香桃木叶提取物的抗霉菌和抗癌特性

Pharmaceuticals Pub Date : 2024-07-02 DOI:10.3390/ph17070872
M. A. Mir, Lamis Ahmad Memish, S. E. Elbehairi, Nasreena Bashir, Faris Saif Masoud, A. Shati, M. Alfaifi, Ahmad M. Alamri, S. A. Alkahtani, Irfan Ahmad
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引用次数: 0

摘要

背景:植物萃取产品或提取物在民间/传统医学中被广泛用于治疗多种感染、疾病或失调。香桃木是一种著名的药草,原产于地中海地区,是一种常绿芳香植物,在世界各地的传统医学中使用已久。材料和方法采用微孔板氨蓝法和孔扩散法分别评估抑制区和 MIC。双盘扩散法用于研究抗生素与提取物之间的协同作用。水晶紫法用于研究生物膜的形成。采用 SulphoRhodamine-B 检测法和 DNA 流式细胞仪来研究细胞的增殖情况以及随后细胞在细胞周期不同阶段的分布情况。流式细胞术与Annexin V-FITC/PI标记相结合,对癌细胞的凋亡期和坏死期进行了检测。使用 IBM SPSS 统计程序进行统计分析,采用单因素方差分析和 Tukey 后检验。结果M.communis的乙醇叶提取物具有很强的生长抑制作用(抑制区:20.3 ± 1.1-26.3 ± 2.5 mm,MIC:4.88-312.5 µg/mL,MBC:39.07-1250 μL):39.07-1250 μg/mL)。细菌细胞的细胞壁受到破坏被认为是产生抗霉菌作用的原因。该提取物抑制了生物膜的形成(MBIC 为 9.7 µg/mL),并根除了烟曲霉菌已经形成的成熟和超成熟生物膜,其 MBEC 值分别为 78 µg/mL 和 156 µg/mL。此外,该提取物还对乳腺癌(MCF-7)、肝癌(HepG2)、宫颈癌(HeLa)和结肠癌(HCT116)等多种癌细胞株具有很强的抗癌作用(IC50:HCT116:83 ± 2.5;HepG2:53.3 ± 0.6;MCF-7:41.5 ± 0.6;HeLa:33.3 ± 3.6),在细胞周期的 G1 阶段使细胞凋亡。结论这些结果表明,马钱子叶提取物是一种潜在的次生代谢物来源,可进一步开发为潜在的抗癌和抗霉菌药物,用于治疗各种类型的癌症和霉菌感染。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Antimycobacterial and Anticancer Properties of Myrtus communis Leaf Extract
Background: Plant-derived products or extracts are widely used in folk/traditional medicine to treat several infections, ailments, or disorders. A well-known medicinal herb, Myrtus communis is an evergreen fragrant plant native to the Mediterranean region that has been used for ages in traditional medicine around the world. Materials and methods: The microplate alamarBlue assay and the well diffusion method were used to evaluate the zone of inhibition and MIC, respectively. The double-disc diffusion method was used to investigate the synergy between antibiotics and the extract. The crystal violet method was used to investigate biofilm development. The SulphoRhodamine-B assay and DNA flow cytometry were used to investigate the proliferation and subsequent distribution of cells among different phases of the cell cycle. The apoptotic and necrotic phases of the cancer cells were examined using flow cytometry in conjunction with Annexin V-FITC/PI labeling. Using the IBM SPSS statistical program, a one-way ANOVA with Tukey’s post hoc test was employed for statistical analysis. Results: The ethanolic leaf extract of M. communis showed a strong growth inhibition effect (zone of inhibition: 20.3 ± 1.1–26.3 ± 2.5 mm, MIC: 4.88–312.5 µg/mL, and MBC: 39.07–1250 μg/mL) against several rapidly growing and slow-growing mycobacterial strains in a dose-dependent manner. Damage to the cell wall of bacterial cells was determined to be the cause of the antimycobacterial action. The extract inhibited biofilm formation (MBIC of 9.7 µg/mL) and eradicated already-formed mature and ultra-mature biofilms of M. smegmatis, with MBEC values of 78 µg/mL and 156 µg/mL, respectively. Additionally, the extract exhibited potent anticancer effects against diverse cancer cell lines of the breast (MCF-7), liver (HepG2), cervix (HeLa), and colon (HCT116) (IC50 for HCT116: 83 ± 2.5, HepG2: 53.3 ± 0.6, MCF-7: 41.5 ± 0.6, and HeLa: 33.3 ± 3.6) by apoptosis after arresting the cells in the G1 phase of the cell cycle. Conclusions: These results suggest that M. communis leaf extract is a potential source of secondary metabolites that could be further developed as potential anticancer and antimycobacterial agents to treat diverse types of cancers and mycobacterial infections.
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