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Aspergillus nidulans Cell Wall Composition and Function Change in Response to Hosting Several Aspergillus fumigatus UDP-Galactopyranose Mutase Activity Mutants

机译:Nidulans曲霉细胞壁组成和功能变化响应容纳几个烟曲霉UDP-Galactopyranose突变酶活性突变体。

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摘要

Deletion or repression of Aspergillus nidulans ugmA (AnugmA), involved in galactofuranose biosynthesis, impairs growth and increases sensitivity to Caspofungin, a β-1,3-glucan synthesis antagonist. The A. fumigatus UgmA (AfUgmA) crystal structure has been determined. From that study, AfUgmA mutants with altered enzyme activity were transformed into AnugmA▵ to assess their effect on growth and wall composition in A. nidulans. The complemented (AnugmA::wild type AfugmA) strain had wild type phenotype, indicating these genes had functional homology. Consistent with in vitro studies, AfUgmA residues R182 and R327 were important for its function in vivo, with even conservative amino (RK) substitutions producing AnugmA? phenotype strains. Similarly, the conserved AfUgmA loop III histidine (H63) was important for Galf generation: the H63N strain had a partially rescued phenotype compared to AnugmA▵. Collectively, A. nidulans strains that hosted mutated AfUgmA constructs with low enzyme activity showed increased hyphal surface adhesion as assessed by binding fluorescent latex beads. Consistent with previous qPCR results, immunofluorescence and ELISA indicated that AnugmA▵ and AfugmA-mutated A. nidulans strains had increased α-glucan and decreased β-glucan in their cell walls compared to wild type and AfugmA-complemented strains. Like the AnugmA▵ strain, A. nidulans strains containing mutated AfugmA showed increased sensitivity to antifungal drugs, particularly Caspofungin. Reduced β-glucan content was correlated with increased Caspofungin sensitivity. Aspergillus nidulans wall Galf, α-glucan, and β-glucan content was correlated in A. nidulans hyphal walls, suggesting dynamic coordination between cell wall synthesis and cell wall integrity.
机译:参与半乳糖呋喃糖生物合成的构巢曲霉ugmA(AnugmA)的缺失或抑制会损害其生长并增加对卡泊芬净(一种β-1,3-葡聚糖合成拮抗剂)的敏感性。烟曲霉UgmA(AfUgmA)晶体结构已经确定。从这项研究中,具有酶活性改变的AfUgmA突变体被转化为AnugmA▵,以评估它们对构巢曲霉生长和壁组成的影响。互补的(AnugmA ::野生型AfugmA)菌株具有野生型表型,表明这些基因具有功能同源性。与体外研究一致,AfUgmA残基R182和R327对于其在体内的功能很重要,甚至保守的氨基(RK)替代也会产生AnugmA?。表型菌株。同样,保守的AfUgmA环III组氨酸(H63)对于Galf的产生也很重要:与AnugmA▵相比,H63N菌株具有部分拯救的表型。总体而言,通过结合荧光乳胶珠评估,寄主了具有低酶活性的突变的AfUgmA构建体的构巢曲霉菌株显示出增加的菌丝表面粘附性。与以前的qPCR结果一致,免疫荧光和ELISA表明与野生型和AfugmA互补菌株相比,AnugmAug和AfugmA突变的构巢曲霉菌株在其细胞壁中具有增加的α-葡聚糖和减少的β-葡聚糖。像AnugmA▵菌株一样,含有突变的AfugmA的构巢曲霉菌株对抗真菌药物(尤其是卡泊芬净)的敏感性提高。 β-葡聚糖含量降低与卡泊芬净敏感性增加相关。构巢曲霉壁Galf,α-葡聚糖和β-葡聚糖含量与构巢曲霉菌丝壁相关,表明细胞壁合成与细胞壁完整性之间存在动态协调。

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