Present address: Department of Neurodegenerative Disease, Institute of Neurology, UCL, Queen Square, London WC1N 3BG, UK.
Hum Mol Genet. 2011 Jun 1;20(11):2081-90. doi: 10.1093/hmg/ddr081. Epub 2011 Mar 1.
More than 120 mutations in the Myelin Protein Zero gene (MPZ, P0) cause various forms of hereditary neuropathy. Two human mutations encoding either P0S63C or P0S63del have been shown to cause demyelination in mice through different gain of function pathomechanisms. P0S63del, for example, is retained in the endoplasmic reticulum (ER) and elicits a pathogenetic unfolded protein response (UPR). As P0 likely forms oligomers, another gain of abnormal function could include a dominant-negative interaction between P0S63del and normal P0 (P0wt). To test this idea, we generated a transgenic mouse that expressed a form of P0wt with a myc epitope tag at the C terminus (P0ct-myc). We show that P0ct-myc is trafficked and functions like P0wt, thus providing a new tool to study P0 in vivo. In mice that express both P0ct-myc and P0S63del, P0S63del specifically delays the transit of P0ct-myc through the ER and reduces the level of P0wt in the myelin sheath by half-a level previously shown to cause demyelination in mice and humans. Surprisingly, P0ct-myc does not co-immunoprecipitate with P0S63del, suggesting an indirect interaction. Thus, P0S63del causes not only a UPR-related toxic mechanism, but also a dominant-negative effect on P0wt that probably contributes to demyelinating neuropathy.
超过 120 种髓鞘蛋白零基因 (MPZ,P0) 的突变导致各种形式的遗传性神经病。已经证明,两种人类突变,分别编码 P0S63C 或 P0S63del,通过不同的功能获得机制在小鼠中引起脱髓鞘。例如,P0S63del 保留在内质网 (ER) 中,并引发致病的未折叠蛋白反应 (UPR)。由于 P0 可能形成寡聚体,另一种异常功能的获得可能包括 P0S63del 和正常 P0 (P0wt) 之间的显性负相互作用。为了验证这一观点,我们生成了一种表达 P0wt 的转基因小鼠,其 C 末端带有 myc 表位标签 (P0ct-myc)。我们表明 P0ct-myc 是可运输的,并且像 P0wt 一样发挥作用,因此为在体内研究 P0 提供了一种新工具。在同时表达 P0ct-myc 和 P0S63del 的小鼠中,P0S63del 特异性延迟 P0ct-myc 通过 ER 的转运,并使 P0wt 在髓鞘中的水平降低一半-先前在小鼠和人类中显示出导致脱髓鞘的水平。令人惊讶的是,P0ct-myc 不会与 P0S63del 共同免疫沉淀,这表明存在间接相互作用。因此,P0S63del 不仅引起与 UPR 相关的毒性机制,而且对 P0wt 还具有显性负效应,这可能导致脱髓鞘性神经病。
