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通过外周髓鞘蛋白22的转基因过表达使髓鞘组装与施万细胞分化解偶联。

Uncoupling of myelin assembly and schwann cell differentiation by transgenic overexpression of peripheral myelin protein 22.

作者信息

Niemann S, Sereda M W, Suter U, Griffiths I R, Nave K A

机构信息

Zentrum für Molekulare Biologie (ZMBH), University of Heidelberg, D-69120 Heidelberg, Germany.

出版信息

J Neurosci. 2000 Jun 1;20(11):4120-8. doi: 10.1523/JNEUROSCI.20-11-04120.2000.

Abstract

We have generated previously transgenic rats that overexpress peripheral myelin protein 22 (PMP22) in Schwann cells. In the nerves of these animals, Schwann cells have segregated with axons to the normal 1:1 ratio but remain arrested at the promyelinating stage, apparently unable to elaborate myelin sheaths. We have examined gene expression of these dysmyelinating Schwann cells using semiquantitative reverse transcription-PCR and immunofluorescence analysis. Unexpectedly, Schwann cell differentiation appears to proceed normally at the molecular level when monitored by the expression of mRNAs encoding major structural proteins of myelin. Furthermore, an aberrant coexpression of early and late Schwann cell markers was observed. PMP22 itself acquires complex glycosylation, suggesting that trafficking of the myelin protein through the endoplasmic reticulum is not significantly impaired. We suggest that PMP22, when overexpressed, accumulates in a late Golgi-cell membrane compartment and uncouples myelin assembly from the underlying program of Schwann cell differentiation.

摘要

我们之前已培育出在施万细胞中过表达外周髓磷脂蛋白22(PMP22)的转基因大鼠。在这些动物的神经中,施万细胞已与轴突以正常的1:1比例分离,但仍停滞在髓鞘形成前期,显然无法形成髓鞘。我们使用半定量逆转录聚合酶链反应和免疫荧光分析检测了这些脱髓鞘施万细胞的基因表达。出乎意料的是,当通过编码髓鞘主要结构蛋白的mRNA表达进行监测时,施万细胞分化在分子水平上似乎正常进行。此外,还观察到早期和晚期施万细胞标志物的异常共表达。PMP22自身获得了复杂的糖基化,这表明髓磷脂蛋白通过内质网的运输并未受到明显损害。我们认为,当PMP22过表达时,它会在高尔基体晚期细胞膜区室中积累,并使髓鞘组装与施万细胞分化的基础程序解偶联。

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New perspectives on the function of myelin galactolipids.髓鞘半乳糖脂功能的新视角。
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