首页> 外文期刊>Journal of Applied Glycoscience >Characterization of Cell Wall α-1,3-Glucan–Deficient Mutants in Aspergillus oryzae Isolated by a Screening Method Based on Their Sensitivities to Congo Red or Lysing Enzymes
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Characterization of Cell Wall α-1,3-Glucan–Deficient Mutants in Aspergillus oryzae Isolated by a Screening Method Based on Their Sensitivities to Congo Red or Lysing Enzymes

机译:基于对刚果红或裂解酶的敏感性筛选方法筛选米曲霉细胞壁α-1,3-葡聚糖缺陷型突变体

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We previously reported that sensitivity to Congo Red (CR) or Lysing Enzymes (LE) is affected by the loss of cell-wall α-1,3-glucan (AG) in Aspergillus nidulans. We found that the amount of CR adsorbed to AG was significantly less than the amount adsorbed to β-1,3-glucan (BG) or chitin, suggesting that loss of cell-wall AG would increase exposure of BG on the cell surface, and thereby increase the sensitivity to CR. Generally, fungal BGs are known as biological response modifiers because of their recognition by Dectin-1 receptors in human immune systems. Therefore, isolation of AG-deficient mutants in Aspergillus oryzae has been used in the Japanese fermentation industry to create strains with increased ability to promote immune responses. Here, we aimed to isolate AG-deficient strains by mutagenizing A. oryzae conidia with chemical mutagens. Based on the increased sensitivity to CR in AG-deficient strains of A. nidulans and A. oryzae, we established a screening method for isolation of AG-deficient strains. Several candidate AG-deficient mutants of A. oryzae were isolated using the screening method; these strains showed increased sensitivity to CR and/or LE. Cytokine production was increased in the dendritic cells co-incubated with germinated conidia of the AG-deficient mutants. Furthermore, according to a Dectin-1 NFAT (nuclear factor of activator T cells)-GFP (green fluorescent protein) reporter assay, Dectin-1 response levels in the AG-deficient mutants were higher than those in wild-type A. oryzae. These results suggest that we successfully isolated AG-deficient mutants of A. oryzae with immunostimulatory effects.
机译:我们以前曾报道过,构巢曲霉中细胞壁α-1,3-葡聚糖(AG)的损失会影响对刚果红(CR)或裂解酶(LE)的敏感性。我们发现,吸附到AG上的CR的量明显少于吸附到β-1,3-葡聚糖(BG)或几丁质的量,这表明细胞壁AG的丢失会增加BG在细胞表面的暴露,并且从而增加了对CR的敏感性。通常,由于真菌BG被人体免疫系统中的Dectin-1受体识别,因此被称为生物反应修饰剂。因此,在日本发酵工业中已经使用了米曲霉中AG缺陷型突变体的分离,以产生具有增强的免疫反应能力的菌株。在这里,我们旨在通过用化学诱变剂诱变米曲霉分生孢子来分离AG缺陷菌株。基于构巢曲霉和米曲霉AG缺陷菌株对CR的敏感性提高,我们建立了一种筛选AG缺陷菌株的筛选方法。使用筛选方法分离了几个候选的AG缺陷型米曲霉突变体。这些菌株显示出对CR和/或LE的敏感性增加。与AG缺陷型突变体的萌发分生孢子共孵育的树突状细胞中细胞因子的产生增加。此外,根据Dectin-1 NFAT(激活性T细胞的核因子)-GFP(绿色荧光蛋白)报告基因检测,AG缺陷型突变体中的Dectin-1响应水平高于野生型米曲霉。这些结果表明,我们成功分离了具有免疫刺激作用的米曲霉AG缺陷型突变体。

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