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Toxicity of Carlina Oxide—A Natural Polyacetylene from the Carlina acaulis Roots—In Vitro and in Vivo Study

机译:Carlina的毒性-一种来自Carlina acaulis根的天然聚乙炔-体内和体外研究

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摘要

There are several reports indicating that the roots of the L. used to be commonly applied as a treatment measure in skin diseases and as an antiparasitic agent, starting from antiquity to the 19th century; however, nowadays, it has lost its importance. Currently, numerous studies are being conducted assessing the possibility of reintroducing -derived extracts to phytotherapy. Determining the safety profile of the main constituents of the plant material is crucial for achieving this goal. Here, we aimed to determine the toxicity profile of carlina oxide, one of the most abundant components of the root extract. We obtained the carlina oxide by distillation of roots in the Deryng apparatus. The purity of the standard was evaluated using GC-MS, and the identity was confirmed by IR, Raman, and NMR spectroscopy. In vitro cytotoxicity was assessed using a panel of human cell lines of skin origin, including BJ normal fibroblasts and UACC-903, UACC-647, and C32 melanoma cells. This was accompanied by an in vivo zebrafish acute toxicity test (ZFET). In vitro studies showed a toxic effect of carlina oxide, as demonstrated by an induction of apoptosis and necrosis in both normal and melanoma cells. Decreased expression of AKT kinase and extracellular signal-regulated kinase 1/2 (ERK1/2) was noted in the UACC-647 melanoma cell line. It was also observed that carlina oxide modified the expression of programmed cell death-ligand 1 (PD-L1) in tested cell lines. Carlina oxide exhibited high in vivo toxicity, with LC = 10.13 µg/mL upon the 96 h of exposure in the ZFET test. Here, we demonstrate that carlina oxide displays toxic effects to cells in culture and to living organisms. The data indicate that -based extracts considered for therapeutic use should be completely deprived of carlina oxide.
机译:有几篇报道表明,从上古到19世纪,L。的根通常被用作皮肤疾病的治疗手段和抗寄生虫剂。但是,如今,它已经失去了重要性。目前,正在进行许多研究,以评估将衍生提取物重新引入植物治疗的可能性。确定植物材料主要成分的安全性对于实现该目标至关重要。在这里,我们旨在确定氧化碳的毒性,氧化碳是根提取物中最丰富的成分之一。我们通过在Deryng装置中根部蒸馏获得氧化卡宴。使用GC-MS评估标准品的纯度,并通过IR,拉曼光谱和NMR光谱确认身份。使用一组皮肤来源的人类细胞系(包括BJ正常成纤维细胞和UACC-903,UACC-647和C32黑色素瘤细胞)评估了体外细胞毒性。伴随着体内斑马鱼急性毒性试验(ZFET)。体外研究表明,氧化钙的毒性作用已被正常和黑色素瘤细胞的凋亡和坏死诱导所证明。在UACC-647黑色素瘤细胞系中,AKT激酶和细胞外信号调节激酶1/2(ERK1 / 2)的表达降低。还观察到,在测试的细胞系中,氧化碳修饰了程序性细胞死亡配体1(PD-L1)的表达。在ZFET测试中暴露96小时后,氧化卡宴表现出很高的体内毒性,LC = 10.13 µg / mL。在这里,我们证明了氧化卡宴对培养中的细胞和活生物体显示出毒性作用。数据表明,应考虑将用于治疗用途的基于提取物的氧化钙完全剥夺。

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