Assessment of the anticancer potential of certain phenolic and flavonoid components in ginger capsules using colorectal cancer cell lines coupled with quantitative analysis

Author:

Al Azzam Khaldun M.1ORCID,Al‐Areer Nadeen Waleed2,Al Omari Rima H.2,Al‐Deeb Ibrahim3ORCID,Bounoua Nadia45,Negim El‐Sayed67,Al‐Samydai Ali2ORCID,Aboalroub Adam A.2,Said Rana2

Affiliation:

1. Department of Chemistry, Faculty of Science The University of Jordan Amman 11942 Jordan

2. Department of Pharmaceutical Sciences, Pharmacological and Diagnostic Research Center (PDRC), Faculty of Pharmacy Al‐Ahliyya Amman University Amman 19328 Jordan

3. Department of Biopharmaceutics and Clinical Pharmacy, Pharmacological and Diagnostic Research Center (PDRC), Faculty of Pharmacy Al‐Ahliyya Amman University Amman 19328 Jordan

4. Laboratory of the Innovation Sponsorship and the Emerging Institution for Graduates of Higher Education of Sustainable Development and Dealing with Emerging Conditions, Department of Exact Sciences Normal Higher School of Bechar Bechar 8000 Algeria

5. Laboratory of Chemical and Environmental Science (LCSE) Bechar Algeria 8000

6. School of Petroleum Engineering Satbayev University 22 Satpayev Street Almaty 050013 Kazakhstan

7. School of Materials Science and Green Technologies Kazakh‐British Technical University 59 Tole bi St. Almaty 050000 Kazakhstan

Abstract

AbstractColorectal cancer (CRC) is the fourth most common cause of malignant tumor death. The development of novel, more effective drugs is desperately needed to treat CRC. Zingiber officinale is believed to possess anticancer properties due to its flavonoids and phenols. Using Soxhlet (SOXT) and maceration (MACR) techniques, the present study aimed to evaluate the amounts of quercetin, gallic acid, rutin, naringin, and caffeic acid in ginger capsules of Z. officinale. High‐performance liquid chromatography (HPLC)/ultraviolet was used for separation and quantitation. In vitro toxicity evaluation of ginger capsules on the CRC cell line HT‐29 was also conducted to assess the anticancer activity of the supplement. The cell line HT‐29 (HTB‐38) colorectal adenocarcinoma was utilized for the antiproliferative effect of 3‐(4,5‐dimethylthiazol‐2‐yl)‐2,5‐diphenyl tetrazolium bromide. Ginger herbal supplement extract at dosages of 200 and 100 μg had strong cytotoxic effects (IC50 < 50 μg/mL) on HT‐29 CRC cells via MACR. This extract is comparable to the SOXT extract, which has an IC50 of less than 50 μg/mL. The anticancer effect of ginger herbal supplement formulations against CRC lines was investigated, and the results obtained from both the MACR and SOXT extraction procedures were noteworthy. The quercetin content was the highest of all the extracts according to the HPLC data.

Publisher

Wiley

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