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N-Glycanase 1 Transcriptionally Regulates Aquaporins Independent of Its Enzymatic Activity

机译:N-糖酵素1转录调节水通道蛋白,与其酶活性无关。

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Patients with pathogenic mutations in NGLY1 cannot make tears and have global developmental delay and liver dysfunction. Traditionally, NGLY1 cleaves intact N-glycans from misfolded, retrotranslocated glycoproteins before proteasomal degradation. We demonstrate that Ngly1- null mouse embryonic fibroblasts, NGLY1 knockout human cells, and patient fibroblasts are resistant to hypotonic lysis. Ngly1 -deficient mouse embryonic fibroblasts swell slower and have reduced aquaporin1 mRNA and protein expression. Ngly1 knockdown and overexpression confirms that Ngly1 regulates aquaporin1 and hypotonic cell lysis. Patient fibroblasts and NGLY1 knockout cells?show reduced aquaporin11 mRNA, supporting NGLY1 as regulating expression of multiple aquaporins across species. Complementing Ngly1 -deficient cells with catalytically inactive NGLY1 (p.Cys309Ala) restores normal hypotonic lysis and aquaporin1 protein. We show that transcription factors Atf1/Creb1 regulate aquaporin1 and that the Atf1/Creb1 signaling pathway is disrupted in Ngly1 -deficient mouse embryonic fibroblasts. These results identify a non-enzymatic, regulatory function of NGLY1 in aquaporin transcription, possibly related to alacrima and neurological symptoms.
机译:NGLY1中具有致病性突变的患者不能流泪,并且具有整体发育迟缓和肝功能障碍。传统上,NGLY1在蛋白酶体降解之前会从错误折叠的逆转位糖蛋白上切割完整的N-聚糖。我们证明Ngly1- null小鼠胚胎成纤维细胞,NGLY1基因敲除人类细胞和患者成纤维细胞对低渗裂解​​有抗性。缺乏Ngly1的小鼠胚胎成纤维细胞膨胀较慢,并且水通道蛋白1 mRNA和蛋白质表达降低。 Ngly1敲低和过度表达证实Ngly1调节Aquaporin1和低渗细胞裂解。患者的成纤维细胞和NGLY1敲除细胞显示出减少的aquaporin11 mRNA,支持NGLY1调节跨物种的多种aquaporin的表达。 Ngly1缺陷细胞与无催化活性的NGLY1(p.Cys309Ala)互补,可恢复正常的低渗裂解和aquaporin1蛋白。我们表明,转录因子Atf1 / Creb1调节水通道蛋白1,并且Atf1 / Creb1信号通路在Ngly1缺陷型小鼠胚胎成纤维细胞中被破坏。这些结果确定了NGLY1在水通道蛋白转录中的非酶调控功能,这可能与红皮病和神经系统症状有关。

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