Pharmacological assessment of the extract and a novel compound of Bacillus velezensis DM derived from the rhizosphere of Datura metel L. with microbial molecular screening.

IF 3.3 2区医学 Q1 INTEGRATIVE & COMPLEMENTARY MEDICINE

BMC Complementary Medicine and Therapies Pub Date : 2025-04-26 DOI:10.1186/s12906-025-04879-x

Mohamed A Awad, Shahenda Mahgoub, Hesham S M Soliman, Sherif F Hammad

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Abstract

Background: Rhizosphere bacteria were considered a prospective reservoir of bioactive compounds with significant pharmacological efficacy.

Methods: From the rhizosphere of Datura metel L., Bacillus velezensis DM was isolated and characterized using 16 S rRNA. PCR screening and sequencing were conducted to identify genes related to bioactive metabolite production. The extraction of secondary metabolites from the bacterial strain was performed via a fermentation process. The ethyl acetate extract of the propagated strain was subjected to fractionation and purification through various chromatographic techniques. The characterization of the isolated compounds was accomplished using different spectroscopic methods, such as 1D and 2D-NMR. An MTT test was conducted to assess the cytotoxic activity of bacterial extract on MCF-7, HepG-2, and HCT-116 cells. Furthermore, its pure compound (1) was tested for its cytotoxicity on HCT-116 and a normal cell (THLE2) to test its safety for normal cells. Apoptosis was identified through flow cytometry on HCT-116 cells after double-staining with PI and annexin V-FITC. The antioxidant action of bacterial extract was assessed through DPPH and ABTS assays. Furthermore, anti-inflammatory evaluations were carried out employing lipoxygenase (5-LOX) and cyclooxygenase (COX-2) inhibition.

Results: The NCBI GenBank database has effectively incorporated the 16 S rRNA gene sequence of Bacillus velezensis DM under the accession number OR364492. Polyketide synthase and two lipopeptide genes for surfactin and iturin A were effectively detected by PCR, and their sequences were included in the Genbank database. A novel compound, 5,6-di(methylamino)hex-5-ene-1,2,3-triol (1), was successfully separated from the strain. Bacterial extract demonstrated significant cytotoxic activity against the evaluated cancer cells, exhibiting the most pronounced effect on HCT-116 cells. Compound (1) showed promising cytotoxic potential against HCT-116 cells with a higher selectivity index (2.5) towards cancer cells in comparison to Doxorubicin (1.49). Apoptosis assay showed that bacterial extract caused apoptosis about 14 folds compared to the control HCT-116 cells. Furthermore, it showed a potent anti-inflammatory outcome (IC₅₀ = 1.927 µg/mL) and antioxidant activity at IC₅₀ of 76.8 µg/mL.

Conclusion: This study revealed the possible pharmacological effects of secondary metabolites generated by Bacillus velezensis DM, making it a valuable resource for isolating bioactive compounds with potential therapeutic and biomedical uses.

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曼陀罗根际提取物及新化合物velezensis DM的药理作用及微生物分子筛选。

背景：根际细菌被认为是具有显著药理功效的生物活性化合物的潜在储存库。方法：从曼陀罗根际分离分离velezensis DM，并利用16s rRNA对其进行鉴定。进行PCR筛选和测序，以确定与生物活性代谢物产生相关的基因。通过发酵过程从菌株中提取次生代谢物。通过各种色谱技术对繁殖菌株的乙酸乙酯提取物进行分离纯化。分离化合物的表征是通过不同的光谱方法完成的，如1D和2D-NMR。采用MTT试验评估细菌提取物对MCF-7、HepG-2和HCT-116细胞的细胞毒活性。此外，对其纯化合物(1)对HCT-116和正常细胞（THLE2）的细胞毒性进行了测试，以检验其对正常细胞的安全性。经PI和膜联蛋白V-FITC双染色，流式细胞术检测HCT-116细胞凋亡。通过DPPH和ABTS测定细菌提取物的抗氧化作用。此外，通过抑制脂氧合酶（5-LOX）和环氧合酶（COX-2）进行抗炎评价。结果：NCBI GenBank数据库有效纳入了芽孢杆菌（Bacillus velezensis DM）的16s rRNA基因序列，登录号为OR364492。聚合酶链反应（PCR）有效检测到surfactin和iturin A的聚酮合成酶和两个脂肽基因，并将其序列纳入Genbank数据库。新化合物5,6-二（甲氨基）己-5-烯-1,2,3-三醇(1)从该菌株中分离得到。细菌提取物对肿瘤细胞具有显著的细胞毒活性，其中对HCT-116细胞的作用最为明显。与阿霉素（1.49）相比，化合物(1)对癌细胞具有更高的选择性指数（2.5），对HCT-116细胞具有潜在的细胞毒性。细胞凋亡实验显示，细菌提取物引起HCT-116细胞的凋亡约为对照细胞的14倍。抗炎IC50为1.927µg/mL，抗氧化IC50为76.8µg/mL。结论：本研究揭示了velezensis DM次生代谢产物可能具有的药理作用，为分离具有潜在治疗和生物医学用途的生物活性化合物提供了宝贵的资源。

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