Tropical Journal of Pharmaceutical Research

Original Research Article | OPEN ACCESS

Modulatory effect of Althaea officinalis L root extract on cisplatin-induced cytotoxicity and cell proliferation in A549 human lung cancer cell line

Yukun Zhang, Fanhua Kong, Lei Zhang, Chao Li, Runqi Zhang

Department of Thorax Surgery, Taian City Central Hospital, Taian City 271000, Shandong Province, China;

For correspondence:- Runqi Zhang Email: drzhangrunqi@hotmail.com Tel:+865386298489

Received: 15 April 2016 Accepted: 16 November 2016 Published: 21 December 2016

Citation: Zhang Y, Kong F, Zhang L, Li C, Zhang R. Modulatory effect of Althaea officinalis L root extract on cisplatin-induced cytotoxicity and cell proliferation in A549 human lung cancer cell line. Trop J Pharm Res 2016; 15(12):2647-2652 doi: 10.4314/tjpr.v15i12.16

© 2016 The authors.
This is an Open Access article that uses a funding model which does not charge readers or their institutions for access and distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/4.0) and the Budapest Open Access Initiative (http://www.budapestopenaccessinitiative.org/read), which permit unrestricted use, distribution, and reproduction in any medium, provided the original work is properly credited..

Abstract

Purpose: To explore the modulatory effect of an Althaea officinalis root extract (AORE) on cisplatin-induced cytotoxicity and cell proliferation in a lung cancer cell line.

Methods: Aqueous AORE was obtained from peeled and powdered roots. The effect of cisplatin on cytotoxicity and cell proliferation was studied. The cisplatin concentrations tested ranged from 0 - 30 mg/mL. Cell viability and proliferation were studied using trypan blue and MTT assays, respectively. The cells were also exposed to a combination of cisplatin and the AORE.

Results: Cisplatin yielded a 50 % inhibitory concentration at 25 mg/mL and exhibited a dose-dependent cell proliferation loss. Combined use of the root extract and cisplatin had significant (R2 = 0.8305) modulatory effects on cytotoxicity and antiproliferative activities. The best inhibitory effects were observed in cells exposed to a combination of 8 or 10 % AORE and 25 mg/mL cisplatin. The optimal effect on cell proliferation was obtained using 25 mg/mL cisplatin and 10 % v/v AORE.

Conclusion: The enhanced activity of cisplatin in combination with AORE was more pronounced for cell proliferation than cytotoxicity, indicating that AOREs may be used to control tumor progression and metastasis.

Keywords: A549 cells, Althaea officinalis, lung cancer, cell proliferation, cell viability, cisplatin, modulatory effect

Introduction

Althaea officinalis (AO), known as common marshmallow or marshmallow, belongs to the Malvaceae family within the order Malvales. This plant has perennial roots and stems that die in the autumn [1]. The Greek meaning of the generic name Althaea is “to cure” or “to heal,” signifying the beneficial application of this plant, especially its perennial roots [2]. Apart from the roots, the leaves, seeds, and flowers of the plant are used in traditional Chinese medicine [3,4]; major therapeutic applications of AO roots include treating ailments of the throat, mucous membranes, digestive system, and structures of the respiratory system, including the bronchial tubes [5]. AO extracts are known to have anti-inflammatory, antimicrobial, anti-tussive, hypoglycaemic, and dermatological healing effects [6,7]. The leaves and roots are either applied topically as a paste or consumed directly. The roots of the plant are also used as a dried powder and as a vegetable. The most common preparation of this plant is marshmallow confectioneries, while the roots of AO are commonly used for their health effects.

The major phytochemicals identified in AO roots are mucilage with many polysaccharides, pectin, and tannins [8,9]. The mucilage content of AO varies between seasons, with maximum and minimum amounts present in winter and summer, respectively [10]. The pharmaceutical importance of AO has been extensively reviewed [11].

A549 is a human non-small cell lung adenocarcinoma cell line of the basal epithelial type. Having a doubling time of 22 – 24 h, this cell line is robust and well-suited for several in vitro applications.

Cisplatin is a chemotherapeutic drug used extensively for cancer therapy, and it has been the drug of choice for several in vitro research applications. Cisplatin functions by inducing apoptosis via DNA cross-linking.

The aim of this work was to determine the effect of AOR on the activity of cisplatin in A549 cells using two end points: cytotoxicity and cell proliferation.

Methods

Plant material collection and extraction

Collection of the AOR extract was performed in the winter of 2013, with the roots dried and peeled. A fine powder was obtained from the peeled roots by mechanical grinding and aliquots of 1 g were stored at -20 °C. A total of 1 g of fine powder was mixed in 10 mL of Milli-Q water at 4 °C, filter-sterilized, and stored at -20 °C before being used for the experiments. The authentication of the plant identity and classification was performed by a taxonomist, Dr Hu Hong of Kunming Institute of Botany, Yunnan Province, China. A voucher specimen has been preserved at South China Botanical Garden Herbarium, Chinese Academy of Sciences (IBSC) with tTaxon Id # 20001368.

Experimental design and cell cultures

The entire study was performed in three steps, as follows: (1) ascertain the 50 % inhibitory concentration (IC₅₀) value of cisplatin in A549 cells, (2) ascertain the effect of direct exposure to an AOR extract on A549 cells, and (3) ascertain the modulatory effect of an AOR extract on cisplatin-induced cell inhibitory effects in the selected cell line. Healthy A549 cells from 85 % confluent T-25 flasks cultured in DMEM supplemented with 10 % FBS were used as a seed stock for all experiments. The seeding density of the cells used was 0.17 x 10⁶ cells/mL in 24-well plates (1 mL cultures) and 1.0 × 10⁵ cells/well in 96-well plates (200 µL cultures). Cell viability and MTT assays were used as end points; cytotoxicity experiments were conducted in 24-well plates, and the MTT assay was performed in 96-well culture plates. For cytotoxicity assays, cells were collected along with the supernatant after mild mixing and attached cells were trypsinized, harvested, and pooled with the supernatants. Cells were washed once in medium without FBS and were analyzed for percent viability using the trypan blue assay. The MTT assay was performed on cells after the respective drug and combination (drug + AOR extract) exposures. After exposure to the drug or the drug + AOR extract, the wells of 96-well plates were filled with 10 µL of MTT (stock: 10 mg/mL) and incubated for 4 h. A total of 10 µL of solubilization buffer containing 10 % SDS and 0.01 N HCl was added to the wells and the plates were incubated overnight at room temperature. The absorbance was measured at 550 nm using a microplate reader. All experiments were performed in triplicate; the average of the triplicate values were taken as the final values.

Evaluation of cisplatin activity on A549 cells

The IC₅₀ value of cisplatin in A549 cells was determined by exposing cells to 10, 15, 20, 25, and 30 mg/mL cisplatin for 24 h. Similarly, cells in the 96-well plates were exposed to the same concentrations of the drug for 24 h and analyzed using the MTT assay.

Evaluation of exposure of AOR extract on A549 cells

AOR extract exposure was performed in 24- and 96-well plates to explore the effects of the AOR extract on A549 cells. In addition, a 10 % stock extract was added to the cell culture wells to obtain a final concentration of 2, 4, 6, 8, and 10 % of the stock. The cultures were incubated for 24 h and analyzed by trypan blue and MTT assays, as described above.

Determination of modulatory effect of the AOR extract on cisplatin-induced cytotoxicity in A549 cells

Cells in 24- and 96-well plates were simultaneously exposed to cisplatin at the IC50 concentration and 2, 4, 6, 8, and 10 % AOR extract (as in step 2). The cultures were incubated for 24 h and analyzed by trypan blue and MTT assays, as described above.

Statistical analysis

A one-way analysis of variance was used to analyze the variables. Standard deviation was expressed as error bars and R-values in the graphs.

Results

Cell morphology

Healthy cells did not show any change in morphology when exposed to the AOR extract. However, morphological changes were observed for cells exposed to cisplatin and a combination of 25 mg/mL cisplatin + 10 % v/v AOR extract ().

Effect of cisplatin on A549 cell viability

The viability of untreated A549 cells was 96 % while the values for cisplatin at concentrations of 0, 0.25, 5, 10, 15, 20, 25, and 30 mg/mL were 96, 92, 81, 72, 63, 56, 52, and 49 %, respectively. The IC₅₀ value of cisplatin was close to 25 mg/mL (a).

Cytotoxicity and cell proliferation

The absorbance value for the control was 0.73 while it was 0.64, 0.61, 0.58, 0.52, 0.47, 0.32, and 0.26 for the seven different cisplatin concentrations, respectively (b).

Cell viability after exposure to AOR extract

There was no significant effect of direct exposure to the AOR extract on A549 cells. However, a marginal decrease in viability was observed in cells exposed to 8 and 10 % AOR stock extract with 94 % viability ().

The MTT assay did not show any significant effect on cell proliferation, with absorbance values close to 0.72 for all concentrations.

Effect of AOR extract on cisplatin-induced cytotoxicity in A549 cells

The cells exposed to 25 mg/mL (IC₅₀) cisplatin and 2, 4, 6, 8, and 10 % AO stock extract produced viability values of 51, 51, 41, 41, and 39 %, respectively. While the 2 and 4 % AOR stock extracts did not have any significant cytotoxicity-enhancing effect, there was a significant increase in cytotoxicity (increased IC₅₀ value of cisplatin) in cultures exposed to 8 and 10 % AOR stock extract (Figures 4 and 5).

Cell proliferation

The absorbance values for cells exposed to 25 mg/mL cisplatin and 0, 2, 4, 6, 8, and 10 % AOR stock extract were 0.31, 0.3, 0.3, 0.23, 0.21, and 0.19, respectively ().

Discussion

The cell line (A549) and drug (cisplatin) used in this study are considered useful materials based on several previous studies. AOR extracts are also commonly used in traditional medicine; the past decade has seen a growing number of scientific reports of studies performed systematically using AOR extracts. The AOR extract in this study was used in combination with cisplatin to study its modulatory effects on two parameters: cytotoxicity and anti-proliferation. While cytotoxicity is an effect of immediate and direct consequence, cell proliferation involves a sequence of events. However, both parameters have relevance to cancer research in terms of killing cancer cells and limiting metastasis. The AOR extract did not induce changes in the morphology, viability, or proliferation of A549 cells, suggesting that it is safe for cells. The extract had marked modulatory effects on cisplatin-induced toxicity and an anti-proliferative effect at 8 and 10 % v/v. The synergistic effect was significant; it induced marked morphologic changes with a reciprocal loss in viability. A combination of 25 mg/mL cisplatin + 10 % v/v AOR extract induced more pronounced anti-proliferative activity compared to cisplatin-induced cytotoxicity.

Conclusion

The findings of this study indicate the usefulness of AOR extract in modulating the effect of cisplatin in A549 cells in terms of cytotoxicity and cell proliferation. The modulatory effect on cell proliferation was greater than the effect on cytotoxicity, demonstrating that AOR extract is a potential anti-cancer agent.

Declarations

Acknowledgement

The authors thank the managers of the affiliated departments and hospitals for their support.

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