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Indian Journal of Pharmacology
Medknow Publications on behalf of Indian Pharmacological Society
ISSN: 0253-7613 EISSN: 1998-3751
Vol. 42, Num. 4, 2010, pp. 234-237

Indian Journal of Pharmacology, Vol. 42, No. 4, July-August, 2010, pp. 234-237

Research Article

Evaluation of Cassia occidentalis for in vitro cytotoxicity against human cancer cell lines and antibacterial activity

Bhagat Madhulika, Saxena AjitKumar

School of Biotechnology, University of Jammu, Jammu
Correspondence Address:School of Biotechnology, University of Jammu, Jammu, madhulikabhagat@rediffmail.com

Date of Submission: 19-Nov-2008
Date of Decision: 13-Aug-2009
Date of Acceptance: 26-Jun-2010

Code Number: ph10066

DOI: 10.4103/0253-7613.68428

Abstract

Objective : To evaluate the in vitro cytotoxicity and antibacterial properties of Cassia occidentalis (whole plant) via alcoholic, hydro-alcoholic, and aqueous extracts against eight human cancer cell lines from six different tissues and four bacterial strains.
Material and Methods : In vitro cytotoxicity against the human cancer cells, cultured for 48h in presence of different concentrations C. occidentalis extracts and percentage of cell viability, was evaluated using the sulforhodamine-B (SRB) assay. The antibacterial activity was performed using the standard protocol against bacterial strains.
Results : It was observed that aqueous extract of C. occidentalis (whole plant) had more potential than hydro-alcoholic and alcoholic extracts against HCT-15, SW-620, PC-3, MCF-7, SiHa, and OVCAR-5 human cancer cell lines at 100, 30, and 10 μg/ml in a dose-dependent manner. The hydro-alcoholic extract showed potential against Bacillus subtillis.
Conclusion : The plant can be explored for the possible development of lead molecules for drug discovery.

Keywords: Antibacterial activity, Cassia occidentalis, cytotoxicity

Introduction

Approximately 80% of the world′s population still relies on traditional medicines for the treatment of common illnesses. [1] It is observed that management of cancer and infectious diseases always require search for new drugs. Although numerous drugs are currently in use for cancer chemotherapy, they exhibit cell toxicity, induces genotoxic, carcinogenic, and teratogenic effects in non-tumor cell. [2] These side effects limit use of chemotherapeutic agents despite their high efficacy in treating target malignant cells. Similarly, antibacterial drug resistance has been a therapeutic problem. [3] Therefore, the search for novel drugs that are both effective and non-toxic bioactive plant products has been increased. [4] Cassia occidentalis (Leguminosae) plant has been extensively used in indigenous and folk-lore medicine system. In Indian system of medicine the plant has been documented as thermogenic, puragative, expectorant, diuretic, and used in the treatment of leprosy, erysipelas, ulcers, cough, bronchitis, constipation, flatulence, dyspepsia, menstrual problems, tuberculosis, and anemia. [5] Reports for its immunosuppressive, [6] antimutagenic, [7] anti-inflammatory, [8] anti-dermatophyte, [9] antibacterial, [10] antiplasmodial, [11] anti-fertility, [12] antimalarial, [13] and antidiabetic [14] activities had been published. The leaf extracts of the plant have been reported to repair, protect, and normalize the liver functions. [15] Considering the therapeutic values of C. occidentalis, the present work was undertaken to evaluate the in vitro cytotoxic and antibacterial activity.

Material and Methods

Chemical Agents

RPMI- 1640, Dulbecco′s minimum essential medium (DMEM), fetal calf serum (FCS), trypsin, gentamycin, penicillin, ethylene diaminetetraacetic acid (EDTA), 5-flurouracil, dimethyl sulfoxide, and sulforhodamine-B were purchased from Sigma Chemical Co., USA. All other chemicals were of high purity and obtained locally.

Plant Material

Whole plant of C. occidentalis was collected locally in the month of December and was authenticated at source by the taxonomist of the institute. A voucher specimen has been deposited at the herbarium of the Institute vide IIIM collection No.17687, Acc. No.19361.

Preparation of Extracts

The authenticated and freshly collected whole plant was chopped and dried under shade. Three extracts of the plant material were made with 95% alcohol, alcohol-water (1:1), and water using repeated solvent extraction procedure. Dried powdered plant material (1 kg) was percolated in 95% alcohol (5 L) at ambient temperature for 16 h. The solvent was decanted and the process was repeated four times. The pooled solvent was evaporated under reduced pressure to yield alcoholic extract (160 g). Similarly, hydro-alcoholic extract was prepared. The dried plant material (200 g) was soaked in alcohol:water (1:1, 1 L) and the extract obtained was 72 g. For aqueous extract the dried powdered plant material (200 g) was heated with distilled water (1.5 L) on steam bath for 2 h, the supernatant was decanted and filtered through celite powder and the process was repeated four times, pooled extract was concentrated on rotavapour and dried in a lyophilizer, and 40 g extract was obtained.

Cell Lines and Culture

The human cancer cell lines were obtained either from National Center for Cell Science, Pune, India, or National Cancer Institute, Fredrick, USA. The cell lines namely colon (HCT-15, SW-620, COLO 205), ovary (OVCAR-5), prostate (PC-3), and lung (HOP-62) were grown and maintained in RPMI-1640 medium, pH 7.4, whereas DMEM was used for breast (MCF-7) and cervix (SiHa).

In vitro Cytotoxicity against Human Tumor Lines

The in vitro cytotoxicity of extracts was determined using sulforhodamine-B (SRB) as described previously. [16] In brief, the stock solution (20 mg/ml) of the alcoholic, hydro-alcoholic, and aqueous extracts was prepared in dimethylsulfoxide (DMSO), dimethylsulfoxide - water (1:1) and hot water. The stock solutions were further diluted with growth medium (RPMI-1640/ DMEM with 2mM glutamine, pH 7.4, 10% fetal calf serum, 100 μg/ml streptomycin and 100 U/ml penicillin) to obtain desired concentrations. The cells were grown in tissue culture flasks in growth medium at 37οC in an atmosphere of 5% CO 2 and 95% relative humidity in a CO 2 incubator. The cells at subconfluent stage were harvested from the flask by treatment with trypsin (0.05% trypsin in PBS containing 0.02% EDTA) and suspended in the growth medium. Cells with more than 97% viability (Trypan blue exclusion) were used for determination of cytotoxicity. An aliquot of 100 μl of cell suspension (10 5 to 2 Χ10 5 cells/ml depending upon mass doubling time of cells) was transferred to a well of 96-well tissue culture plate and incubated for 24 h. The test materials (100 μl) were then added to the wells and incubated for another 48 h. The cell growth was stopped by 50 μl of 50% trichloroacetic acid and plates were further incubated at 4οC for an hour. The plates were washed with distilled water and air-dried. Sulforhodamine B (100 μl, 0.4% in 1% acetic acid) was added to each well and plates were incubated at room temperature for 30 min. The unbound SRB was removed by washing with 1% acetic acid and air-dried. Tris-HCL buffer (100 μl, 0.01 M, pH 10.4) was added to all the wells and stirrer. The optical density was recorded on ELISA reader at 540 nm. Suitable blanks and positive controls were also included. Each test was done in triplicate.

The percentage of cell viability was calculated according to the following equation.

OD of control cells

Statistical Analysis

The experiments were repeated three times and the results were expressed as mean ± SD.Statistical analysis was done using unpaired Student′s t-test and P values < 0.01 were considered significant.

Antibacterial Assay

The antibacterial assays were performed using the standard protocols. [17]

Results

In vitro Cytotoxic Effect against Human Cancer Cell Lines

In vitro cytotoxicity of all the three extracts (alcoholic, hydro-alcoholic and aqueous) of C. occidentalis (whole plant) was evaluated at 10, 30, and 100 μg/ml against eight human cancer cell lines from six different tissues origin, namely colon, prostate, breast, cervix, ovary, and lung [Figure - 1]. Growth inhibition in a dose-dependent manner was observed in all the cell lines by all there extracts. It was also observed that aqueous extract was most active than hydro-alcoholic and alcoholic extract against all the human cancer cell lines except lung (HOP-62) cancer cell lines where the percent growth inhibition was less than 50%, in comparison to the positive control paclitaxel. When compared with the different positive controls (5-FU, mitomycin C, adriamycin, and paclitaxel) specific for different cell lines the growth inhibition of aqueous extract was found higher than other two extracts. At 100 μg/ml out of eight cancer cell lines aqueous extract showed more than 70% growth inhibition against four cancer cell lines, namely 81% against HCT-15 (colon), 76% against SW-620 (colon), 78% against SiHa (cervix), and 76% against OVCAR-5 (ovary) human cancer cell lines [Figure - 1]. Further on lower doses of 30 and 10 μg/ml percent growth inhibition observed by aqueous extract was 71 and 43% against HCT-15 (colon), 64 and 40% against SW-620 (colon), and 76 and 42% against SiHa (cervix) human cancer cell lines. Hydro-alcoholic extract showed highest cytotoxicity against HEP-2, followed by COLO 205 with 96% and 89% growth inhibition at 100 μg/ml, further on lower doses of 30 and 10 μg/ml percent growth inhibition observed was 74 and 39% against HEP-2, 18, and 28 against COLO 205 human cancer cell lines, minimum cytotoxic effect by hydro-alcoholic extract was observed against MCF-7 cancer cell line, and for rest of the cancer cell lines growth inhibition was observed less than 70% at 100 μg/ml. The alcoholic extract showed comparatively less activity against all the eight human cancer cell lines [Figure - 1].

Antibacterial Assay

The in vitro antibacterial activity of the three extracts of C. occidentalis (whole plant) was found less than that of chloramphenicol, which was used as standard. Out of all the three extracts, hydro-alcoholic extract demonstrated more sensitivity against Bacillus subtillis than alcoholic and aqueous extracts. Whereas all the three extracts were found to be inactive against Escherichia coli, Pseudomonas aeruginosa, and Staphylococcus aureus [Table - 1].

Discussion

The present study observed that the aqueous and hydroalcoholic extracts of C. occidentalis inhibits the proliferation of eight human cancer cell lines. The cytotoxicity effect was highest with aqueous extract and least for alcoholic extract. Although the activity demonstrated by the whole plant was low, this may be due to the crude nature of the extracts that can be further enhanced by the purification. The cytotoxicity was concentration-dependent and cell line specific. This clearly indicates the presence of potent bioactive principles in the crude extract that might be useful as antiproliferative and antitumoragents.[18] Although the mechanism of the action have not been elucidated, but there are report that aqueous extracts from leaves of C. occidentalis to contain flavonoids and antioxidant polyphenolic compounds.[19] These compounds are known to scavenge the formation of free radicals, have great potential in ameliorating disease processes like cancer and diabetes.[20] The extracts could have exerted its actions by some unknown mechanism ether alone or in combination. Thus the active principle(s) need to be identified.

Similarly, hydro-alcoholic extract of C. occidentalis showed potent antibacterial activity against Bacillus subtillis strain indicating the presence of chemical constituents responsible for antibacterial activity. The prokaryotic cell structure of a bacterial cell is different than eukaryotic cells. Therefore, both in vitro cytotoxicity and antimicrobial bioassays help us to understand the potential activity of a natural compound(s) or a crude extract.[21] The present study shows that whole plant C. occidentalis possess both in vitro cytotoxicity and antibacterial activity. The plant can be further explored for its potential therapeutic uses.

Acknowledgements

Authors are grateful to National Centre for Cell Science, Pune (India) and National Cancer Institute, Frederick, MD, U.S.A for providing human cancer cell lines.

References

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