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Structure of a β-glucan from Grifola frondosa and its antitumor effect by activating Dectin-1/Syk/NF-κB signaling

机译:灰树花β-葡聚糖的结构及其通过激活Dectin-1 / Syk /NF-κB信号传导的抗肿瘤作用

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摘要

A soluble homogeneous β-glucan, GFPBW1, with a molecular mass of 300 kDa was purified from the fraction of the fruit bodies of Grifola frondosa extracted with 5 % NaOH. Using various methods, such as infrared spectroscopy, NMR, methylation and monosaccharide composition analysis, its structure was determined to be a β-D- (1-3)-linked glucan backbone with a single β-D-(1-6)- linked glucopyranosyl residue branched at C-6 on every third residue. It induced TNF-a and IL-6 production and the activation of Syk and NF-κB signaling in resident peritoneal macrophages from ICR mice, which could be significantly inhibited by the blocking reagent laminarin. A competitive phagocytosis assay with FITC-zymosan indicated that GFPBW1 could bind to DC-associated C-type lectin 1 (Dectin-1). The TNF-a secretion and activation of Syk/NF-κB signaling triggered by GFPBW1 were enhanced in RAW264.7 cells overexpressing wild but not mutant (δ38 and Y15S) Dectin-1. Furthermore, GFPBW1 potentiated the Concanavalin A-induced proliferative response of splenocytes and inhibited Sarcoma-180 growth allografted in ICR mice but not in immunodeficient BALB/c nuu mice. These results suggested that the antitumor activity of GFPBW1 was partially associated with the activation of macrophages via the Dectin-1/Syk/NF-κB signaling pathway. This molecule could be a promising biological response modifier with clear application for antitumor therapies.
机译:从用5%NaOH提取的灰树花的子实体部分中纯化出分子量为300 kDa的可溶性均质β-葡聚糖GFPBW1。使用多种方法,例如红外光谱,NMR,甲基化和单糖组成分析,确定其结构为具有单个β-D-(1-6)-的β-D-(1-3)-连接的葡聚糖骨架。连接的吡喃葡萄糖基残基在每三个残基的C-6处分支。它诱导了ICR小鼠体内腹膜巨噬细胞中TNF-a和IL-6的产生以及Syk和NF-κB信号的激活,这可能被阻断剂层板蛋白显着抑制。用FITC-zymosan进行的竞争性吞噬实验表明,GFPBW1可以与DC相关的C型凝集素1(Dectin-1)结合。 GFPBW1触发的TNF-a分泌和Syk /NF-κB信号的激活在过表达野生但未突变的(δ38和Y15S)Dectin-1的RAW264.7细胞中得到增强。此外,GFPBW1增强了伴刀豆球蛋白A诱导的脾细胞增殖反应,并抑制了同种异体移植到ICR小鼠中的肉瘤180生长,但在免疫缺陷的BALB / c nu / nu小鼠中却没有。这些结果表明,GFPBW1的抗肿瘤活性与通过Dectin-1 / Syk /NF-κB信号通路的巨噬细胞活化部分相关。该分子可能是一种有前途的生物反应修饰剂,在抗肿瘤治疗中有明确的应用。

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