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Assessing anti oxidant, antidiabetic potential and GCMS profiling of ethanolic root bark extract of Zanthoxylum rhetsa (Roxb.) DC: Supported by in vitro, in vivo and in silico molecular modeling.
Barman, Apurba Kumar; Mahadi, Sumaiya; Hossain, Md Arju; Begum, Rahima; Acharyya, Rabindra Nath; Alam, Marjana; Rahman, Md Habibur; Biswas, Nripendra Nath; Hossain, A S M Monjur Al.
Affiliation
  • Barman AK; Department of Pharmacy, R. P. Shaha University, Naryanganj, Bangladesh.
  • Mahadi S; Department of Pharmacy, R. P. Shaha University, Naryanganj, Bangladesh.
  • Hossain MA; Department of Microbiology, Primeasia University, Banani, Bangladesh.
  • Begum R; Department of Pharmacy, Noakhali Science and Technology University, Noakhali, Bangladesh.
  • Acharyya RN; Pharmacy Discipline, Life Science School, Khulna University, Khulna, Bangladesh.
  • Alam M; Department of Pharmacy, R. P. Shaha University, Naryanganj, Bangladesh.
  • Rahman MH; Department of Computer Science and Engineering, Islamic University, Kushtia, Bangladesh.
  • Biswas NN; Center for Advanced Bioinformatics and Artificial Intelligent Research, Islamic University, Kushtia, Bangladesh.
  • Hossain ASMMA; Pharmacy Discipline, Life Science School, Khulna University, Khulna, Bangladesh.
PLoS One ; 19(8): e0304521, 2024.
Article in En | MEDLINE | ID: mdl-39159188
ABSTRACT
Zanthoxylum rhetsa (ZR) is used traditionally to manage a variety of ailments, including diabetes. Oxidative stress may accelerate the diabetic condition. The available antidiabetic and antioxidant drugs have many shortcomings including resistance, inefficiency, higher dose, side effects and costs. The goal of the current investigation was to assess the antioxidant capacity and antidiabetic activity of an ethanolic extract of Zanthoxylum rhetsa root bark (ZRRB) through in vitro, in vivo, and in silico methods. The antioxidant capacity of the ZRRB extract was measured using both the DPPH radical assay and the total antioxidant activity test. The oral glucose tolerance test (OGTT) and alloxan-induced diabetic mice model were also used to examine in vivo antidiabetic efficacy. Phytochemicals identification was done by GCMS analysis. Additionally, computational methods such as molecular docking, ADMET analysis, and molecular dynamics (MD) modeling were performed to determine the above pharmacological effects. The extract demonstrated significant DPPH scavenging activity (IC50 = 42.65 µg/mL). In the OGTT test and alloxan-induced diabetes mice model, the extract effectively lowered blood glucose levels. Furthermore, in vitro inhibition of pancreatic α-amylase studies demonstrated the ZRRB extract as a good antidiabetic crude drug (IC50 = 81.45 µg/mL). GCMS investigation confirmed that the crude extract contains 16 major phytoconstituents, which were docked with human peroxiredoxin-5, α-amylase, and sulfonylurea receptor 1. Docking and pharmacokinetic studies demonstrated that among 16 phytoconstituents, 6H-indolo[3,2,1-de] [1,5]naphthyridin-6-one (CID 97176) showed the highest binding affinity to targeted enzymes, and imitated Lipinski's rule of five. Furthermore, MD simulation data confirmed that the aforementioned compound is very steady to the binding site of α-amylase and sulfonylurea receptor 1 receptors. Findings from in vitro, in vivo and in silico investigation suggest that ZRRB extract contains a lead compound that could be a potent source of antidiabetic drug candidate.
Subject(s)

Full text: 1 Database: MEDLINE Main subject: Plant Extracts / Plant Bark / Zanthoxylum / Diabetes Mellitus, Experimental / Molecular Docking Simulation / Hypoglycemic Agents / Antioxidants Limits: Animals Language: En Journal: PLoS One Journal subject: CIENCIA / MEDICINA Year: 2024 Type: Article Affiliation country: Bangladesh

Full text: 1 Database: MEDLINE Main subject: Plant Extracts / Plant Bark / Zanthoxylum / Diabetes Mellitus, Experimental / Molecular Docking Simulation / Hypoglycemic Agents / Antioxidants Limits: Animals Language: En Journal: PLoS One Journal subject: CIENCIA / MEDICINA Year: 2024 Type: Article Affiliation country: Bangladesh