Anti-ulcerogenic Evaluation of Gloriosa Superba Tuber Extracts In-vivo and Anthelmintic Activity In-vitro: A Comparison.

Abstract

Gloriosa Superba(Liliaceae) is a semi-woody herbaceous climber native of tropical Asia, Africa and reported by tribal people of India for its several clinical uses. Traditionally, the tubers and other parts of the plant are widely being used in the treatment of ulcers, piles, inflammation, abdominal pain, infertility, parasitic skin infections and leprosy. The present study was carried out to investigate the antiulcerogenic activity of ethanolic extract of Gloriosa superba L. tuberous rhizomes (GST) and compare with Zingiber officinale (rhizomes) and Glycyrrhiza glabra (roots) ethanolic extracts on experimental ulcers induced by aspirin (chemically induced ulcers) couple with stress and on pylorus ligation-induced ulcers in Wistar rats. The anthelmintic activity of various extracts of GST was also evaluated in vitro against two types of intestinal worms; a) Earthworms and b) Ascardia Galli (a parasitic roundworm). Test extracts were administered orally 60 and 30 min before for aspirin and pylorus ligation-induced ulcer models respectively. GST extract showed superior protection when compared with other test extracts on both the ulcer models tested. The extract significantly increased the pH and decreased both the volume and total acidity ofgastricsecretion in pylorus ligation-induced ulcer model. The antiulcerogenic effect exhibited by GST extract was comparable with ranitidine (standard drug) in particular at higher dose. Aqueous, alcoholic and chloroform extracts of GST showed significant anthelmintic activity in vitro against both types of intestinal worms. Therefore, the results indicate that the herbal preparations containing GST would be beneficial to treat gastric ulcers more effectively for improved clinical outcome.

Keywords

Gloriosa, gastric ulcer, pylorus ligation,Zingiber,Glycyrrhiza, anthelmintic

Introduction

Gloriosa Superba(Liliaceae) is a semi-woodyherbaceousclimber native of tropical Asia and Africa. Several parts of the plant were used traditionally by tribal people for the treatment of various diseases [1-3]. It is known as ‘Malabar glory lily’ in English, ‘Agnisikha’ in Sanskrit and its trade name is ‘Glory lily’ [4-6]. Glory lily is an industrial medicinal crop in South India because of its high colchicine content and potential long list of reported clinical uses. Glory lily is one of the most valued medicinal plants, due to its over-exploitation is on the verge of extinction [7,8]. Both its tuber and seeds have similar medicinal properties [9].

Traditionally the tubers and other parts of the plant are widely being used in the treatment of ulcers, piles, inflammation, abdominal pain, bruises, parasitic skin infections, infertility, leprosy and as anthelmintic and laxative [2,3]. In Folklore it is being used to treat pimples, skin eruptions, baldness, killing lice in the hair and also as sedative [10,11].

Aspirinis well known for its undesirable side effects mainly inducing gastrointestinal ulcers and bleeding in stomach especially at higher doses. The induction of gastric damage by aspirin is due to activated macrophages and characterized by infiltration of neutrophils, growth factor inhibition and elevation of cytokines [12,13].Cytokinessuch as tumor necrosis factor-alpha (TNF-α), interleukin-6 (IL-6) and interleukin-10 (IL-10) play important roles in the acute phase inflammation as well as in maintenance and regulation of the severity of gastric ulcer [14]. Extreme mental and psychological stresses to rodents, stimulates gastric secretion related to central nervous system as well as pituitary renal hormonal axis [15-18]. Long-term pylorus ligation induces retention of gastric acid secreted by cholinergic activation and stimulates activity of pepsin, resulting in gastric wall injury [16,17,19].

胃溃疡是由荷兰国际集团(ing)产生严重伤害estion of spicy food or alcohol, due to extremestressor gastric surgery and Helicobacter (H.) pylori [17]. The enzyme H+/K+-ATPase pumps protons in exchange for potassium ions across the apical membrane to secrete gastric acid by parietal cells [19]. Histamine antagonists including cimetidine and ranitidine as well as proton pump inhibitors such as omeprazole and lansoprazole are well known effective drugs for the treatment of gastric ulcers by decreasing the gastric secretions [17].

The objective of this study was to investigate theGloriosa superbaL tuber (GST) ethanolic extract for its anti-ulcerogenic activity and compare withZingiber officinale(rhizomes) andGlycyrrhiza glabra(roots) ethanolic extracts in aspirin induced ulcers coupled with stress and pylorus ligation-induced ulcer models after per oral administration to male Wistar rats.Zingiber officinale[20,4] andGlycyrrhiza glabra[7,21,22] were selected in this study for comparison of their anti-ulcerogenic activity based on the published literature. Anthelmintic activity of aqueous, ethanolic and chloroform extracts of GST was also investigatedin vitroagainst two types of intestinal worms. Ranitidine and piperazine citrate was selected as standard drugs for the evaluation of antiulcerogenic activityin vivoand anthelmintic activityin vitrorespectively.

Materials and Methods

Plant material

The tubers ofGloriosa superba(Liliaceae) were obtained and authenticated by Dr. K. Madhava Chetty, Department of Botany, Sri Vankateshwara University, Tirupati, India. Rhizomes ofZ. officinaleand roots ofG. glabrawere collected from different regions of India and authenticated by Prof. Raju of Kakatiya University, Warangal, India. All the voucher specimens have been deposited at the department of botany herbarium, Vaagdevi College of Pharmacy, Warangal, India. The collected tubers, rhizomes and roots were washed, cut in to small pieces, air dried in the shade, reduced to fine powder, packed in tightly closed containers and stored at room temperature for subsequent extraction and pharmacological evaluation.

Drugs and chemicals

Ranitidine, Aspirin and Piperazine citrate were purchased from Dr. Reddy’s Laboratories Pvt. Ltd., India. Gum acacia, sodium carboxymethylcellulose, ethanol,chloroform, Whatmann filter papers were purchased from E. Merck India Pvt. Ltd. MilliQ water from MilliQsystem (Millipore, France) was used throughout the study.

Preparation of test extracts

The extracts of G. superba (tubers),Z. officinale(rhizomes) andG. glabra(roots) were prepared using shade dried and coarsely powdered materials by cold maceration extraction process using ethanol as solvent. Each plant material (100 g) was soaked in 500 ml of ethanol in stoppered glass container for 72 hours with intermittent shaking at room temperature and then filtered through Whatmann filter paper no. 41. The last traces of the solvent was removed and concentrated to dryness under vacuum by using a rotary evaporator. The dried extracts were stored in a refrigerator until use. The extracts were suspended in aqueous 1.0 % w/v sodium carboxymethylcellulose before administration to the test animal. Aqueous and chloroform extracts of G. superba (tubers) were prepared by following the above procedure.

Animals

Male Wistar rats weighing 160 to 200 g were purchased from Mahaveer Enterprises, Hyderabad, India. Animals were housed in a room maintained at 22 ± 2 °C with an alternating light-dark cycle. Food and water were available adlibitum. All the animals were acclimatized to laboratory conditions for 7 days when they are out from quarantine. All the procedures described were reviewed and approved by the Institutional Animals Ethics Committee, Vaagdevi College of Pharmacy, Kakatiya University, Warangal, Andhra Pradesh, India and conducted as per the guidelines provided by CPCSEA (Committee for the Purpose of Control and Supervision on Experiments on Animals).

Experimental procedures

Restraint plus aspirin induced gastric ulcers

Male Wistar rats weighing 160 – 200 g were divided into eight groups, each group comprising of six rats. Animals were deprived of food for 24 h with access to water ad-libitum. After 24 h, test compounds were administered by p.o. route and 60 min after test compound administration aspirin (50 mg/kg, 10.0 mL/kg) was administered in 1.0 % carboxymethylcellulose sodium (Sodium CMC) by p.o. route. The doses of G. superba (7.5, 3.75 mg/kg);Z. officinale(700, 350 mg/kg);G. glabra(250,100 mg/kg), ranitidine (30 mg/kg) were selected from the published results. Gloriosa was tested only at low doses considering possible toxicity of colchicine. All the animals were returned to their cages, and after 30 minutes, they were subjected to manual restraint. Rats were subjected to restraint by placing them individually in a piece of galvanized steel window screen that is molded tightly around and held with adhesive tapes so that the animals cannot move. After 6 hours of restraint, all the animals were sacrificed under ether anesthesia followed by decapitation and the stomachs were cut opened through the greater curvature and tissues were rinsed with saline and examined by 5-fold binocular magnifier to assess the ulcer formation. The number of ulcers was counted and scoring was done as per the reported methods [23-25].

0.0 - Normal stomach, 0.5 - Pink or Red coloration of stomach, 1.0 - Superficial ulcer, 1.5 - Spot ulcer, 2.0 - Hemorrhage spot, 2.5 - Scattered Hemorrhage streak, 3.0 - Bleeding ulcer, 4.0 - Perforated ulcer.

Ulcer index was calculated using the formula

U_I= U_N+U_S+ U_P× 10^-1

Where U_I- Ulcer index, U_N- Avg. no. of ulcer’s/ animal, U_S- Avg. of severity score,

U_P- Percentage of animals with ulcers.

And the inhibition percentage was calculated by the formula

% of inhibition = [(U_Icontrol – U_Itreated) / (U_Icontrol)] × 100[26-28]

Gastric secretion in Pylorus ligated rats

Male Wistar rats weighing 160 - 200 g were divided into nine groups, each group comprising six rats. Group-I received vehicle (sodium CMC, 10 mL/kg), Group-II and Group-III received G. superba at 7.5, 3.75 mg/kg dose; Group-IV and Group-V receivedZ. officinaleat 700, 350 mg/kg dose; Group-VI and Group-VII receivedG. glabraat 250,100 mg/kg dose respectively and Group-VIII received ranitidine at 30 mg/kg dose. Test extracts and ranitidine was administered orally for three consecutive days 3 hours prior to the aspirin administration (50 mg/kg) suspended in 1.0 % sodium CMC.

Animals were fasted for 24 h after the last dose, 24 h later all the rats were subjected to ligation of the pylorus by opening their abdomen from midline incision. The pylorus connected to duodenum was ligated, and the peritoneum and skin were sutured [29-31]. The animals were sacrificed 4 hours after pylorus ligation, and their stomachs were removed after clamping the esophagus. The gastric contents were collected into centrifuge tube and centrifuged @ 5000 rpm for 5.0 min. The pH, volume of gastric secretion from each animal was precisely measured and volume was reported as mL/100 g body weight. While the total acidity of the gastric secretions was determined by titrating the undiluted gastric juice with 0.01N NaOH using phenolphthalein as an indicator and expressed as μEq/l.

Anthelmintic activity

Test worms collection and authentication

Adult earthworms (Pheretima posthuma), roundworms (Ascardia galli) were used to evaluate anthelmintic activityin vitro．印度成人蚯蚓从月收集t soil of the vermiculture plants and washed with normal saline to remove all the fecal and soil matter, while roundworms were collected from freshly slaughtered fowls infested intestines. The intestines were washed with normal saline solution to remove all the fecal matter, dissected; worms were collected and kept in normal saline solution. The average length of earthworm was 6-8 cm and round worm was 5-7 cm. The collected worms were authenticated by experts in the Department of Zoology, Kakatiya University, Warangal and also verified by veterinary practitioners, Warangal, India.

Test sample preparation forin vitroassay

Test samples forin vitrostudy were prepared by suspending each extract in ~1.0 % of dimethylformamide (DMF) and the volume was adjusted with normal saline to obtain stock solution concentrations of 2.5, 5.0 and 7.5 mg/mL.

Experimental procedure

The anthelmintic assay was carried out as per the published methods [25,32,33] with minor modifications. Piperazine citrate was added at 10 mg/mL concentration and included in the assay as positive control. Approximately equal sized six earthworms to 11 petri dishes and 6 roundworms to second set of 11 petri dishes at room temperature containing the extracts at different concentrations and standard drug at one concentration along with normal control. Each petri dish was observed for time taken to induce paralysis (no movement even after tapping) or death of an individual worm. While the time for death was recorded after ascertaining that worms neither moved when tapping the petri dish nor when dipped in warm water (~50 °C) followed by fading away of their body colors. The results from these experiments are presented intable 3andtable 4．

Statistical Analysis

Statistical analysis was carried out using GraphPad Prism, version 5.02. Data was analyzed by one-way analysis of variance (ANOVA) followed by Dunnett’s multiple comparison test. All data are presented as mean ± S. D. A “P” value of <0.05 was considered statistically significant.

Observations and Results

Oral administration of aspirin to Wistar rats produced characteristic mucosal lesions. This damage may be due to its direct action of the gastric epithelium. Aspirin is known to cause gastric injury and to delay ulcer healing. Histologically, an ulcer consists of two major structures; a distinct ulcer margin formed by the adjacent non-necroticmucosa, the epithelial component, granulation tissue at the ulcer base and the connective tissue component. The latter consists of fibroblasts, macrophages and proliferating endothelial cells forming micro vessels. Ulcer healing is a complex process, which involves cell migration, proliferation, re-epithelialization,angiogenesisand matrix deposition, all ultimately leading to scar formation. All these processes are controlled by growth factors, transcription factors and cytokines [34-36].

In the present study, the antiulcerogenic effects ofGloriosa Superba(tuber),Zingiber Officinale(rhizome) and Glycyrhiza Glabra (root) extracts were evaluated and compared in stress plus aspirin induced ulcers and pylorus ligation-induced ulcer models in male Wistar rats. Ranitidine was used as a positive control drug for comparison and the results are presented intable 1．Stress plus aspirin induced linear type of hemorrhagic ulcers with a mean diameter of 10.89 mm (Table 1). Such hemorrhagic lesions were attenuated by pretreatment with ranitidine. The ulcer index was inhibited to 97% (ranitidine), 93% (Gloriosa, 7.5 mg/kg) followed by 83% (Zingiber, 700 mg/kg) and 76% (Glycyrhiza, 250 mg/kg). Such an excellent antiulcerogenic effect of Gloriosa could be due to the facilitation of gastric secretion during severe stress. Its cytoprotective activity would be contributed to the observed strong anti-ulcer activity.

Four hours pylorus ligation significantly increased volume and acidity of the gastric juice in control group of animals received vehicle. Ranitidine effectively controlled the volume, acidity and maintained the pH compared to control group. Gloriosa exhibited strong anti-ulcerogenic effect comparable to ranitidine at high dose (7.5 mg/kg). However, Glycyrhiza and Zingiber failed to exert similar effect even at high doses (table 2).

In spite of multiple mechanisms, gastric secretion is one of the main factors for ulceration, because most types of the ulcers induced by diverse agents were attenuated by the secretion inhibitors. Inhibition of gastric secretion by irreversibly inhibiting the proton-pump H+/K+-ATPase is well known. In addition to gastric secretion, however, several factors such as cell death and recovery, inflammation, stasis and blood flow are involved in the process of ulcer formation [37].

In the present study, it has been demonstrated thatGloriosa Superbatuber extracts exerted strong anti-ulcerogenic effects by controlling gastric acid secretion, acidity and by maintaining the pH of the gastric contents. However, further studies needs to be conducted in appropriate disease models, higher animals and focus should be on isolating and characterizing active constituent(s) responsible for its astounding antiulcerogenic activity in rat model.

Gloriosa Superbatuber aqueous, ethanolic and chloroform extracts were evaluated for the anthelmintic activityin vitroagainst earthworms and roundworms. Results from these studies are presented intable 3andtable 4．Anthelmintic activity exhibited with all the extracts fits this hierarchy from highest to lowest chloroform extract>aqueous extract>ethanolic extract. Chloroform extract exhibited time to death against both the intestinal worms in a dose related way, whereas conventionally used drug piperazine citrate has moderate anthelmintic activity. Our results confirm the reported claims in the literature on its potent anthelmintic activity. However,in vivostudies in disease models need to be conducted to establish its efficacy in treating chronic intestinal infections.

Conclusion

The results of this comprehensive study reveals that theGloriosa superba块茎提取物有显著的antiulcerogenic activity compared to other extracts and standard drug ranitidine. The effects on gastric contents and pH suggest, the extract exerted antispasmodic and acid neutralizing effects. However, experiments in disease models need to be conducted, to delineate its mechanism of action and benefit in the management of gastrointestinal disorders.

Similarly, superior anthelmintic activity foundin vitro需要评估in vivoin appropriate disease models to establish its efficacy.

Acknowledgement

The authors would like to thank Farmiza Begum and N. Srilatha for their help in the execution of studies and Vaagdevi College of Pharmacy for providing necessary facilities to complete this research project.

References

1. Bhargav B, Rabinarayan A. Uses of Langali (GloriosaSuperba Linn.): An ethnomedicinal perspective. AyurpharmInt J AyurAlli Sci. 2012; 1(3):65-72.
2. Parrotta JA.Healing Plants of Peninsular India. Wallingford (UK), CBBI Publishing House. 2001; pp. 221-2.
3. MadhavaChetty K, Sivaji K, Tulasi R. Flowering Plants of Chittor District Andhra Pradesh, India. 1st ed. Tirupati, Offset printers, 2008; pp. 358.
4. Siddaraju MN, Shylaja M. Dharmesh.Inhibition of gastric H+K+ ATPase and H. pylori growth by phenolic anti-oxidants of Zingiberofficinale J Ethnopharmacol.2005; 97:163-76.
5. Geol RK, Sairam K. Anti-ulcer drugs from indigenous sources with emphasis on Zingiberofficinale. J Ethnopharmacol.2002; 34:100-10.
6. Al-Yahya MA, Rafatullah S, Mossa JS, Ageel AM, Parmar NS, Tariq M. Gastroprotective activity of ginger (Zingiberofficinalerosc.) in Albino rats. American J. China med.1989; 17(1-2):51-6.
7. Adel M Aly, Laith AL Alousi, Hatem A. Salem, Licorice: A possible anti-inflammatory and anti-ulcer drug. Aapspharmsci Tech. 2005; 6(1) article13: E74-E82.
8. Sivakumar G•千伏．Gloriosasuperba L., a Very Useful Medicinal Plant, Series Recent Progress in Medicinal Plants, vol. 7, Ethnomedicine and Pharmacognosy, Part II, Singh VK, Govil JN, Hashmi S, Singh G, Eds; Texas, Sci. Techn. Publ. 2002; pp. 465-482.
9. Samy RP, Thwin MM, Gopalakrishnakone P, Savarimuthu SI. Ethanobotanical survey of folk plants for the treatment of snakebites in Southern part of Tamilnadu, India.J Ethanopharmacol. 2008; 115(2): 302-12.
10. Khare CP. Encyclopedia of Indian medicinal Plants.Heidelburg: Springer Verlag. 2004; pp. 232-33.
11. Panda H. Hand Book on Herbal Drugs and its Plant Sources.Delhi, National Institute of Industrial Research. 2001; pp. 426-27.
12. Konturek PC, Kania J, Gessner U, Konturek SJ, Hahn EJ, Konturek JW. Effect of ascorbic acid-releasing acetyl salicylic acid on gastric mucosal damage before and afterH. Pylorieradication therapy.European J Pharmacol.2004; 506: 69-77.
13. Sanchez-Fidalgo S, Martin-Lacave I, Illanes M, Motilva V. Angiogenesis, cell proliferation and apoptosis in gastric ulcer healing. Effect of a selective COX-2 inhibitor.European J Pharmacol.2004; 505: 187-194.
14. Rogler G, Andus T. Cytokines in inflammatory bowel disease.World Journal of Surgery.1998; 22: 382-389.
15. Kitagawa H, Fujiwara M, Osumi Y. Effects of water-immersion stress on gastric secretion and mucosal blood flow in rats. Gastroenterol.1979; 77: 298-302.
16. Wallace JL, Granger DN. The cellular and molecular basis of gastric mucosal defense.FASEB J. 1996; 10: 731-740.
17. Neal MJ.Medical Pharmacology at a Glance. 3rd ed, Blackwell Publishing Inc, London. 2003; pp. 30-31.
18. Byun SK, Lee YE, Shin SH, Jang JY, Choi BI, Park DS, Jeon JH, Nahm SS, Hwang SY, Kim YB. The role of corticosteroids in stress-induced gastric ulceration in rats.Lab Anim Res. 2007; 23: 127-131.
19. Wallmark B, Larsson H, Humble L.The relationship between gastric acid secretion and gastric H+, K+-ATPase activity. J BiolChem 1985; 260(25):13681-13684.
20. Mohsen M, Alireza G, Alireza K. Anti-ulcerogenic effect of ginger (Rhizome ofZingiberofficinaleRoscoe) on cystemine induced duodenal ulcer in rats. DARU. 2006; 14(2):97-101.
21. Bennett A, Clark-Wibberley T, Stamford IF. Aspirin-induced gastric mucosal damage in rats: cimetidine and deglycyrrhizinatedliquorice together give greater protection than low doses of either drug alone. J Pharm Pharmacol. 1980; 32(2):150.
22. Toshio F et al. Anti-Helicobacter pylori flavonoids from Licorice extracts. Life sci. 2002; 71: 1449-63.
23. Kaushik RK, Katiyar JC, Sen AB. Studies on the mode of the action of anthelmintics withAscardiagalli作为测试寄生虫。印度J实用医学杂志1974;62: 1367-75.
24. Lal J, Chandra S, Raviprakash V, Sabir M. In vitro anthelmintic action of some indigenous medicinal plants onAscardiagalliworms.Indian J PhysiolPharmacol.1976; 20: 64-8.
25. Ajaiyeoba EO, Onocha PA, Olarenwaju OT. In vitro anthelmintic properties ofBuchholziacoriaceaeandGynandropsisgynandraextract. Pharm Biol. 2001; 39: 217-20.
26. Martin RJ.Modes of action of anthelmintic drugs. Vet J. 1997; 154(1): 11-34.
27. Niezen JH, Waghorn TS, Charleston WA. Growth and gastrointestinal nematode parasitism in lambs grazing either lucerne (Medicago sativa) or sulla (Hedysarumcoronarium) which contains condensed tannins. J Agri Sci. 1995; 125: 281-289.
28. Athnasiadou S, Kyriazakis I, Jackson F, Coop RL. Direct anthelmintic effects of condensed tannins towards different gastro intestinal nematodes of sheep: In vitro and in vivo studies. Vet Parasitol. 2001; 99: 205-219.
29. Thomson DP, Geary TG.The structure and function of helminth surfaces. In: Marreds. Biochemistry and Molecular Biology of Parasites; Academic Press, New York. 1995; pp. 203-232.
30. Cao H, Wang MW, Sun LX, Ikejima T, Hu ZQ, Zhao WH. Pharmacodynamic comparison of pantoprazole enantimers: inhibition of acid-related lesions and acid secretion in rats and guinea-pigs. J Pharm Pharmacol.2005; 57: 923-927.
31. Bae DK, Park D, Lee SH, Yang G, Yang YH, Kim TK, Choi YJ, Kim JJ, Jeon JH, Jang MJ, Choi EK, Hwang SY, Kim YB. Different antiulcer activities of pantoprazole in stress, alcohol and pylorus ligation-Induced ulcer models. Lab Anim Res. 2011: 27(1): 47-52.
32. Raut DN, Pal SC, Mandal SC. Anthelmintic potential ofDendrophthoefalcataetting．(L.F.) leaf.IJPRD.2009; 6: 1-7.
33. Girme AS, Bhalke RD, Ghogare PB, Tambe VD, Jadhav RS, Nirmal SA.Comparative In vitro Anthelmintic Activity ofMenthapiperitaandLantana camarafrom Western India. Dhaka Univ. J. Pharm. Sci. 2006; 5(1-2): 5-7.
34. Mallika J, Shyamala Devi CS. Gastroprotective action ofCissusquadrangularisextract against NSAID induced gastric ulcer: role of proinflammatory cytokines and oxidative damage. Chemico-Biological Interactions.2006; 161: 262-270.
35. Tarnawski AS.The Stomach, W. Domschke, S. J. Konturek (Eds.), Cellular Mechanisms of Gastric Ulcer Healing, Springer, Berlin/New York. 1993; pp. 177-192.
36. Tarnawski AS. Cellular amd molecular mechanisms of gastrointestinal ulcer helaing: State of the art. GastroenterologiaPolska. 2010; 17(3): 171-179.
37. Lou LX, Geng B, Yu F, Zhang J, Pan CS, Chen L, Qi YF, Ke Y, Wang X, Tang CS. Endoplasmic reticulum stress response in involved in the pathogenesis of stress induced gastric lesions in rats. Life Sci. 2006; 79: 1856-1864.