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Targeting CpG DNA to screen and isolate anti-sepsis fraction and monomers from traditional Chinese herbs using affinity biosensor technology.

机译:使用亲和生物传感器技术靶向CpG DNA来筛选和分离中草药中的防腐成分和单体。

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摘要

Bacterial DNA/CpG DNA is recognized as a key molecule during the pathogenesis of sepsis. Therefore, preventing CpG DNA from binding to its receptor is considered as the most promising strategy. In the present experiments, Radix et Rhizoma Rhei had the highest CpG DNA-binding ability among the seventy-eight traditional Chinese herbs. After the isolation of silica gel chromatography and high performance liquid chromatography (HPLC) and evaluation with affinity biosensor, the active fraction was confirmed and named Fraction D. It was found that in vitro, Fraction D bound to both CpG DNA and lipid A with high affinity, and strongly inhibited LPS- and CpG DNA-induced TNF-alpha release from RAW264.7 cells in a dose-dependent manner. Furthermore, Fraction D reduced the expression of TLR9 mRNA up-regulated by CpG DNA. In vivo, Fraction D protected mice challenged with lethal heat-killed E. coli. Using HPLC method, two monomers with high affinity for CpG DNA were isolated and identified as rhein and emodin. Rhein could significantly reduce CpG DNA- and LPS-induced TNF-alpha release, but emodin only reduced CpG DNA-induced TNF-alpha release. Rhein in combination with emodin could play synergistic inhibitory effect on both CpG DNA and LPS-induced TNF-alpha release, which contributed to the bioactivity of Fraction D. In conclusion, we successfully established the platform to screen anti-CpG DNA components of traditional Chinese herbs using affinity biosensor technology, got active Fraction D from Radix et Rhizoma Rhei and determined rhein and emodin as the main bioactive ingredients in Fraction D.
机译:细菌DNA / CpG DNA被认为是脓毒症发病过程中的关键分子。因此,防止CpG DNA与其受体结合被认为是最有前途的策略。在目前的实验中,大黄等在七十八种中草药中具有最高的CpG DNA结合能力。分离硅胶色谱和高效液相色谱(HPLC),并用亲和生物传感器评估后,确认了活性级分,并命名为馏分D。发现在体外,馏分D与CpG DNA和脂质A结合的程度很高。亲和力,并以剂量​​依赖的方式强烈抑制LPS和CpG DNA诱导的TNF-α从RAW264.7细胞释放。此外,级分D减少了由CpG DNA上调的TLR9 mRNA的表达。在体内,级分D保护了用致死性热杀死大肠杆菌攻击的小鼠。使用HPLC方法,分离出对CpG DNA具有高亲和力的两种单体,并将其鉴定为大黄酸和大黄素。大黄酸可以显着降低CpG DNA和LPS诱导的TNF-α释放,但是大黄素只能降低CpG DNA诱导的TNF-α释放。大黄酸与大黄素联用对CpG DNA和LPS诱导的TNF-α释放均具有协同抑制作用,这有助于组分D的生物活性。总之,我们成功建立了筛选中国传统抗CpG DNA成分的平台草药使用亲和生物传感器技术,从Radix et Rhizoma Rhei获得了活性级分D,并确定了大黄酸和大黄素是级分D中的主要生物活性成分。

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