首页> 美国卫生研究院文献>Cannabis and Cannabinoid Research >Identification of Synergistic Interaction Between Cannabis-Derived Compounds for Cytotoxic Activity in Colorectal Cancer Cell Lines and Colon Polyps That Induces Apoptosis-Related Cell Death and Distinct Gene Expression
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Identification of Synergistic Interaction Between Cannabis-Derived Compounds for Cytotoxic Activity in Colorectal Cancer Cell Lines and Colon Polyps That Induces Apoptosis-Related Cell Death and Distinct Gene Expression

机译:大麻衍生化合物在大肠癌细胞系和结肠息肉中诱导细胞凋亡相关细胞死亡和不同基因表达的细胞毒性活性之间的协同相互作用的鉴定。

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摘要

>Introduction: Colorectal cancer remains the third most common cancer diagnosis and fourth leading cause of cancer-related mortality worldwide. Purified cannabinoids have been reported to prevent proliferation, metastasis, and induce apoptosis in a variety of cancer cell types. However, the active compounds from Cannabis sativa flowers and their interactions remain elusive.>Research Aim: This study was aimed to specify the cytotoxic effect of C. sativa-derived extracts on colon cancer cells and adenomatous polyps by identification of active compound(s) and characterization of their interaction.>Materials and Methods: Ethanol extracts of C. sativa were analyzed by high-performance liquid chromatography and gas chromatograph/mass spectrometry and their cytotoxic activity was determined using alamarBlue-based assay (Resazurin) and tetrazolium dye-based assay (XTT) on cancer and normal colon cell lines and on dysplastic adenomatous polyp cells. Annexin V Assay and fluorescence-activated cell sorting (FACS) were used to determine apoptosis and cell cycle, and RNA sequencing was used to determine gene expression.>Results: The unheated cannabis extracts (C2F), fraction 7 (F7), and fraction 3 (F3) had cytotoxic activity on colon cancer cells, but reduced activity on normal colon cell lines. Moreover, synergistic interaction was found between F7 and F3 and the latter contains mainly cannabigerolic acid. The F7 and F7+F3 cytotoxic activity involved cell apoptosis and cell cycle arrest in S or G0/G1 phases, respectively. RNA profiling identified 2283 differentially expressed genes in F7+F3 treatment, among them genes related to the Wnt signaling pathway and apoptosis-related genes. Moreover, F7, F3, and F7+F3 treatments induced cell death of polyp cells.>Conclusions: C. sativa compounds interact synergistically for cytotoxic activity against colon cancer cells and induce cell cycle arrest, apoptotic cell death, and distinct gene expression. F3, F7, and F7+F3 are also active on adenomatous polyps, suggesting possible future therapeutic value.
机译:>简介:结直肠癌仍然是全球第三大最常见的癌症诊断方法,也是癌症相关死亡率的第四大诱因。据报道,纯化的大麻素可预防多种癌细胞类型的增殖,转移并诱导细胞凋亡。然而,来自大麻花的活性化合物及其相互作用仍然难以捉摸。>研究目的:本研究旨在通过鉴定鉴定苜蓿提取物对结肠癌细胞和腺瘤性息肉的细胞毒性作用。 >材料和方法:高效液相色谱法和气相色谱/质谱法分析苜蓿的乙醇提取物,并用高效液相色谱法测定其细胞毒活性。基于alamarBlue的测定法(Resazurin)和基于四唑鎓染料的测定法(XTT)用于癌症和正常结肠细胞系以及异常增生的腺瘤性息肉细胞。 >结果:未加热的大麻提取物(C2F),馏分7,用膜联蛋白V测定法和荧光激活细胞分选术(FACS)确定细胞凋亡和细胞周期,并用RNA测序确定基因表达。 (F7)和级分3(F3)对结肠癌细胞具有细胞毒活性,但对正常结肠细胞系的活性降低。此外,在F7和F3之间发现了协同相互作用,而后者主要包含大麻二酸。 F7和F7 + F3细胞毒活性分别涉及S或G0 / G1期的细胞凋亡和细胞周期停滞。 RNA谱分析在F7 + F3处理中鉴定了2283个差异表达的基因,其中包括与Wnt信号通路和凋亡相关基因相关的基因。此外,F7,F3和F7 + F3处理可诱发息肉细胞死亡。>结论:苜蓿化合物可协同相互作用,对结肠癌细胞产生细胞毒活性,并诱导细胞周期停滞,凋亡性细胞死亡,和独特的基因表达F3,F7和F7 + F3在腺瘤性息肉上也有活性,提示其未来的治疗价值。

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