, and the resulting blue color was measured at 600 nm. For RNA determination, orcinol reagent was added to the extracts and the intensity of the green color was measured at 660 nm. In addition, the Lowry method (33) was used to determine the TP content in the colon tissues, using bovine plasma albumin (BDH Chemicals, Poole, UK) as a standard.

Determination of levels of inflammatory biomarkers in the rat colon tissues

The levels of TNF-α, IL-10, IL-1β, IL-6, PGE2 and NO in the rat colon tissues were determined using ELISA kits, according to a previous study by Mousavizadeh et al (26). The results are expressed as pg/mg protein.

Histopathological analysis of UC

Cross sections of the rat colon tissues were fixed in 10% formaldehyde solution, embedded in paraffin wax blocks and cut into 5-µm sections using a microtome. Samples were then stained with hematoxylin and eosin, mounted and observed under a light microscope. Histopathological sections were graded with scores of 0–4 according to inflammatory cellular infiltration, surface ulceration and necrosis, edema and hyperemia, and goblet cell hyperplasia. The scores demonstrated the percentage of damage or active changes, as follows: Score of 1, <25%; score of 2, <50%; score of 3, <75%; and score of 4, >75% damage or active changes. The total score for the degree of colonic inflammation was determined, as follows: <4, minimal inflammatory changes; 4–8, mild inflammatory changes; 9–12, moderate inflammatory changes; and 13–16, severe inflammatory changes.

Statistical analysis

Data are expressed as the mean ± standard error of the mean. Statistical analyses involved one-way analysis of variance followed by Student-Newman-Keuls post-hoc test, and were performed using GraphPad Prism software, version 5 (GraphPad Software, Inc., La Jolla, CA, USA). P<0.05 was considered to indicate a statistically significant difference.

Results

Effect of myrrh on colon weight/length ratio and mucus content in rats with AA-induced UC

The mean colonic weights were significantly increased in the AA group, as compared with the control group (P<0.01). As shown in Fig. 1A, 7 days of pretreatment with various doses of myrrh or 300 mg/kg/day MES resulted in a significant decline in the mean colon weights, as compared with the AA group (P<0.01). In addition, the rat colon mucus content was significantly decreased in the AA group, as compared with the control group (P<0.01). Pretreatment with a higher dose of myrrh (500 mg/kg/day) or 300 mg/kg/day MES significantly increased the mucus content of the rat colons, as compared with the AA group (P<0.05; Fig. 1B). These results suggest that myrrh has an anti-inflammatory and protective role against colon weight increase and gastric mucus depletion.

Effect of myrrh on the colonic levels of inflammatory cytokines in AA-induced UC rats

In the AA group, the levels of the pro-inflammatory cytokines TNF-α, IL-1β and IL-6 were significantly increased, while the levels of the anti-inflammatory cytokine IL-10 were significantly decreased, as compared with the control group (all P<0.01; Fig. 2). In the 250 and 500 mg/kg/day myrrh and MES pretreated groups, the levels of TNF-α, IL-1β and IL-6 were significantly decreased, as compared with the AA group (P<0.05 and P<0.01). However, in the 125 mg/kg/day myrrh group, only the levels of TNF-α and IL-1β, but not IL-6, were significantly decreased, as compared with the AA group. Furthermore, the levels of IL-10 were significantly increased in the 250 and 500 mg/kg/day myrrh and MES pretreated groups, as compared with the AA group (P<0.05; Fig. 2). These results demonstrated the anti-inflammatory property of myrrh, as myrrh pretreatment inhibited the expression of colonic proinflammatory cytokines.

Effect of myrrh on the colonic levels of TBARS and NP-SH, and on the activities of SOD and CAT in AA-induced UC rats

At 24 h following AA administration, TBARS levels were significantly increased in the AA group, as compared with the control rats (P<0.01). However, pretreatment with 250 and 500 mg/kg/day myrrh or with MES resulted in a significant decline in TBARS levels, as compared with the AA group (P<0.01; Fig. 3A). In addition, the levels of NP-SH were significantly decreased in the colon tissues of AA group rats, as compared with the control group (P<0.01). By contrast, the levels of NP-SH were significantly increased in rats pretreated with high doses of myrrh (250 and 500 mg/kg) or 300 mg/kg MES, as compared with the AA group rats (P<0.05; Fig. 3B). The results also indicated that the activities of the antioxidative enzymes SOD and CAT were significantly inhibited in the colons of AA-treated rats, as compared with those in control rats (P<0.01). Pretreatment with 500 mg/kg/day myrrh and MES resulted in significant increases in SOD and CAT activities, as compared with the AA group (P<0.05; Fig. 3C and D). These results demonstrated the antioxidative effect of myrrh, as myrrh pretreatment induced a marked reduction in TBARS levels, increased NP-SH and enhanced the enzymatic activities of SOD and CAT.

Effect of myrrh on colonic levels of nucleic acids and TP content in AA-induced UC rats

The levels of DNA, RNA and TP in the rat colon tissues were significantly decreased in the rats administered AA, as compared with the control rats (P<0.01). Pretreatment with myrrh (500 mg/kg) and MES resulted in significant increases in the levels of DNA (P<0.01), RNA (P<0.01) and TP (P<0.05), as compared with the AA group (Table I). These dose-dependent improvements in nucleic acid levels demonstrated the cytoprotective effects of myrrh.

Table I.

Effect of myrrh on the colonic levels of DNA, RNA and TP in rats with AA-induced ulcerative colitis.

Table I.

Effect of myrrh on the colonic levels of DNA, RNA and TP in rats with AA-induced ulcerative colitis.

GroupDNARNATP
Control 524.7±33.03 360.8±31.12 3.4±0.22
AA 192±20.38a 159.1±20.75a 1.31±0.19a
Myrrh (mg/kg/day)
  125 288.6±56.64 194.9±27.09 1.62±0.25
  250 359.3±51.33 225.3±17.13 1.9±0.25
  500 467.6±57.67b 309.7±33.51b 2.82±0.33c
MES (300 mg/kg/day) 473.7±76.87b 345.2±43.07b 2.96±0.3c

{ label (or @symbol) needed for fn[@id='tfn1-etm-0-0-3398'] } Data are expressed as the mean ± standard error of the mean (n=6) and were analyzed using one-way analysis of variance followed by Student-Newman-Keuls multiple comparisons test.

a P<0.01 vs. the control group

b P<0.01

c P<0.05 vs. the AA group. TP, total protein; AA, acetic acid; MES, mesalazine.

Effect of myrrh on colonic levels of PGE2 and NO in AA-induced UC rats

PGE2 and NO levels were significantly increased in the colonic cells of rats administered AA, as compared with the control rats (P<0.01). After 7 days of pretreatment with myrrh (500 mg/kg) or MES, a significant decrease was observed in the levels of PGE2 and NO in rat colon tissues, as compared with those in the AA group (P<0.05; Fig. 4). These results suggested the anti-inflammatory potential of myrrh, as myrrh pretreatment induced a marked inhibition of the elevated levels of PGE2 and NO in colon tissue.

Effect of myrrh on histopathological changes in the colons of AA-induced UC rats

As shown in Table II and Fig. 5, a histopathological analysis of rat colon sections revealed minimal inflammatory cell infiltration, surface necrosis and ulceration, as well as no evidence of edema, hyperemia or goblet cell hyperplasia, in the colons of the control group rats. Therefore, the clinical diagnosis was unremarkable pathological changes (Fig. 5A). Conversely, histopathological analysis in the AA group demonstrated diffused severe inflammatory cell infiltration with marked surface ulceration, necrosis, edema and hyperemia, as well as moderate goblet cell hyperplasia, and the clinical diagnosis was diffused severe inflammatory changes (Fig. 5B). Myrrh pretreatment appeared to exert a dose-dependent effect on the AA-induced histopathological changes in the rat colons. In rats pretreated with 125 mg/kg/day myrrh, diffuse moderate inflammatory cell infiltration with focal moderate surface ulceration, necrosis, edema and hyperemia, as well as mild focal goblet cell hyperplasia, were observed, and the clinical diagnosis was focal moderate inflammatory changes (Fig. 5C). In the 250 mg/kg/day myrrh group, diffused mild inflammatory cell infiltration with focal surface necrosis and ulceration and moderate edema and hyperemia, as well as mild goblet cell hyperplasia, were observed, and the clinical diagnosis was focal mild inflammatory changes (Fig. 5D). In the 500 mg/kg/day myrrh group, the analysis revealed diffused mild inflammatory cell infiltration with minimal edema and hyperemia, with the absence of surface necrosis, ulceration and goblet cell hyperplasia. The clinical diagnosis for the 500 mg/kg/day myrrh group was diffused minimal inflammatory changes (Fig. 5E). Similarly, pretreatment with 300 mg/kg/day MES resulted in minimal focal inflammatory changes, necrosis, ulceration, edema, hyperemia and goblet cell hyperplasia. The clinical diagnosis of this group was diffused minimal inflammatory changes (Fig. 5F).

Table II.

Effect of myrrh on histopathological changes in the colonic tissues of rats with AA-induced ulcerative colitis.

Table II.

Effect of myrrh on histopathological changes in the colonic tissues of rats with AA-induced ulcerative colitis.

GroupInflammatory cell infiltrationSurface ulceration and necrosisEdema and hyperemiaGoblet cell hyperplasiaTotal score
Control00000
AA444315
Myrrh (mg/kg/day)
  12533219
  25022228
  50020103
MES (300 mg/kg/day)11103

[i] Sections were scored for inflammatory cell infiltration, surface ulceration and necrosis, edema and hyperemia and goblet cell hyperplasia, as follows: 1, <25% damage or active changes; 2, <50% damage or active changes; 3, <75% damage or active changes; and 4, >75% damage or active changes. A total score of <4 indicated minimal inflammatory changes, a score of 4–8 indicated mild inflammatory changes, a score of 9–12 indicated moderate inflammatory changes and a score of 13–16 indicated severe inflammatory changes. AA, acetic acid; MES, mesalazine.

Discussion

The present study aimed to investigate the protective effects of myrrh in a rat model of AA-induced UC. The AA-induced UC model, which is similar to human UC in terms of histological features, has been used in various previous studies (12,34). The histopathological analysis performed in the present study demonstrated that AA treatment resulted in disruption of the entire colonic mucosa, erosion, ulceration, congestion, inflammation and necrosis. Pretreatment with myrrh at three different doses (125, 250 or 500 mg/kg/day) for 7 days was shown to preserve the functional cytoarchitecture of the colon to varying extents. In addition, myrrh markedly protected against AA-induced loss of the colonic mucosal content and prevented colonic oxidative and inflammatory responses to AA in a dose-dependent manner. The present study also compared the anti-ulcerogenic effect of myrrh with a standard drug, MES. The effect of MES pretreatment was similar to that observed for the 500 mg/kg/day myrrh pretreatment.

Under normal physiological conditions, the mucosa of the colon contains relatively low levels of endogenous antioxidants. Oxidative stress may inhibit the endogenous defense systems that regulate ROS production (35). High levels of ROS lead to oxidative stress and DNA damage due to an imbalance between innate and exogenous antioxidants and ROS (36,37). In addition, it may promote the infiltration of leukocytes into the damaged area, the rupture of the colonic barrier, and the release of inflammatory mediators, including cytokines and arachidonic acid metabolites (38,39). In the present study, the rectal administration of AA significantly increased the weight of the rat colon, and this was associated with severe tissue ulceration, inflammatory cell infiltration, necrosis and goblet cell hyperplasia, as demonstrated by the histopathological analysis. These results are consistent with those reported in previous studies using the same animal model (40,41). Defects in the colonic mucosal barrier and functions are among the etiological factors that characterize IBDs (42). In the present study, the protective colonic mucus was markedly altered by AA, which is in line with earlier studies conducted in our labs (43,44). Pretreatment with myrrh at various doses for 7 days significantly reduced the colon weight and inhibited colonic wall mucus depletion.

Oxidative stress is known to serve a major role in the initiation and progression of IBD (45,46). A previous study reported vascular dilatation and white blood cell accumulation in an AA-induced model of IBD, which was associated with an increased blood flow and production of ROS (47). ROS attack cellular macromolecules, thereby disrupting epithelial cell integrity and hindering mucosal recovery, in particular in patients with an impaired endogenous defense system (48). Furthermore, the superoxide anion radical, hydrogen peroxide and hydroxyl radicals, which are secreted by neutrophils and phagocytes, accumulate in the inflammatory lesion, leading to destabilization of the cell membrane, cell death via LPO, and damage to tissue proteins and DNA (49,50). TBARS, which are markers of LPO, interact with DNA and proteins leading to pathological changes (51). The present study demonstrated that myrrh was able to significantly reduce the levels of TBARS in the colonic tissues of rats administered AA, thereby disrupting the feedback loop and attenuating damage to colonic tissues. Endogenous antioxidants, such as NP-SH, and antioxidant enzymes, including SOD and CAT (52), serve a major role in preventing excessive free radical generation under pathogenic conditions. In the present study, the concentration of NP-SH and the activities of SOD and CAT were significantly reduced in the colon tissues of AA-treated rats. In addition, the levels of critical cellular macro- and micro-molecules, including nucleic acids and proteins, were decreased in the AA group rats. These results were consistent with our previous findings (43,44), and indicated that AA was able to exert harmful effects on cellular macromolecules, impair epithelial cell integrity and hinder mucosal recovery.

IBD is a complex multi-factorial intestinal inflammatory disease, involving immunological, genetic and environmental factors (53). Pro-inflammatory mediators are able to modulate the mucosal immune system and disrupt the epithelial integrity by promoting the infiltration of neutrophils and macrophages (54). The migration of granulocytes and other leukocytes to the inflamed mucosa and superficial ulcers results in the overproduction of pro-inflammatory cytokines (55,56), which is an indicator of the disease severity. In the coordinated network of inflammatory response, TNF-α serves an important signaling role in the inflammatory cascade following its secretion. Specifically, it activates monocytes, macrophages and intestinal immune cells in order to produce PGE2, proteases and chemotactic cytokines (57). IL-6 is a pleiotropic cytokine that has a central role in immune regulation and inflammation (58). IL-6-activated macrophages and colon epithelial cells secrete inflammatory cytokines, including TNF-α and IL-1β, that contribute to the development of colitis (59). In the present study, the levels of IL-1β, TNF-α, IL-6, NO and PGE2 were significantly increased in colon tissues of AA-treated rats. These results suggested that the colons of the AA-treated rats were inflamed, which was supported by the histopathological results. In addition, these results were consistent with those of previous experimental and clinical studies (27,40,60,61).

In accordance with previous studies (62,63), the antioxidant effects of myrrh were also demonstrated in the present study. The levels of NP-SH and the activities of SOD and CAT in rat colonic tissues were increased in myrrh-treated rats in a dose-dependent manner, with higher myrrh doses resulting in a greater effect. The cytoprotective and antioxidant effects of myrrh demonstrated in the present study may have been due to the presence of several pharmacologically active constituents. The distribution of 51 constituents and medical applications of Commiphora were reviewed in 2003 by El Ashry et al (19). myrrh contains volatile oil, which in turn consists of heerabolene, a-cadinene, elemol, eugenol, cuminaldehyde, terpenes (such as furanodiene, furanodienone, curzerenone, lindestrene, 2-methoxyfuranodiene and 3-epi-alpha-amyrin), and various other compounds (64). In addition, myrcene, a-camphorene and various steroids, including Z-guggulsterol and guggulsterol I, II and III, have been detected (65), while a previous study reported that tannins were also found in myrrh (66). Therefore, these antioxidative constituents may, at least in part, be responsible for the protective effect of myrrh pretreatment against AA-induced UC. Furthermore, the anti-inflammatory properties of myrrh have previously been reported (67). Consistent with this, the present study observed that AA treatment resulted in a marked reduction in the colonic levels of pro-inflammatory cytokines, including IL-1β, IL-6 and TNF-α, which are principally responsible for causing oxidative damage (68). Therefore, it may be hypothesized that the anti-inflammatory effects of myrrh are regulated by its antioxidative activities.

In conclusion, the results of the present study provided support for the beneficial effects of myrrh against AA-induced experimental colitis. The protective properties of myrrh may be attributed to its ability to inhibit free radical production and potentiate the endogenous enzymatic or nonenzymatic antioxidant system. Furthermore, myrrh was shown to decrease the levels of inflammatory mediators, thus suggesting that it may have a role as an anti-inflammatory compound. The results of the present study suggest that myrrh may be a promising novel candidate compound for the treatment of IBDs.

Acknowledgements

The present study was supported by the Deanship of Scientific Research at King Saud University (grant no. RGP-VPP-103).

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Spandidos Publications style
Fatani AJ, Alrojayee FS, Parmar MY, Abuohashish HM, Ahmed MM and Al‑Rejaie SS: Myrrh attenuates oxidative and inflammatory processes in acetic acid-induced ulcerative colitis. Exp Ther Med 12: 730-738, 2016
APA
Fatani, A.J., Alrojayee, F.S., Parmar, M.Y., Abuohashish, H.M., Ahmed, M.M., & Al‑Rejaie, S.S. (2016). Myrrh attenuates oxidative and inflammatory processes in acetic acid-induced ulcerative colitis. Experimental and Therapeutic Medicine, 12, 730-738. https://doi.org/10.3892/etm.2016.3398
MLA
Fatani, A. J., Alrojayee, F. S., Parmar, M. Y., Abuohashish, H. M., Ahmed, M. M., Al‑Rejaie, S. S."Myrrh attenuates oxidative and inflammatory processes in acetic acid-induced ulcerative colitis". Experimental and Therapeutic Medicine 12.2 (2016): 730-738.
Chicago
Fatani, A. J., Alrojayee, F. S., Parmar, M. Y., Abuohashish, H. M., Ahmed, M. M., Al‑Rejaie, S. S."Myrrh attenuates oxidative and inflammatory processes in acetic acid-induced ulcerative colitis". Experimental and Therapeutic Medicine 12, no. 2 (2016): 730-738. https://doi.org/10.3892/etm.2016.3398