Статья

Cytotoxicity of Anchusa arvensis Against HepG-2 Cell Lines: Mechanistic and Computational Approaches

Sajid HussainDepartment of Pharmacy, University of Malakand, Malakand, PakistanFarhat UllahDepartment of Pharmacy, Kohat University of Science & Technology, Kohat, PakistanAbdul SadiqDepartment of Pharmacy, University of Malakand, Malakand, PakistanMuhammad AyazDepartment of Pharmacy, University of Malakand, Malakand, PakistanAzhar-ul-Haq Ali ShahDepartment of Chemistry, Kohat University of Science & Technology, Kohat, PakistanSyed Adnan Alı ShahDepartment of Pharmacy, University of Malakand, Malakand, PakistanSyed Majid ShahDepartment of Pharmacy, University of Malakand, Malakand, PakistanAkhtar NadhmanInstitute of Integrative Biosciences IIB, CECOS University, Peshawar, PakistanFarman UllahDepartment of Pharmacy, University of Malakand, Malakand, PakistanAbdul WadoodDepartment of Biochemistry, Abdul Wali Khan University Mardan, Mardan, PakistanMohamed El‐ShazlyDepartment of Pharmacognosy and Natural Products Chemistry, Faculty of Pharmacy, Ain-Shams University, Cairo, Egypt

2019en

ABI

Аннотация

BACKGROUND: Liver cancer is a devastating cancer with increasing incidence and mortality rates worldwide. Plants possess numerous therapeutic properties, therefore the search for novel, naturally occurring cytotoxic compounds is urgently needed. METHODS: The anticancer activity of plant extracts and isolated compounds from Anchusa arvensis (A. arvensis) were studied against the cell culture of HepG-2 (human hepatocellular carcinoma cell lines) using 3-(4,5-Dimethylthiazol-yl)-diphenyl tetrazoliumbromide (MTT) assay. Apoptosis was investigated by performing Acridine orange -ethidium bromide staining, styox green assay and DNA interaction study. We also used tools for computational chemistry studies of isolated compounds with the tyrosine kinase. RESULTS: In MTT assay, the crude extract caused a significant cytotoxic effect with IC50 of 34.14 ± 0.9 μg/ml against HepG-2 cell lines. Upon fractionation, chloroform fraction (Aa.Chm) exhibited the highest antiproliferative activity with IC50 6.55 ± 1.2 μg/ml followed by ethyl acetate (Aa.Et) fraction (IC50, 24.59 ± 0.85 μg/ml) and n-hexane (Aa.Hex) fraction (IC50 29.53 ± 1.5μg/ml). However, the aqueous (Aa.Aq) fraction did not show any anti-proliferative activity. Bioactivity-guided isolation led to the isolation of two compounds which were characterized as para-methoxycatechol (1) and decane (2) through various spectroscopic techniques. Against HepG-2 cells, compound 1 showed marked potency with IC50 6.03 ± 0.75 μg/ml followed by 2 with IC50 18.52 ± 1.9 μg/ml. DMSO was used as a negative control and doxorubicin as a reference standard (IC50 1.3 ± 0.21 μg/ml). It was observed that compounds 1-2 caused apoptotic cell death evaluated by Acridine orange -ethidium bromide staining, styox green assay and DNA interaction study, therefore both compounds were tested for molecular docking studies against tyrosine kinase to support cytotoxic activity. CONCLUSION: This study revealed that the plant extracts and isolated compounds possess promising antiproliferative activity against HepG-2 cell lines via apoptotic cell death.

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Идентификаторы

DOI: 10.2174/1568026619666191105103801

Цитирования и источники

Цитирований: 2Использованных источников: 0

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