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Autophagy is dispensable to overcome ER stress in the filamentous fungus Aspergillus niger

机译:自噬对于克服丝状真菌黑曲霉中的内质网应激是必不可少的

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Abstract Secretory proteins are subjected to stringent quality control systems in the endoplasmic reticulum (ER) which include the targeting of misfolded proteins for proteasomal destruction via the ER-associated degradation (ERAD) pathway. Since deletion of ERAD genes in the filamentous fungus Aspergillus niger had hardly any effect on growth, this study investigates whether autophagy might function as an alternative process to eliminate misfolded proteins from the ER. We generated A. niger double mutants by deleting genes essential for ERAD ( derA ) and autophagy ( atg1 or atg8 ), and assessed their growth both under normal and ER stress conditions. Sensitivity toward ER stress was examined by treatment with dithiothreitol (DTT) and by expressing a mutant form of glucoamylase (mtGlaA::GFP) in which disulfide bond sites in GlaA were mutated. Misfolding of mtGlaA::GFP was confirmed, as mtGlaA::GFP accumulated in the ER. Expression of mtGlaA::GFP in ERAD and autophagy mutants resulted in a twofold higher accumulation in ????derA and ????derA????atg1 strains compared to ????atg1 and wild type. As ????derA????atg1 mutants did not show increased sensitivity toward DTT, not even when mtGlaA::GFP was expressed, the results indicate that autophagy does not act as an alternative pathway in addition to ERAD for removing misfolded proteins from the ER in A. niger .
机译:摘要分泌蛋白在内质网(ER)中受到严格的质量控制体系的控制,包括通过ER相关降解(ERAD)途径靶向错误折叠的蛋白以进行蛋白酶体破坏。由于丝状真菌黑曲霉中ERAD基因的缺失几乎对生长没有任何影响,因此本研究调查自噬是否可以作为消除ER中错误折叠蛋白的替代方法。我们通过删除ERAD(derA)和自噬(atg1或atg8)必需的基因产生了黑曲霉双突变体,并评估了它们在正常和内质网应激条件下的生长。通过用二硫苏糖醇(DTT)处理并表达葡糖淀粉酶的突变形式(mtGlaA :: GFP)来检查对ER应激的敏感性,其中GlaA中的二硫键位点发生了突变。确认mtGlaA :: GFP的错误折叠,因为mtGlaA :: GFP在ER中积累。 mtGlaA :: GFP在ERAD和自噬突变体中的表达导致与Δtg1和野生型相比,ΔtderA和ΔderAΔtatg1菌株中的蓄积高两倍。由于即使在表达mtGlaA :: GFP的情况下,derA ??? atg1突变体也未显示出对DTT的敏感性增加,结果表明自噬除ERAD以外不作为替代途径去除错误折叠的蛋白质。来自黑曲霉的急诊室。

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