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血清剥夺通过蛋白酶体和溶酶体途径下调 PC12 细胞中的神经酰胺激酶:神经生长因子的保护作用及其在胞吐作用中的作用。

Down-regulation of ceramide kinase via proteasome and lysosome pathways in PC12 cells by serum withdrawal: Its protection by nerve growth factor and role in exocytosis.

机构信息

Laboratory of Chemical Pharmacology, Graduate School of Pharmaceutical Sciences, Chiba University, Chiba, Japan.

Laboratory of Chemical Pharmacology, Graduate School of Pharmaceutical Sciences, Chiba University, Chiba, Japan; Research Coordination Group, Research Management Department, DaiichiSankyo RD Novare Co., Ltd., 1016-13 Kitakasai, Edogawa-ku, Tokyo 134-8630, Japan.

出版信息

Biochim Biophys Acta Mol Cell Res. 2020 Jul;1867(7):118714. doi: 10.1016/j.bbamcr.2020.118714. Epub 2020 Apr 1.

DOI:10.1016/j.bbamcr.2020.118714
PMID:32246947
Abstract

Ceramide kinase (CerK) phosphorylates ceramide to ceramide-1-phosphate (C1P). CerK is highly expressed in the brain, and its association with the neuronal function has been reported. Previous reports showed that the activity of CerK is regulated by post-translational modifications including phosphorylation, whereas the cellular fate of CerK protein and its role in neuronal functions have not been clearly elucidated. Therefore, we investigated these issues in PC12 cells. Treatment with nerve growth factor (NGF) for 6 h increased the formation of C1P but not CerK mRNA. Knockdown of CerK and overexpression of HA-tagged CerK down- and up-regulated the formation of C1P, respectively. In PC12-CerK-HA cells, serum withdrawal caused ubiquitination of CerK-HA protein and down-regulated both CerK-HA protein and C1P formation within 6 h, and these down-regulations were abolished by co-treatments with NGF or proteasome inhibitors such as MG132 and clasto-lactacystin. Microscopic analysis showed that treatment with the proteasome inhibitors increased CerK-HA in puncture structures, possibly endosomes and/or vesicles, in cells. Treatment with the lysosome inhibitors reduced serum withdrawal-induced down-regulation of CerK-HA protein but not C1P formation. When knockdown or overexpression of CerK was performed, Ca-induced release of [H] noradrenaline was reduced or enhanced, respectively, but neurite extension was not modified. There was a positive correlation between noradrenaline release and formation of C1P and/or CerK-HA levels in NGF- and clasto-lactacystin-treated cells. These results suggest that levels of CerK were down-regulated by the ubiquitin/proteasome and lysosome pathways and the former pathway-sensitive pool of CerK was suggested to be linked with exocytosis in PC12 cells.

摘要

神经酰胺激酶(CerK)将神经酰胺磷酸化为神经酰胺-1-磷酸(C1P)。CerK 在大脑中高度表达,其与神经元功能的关系已被报道。先前的报告表明,CerK 的活性受包括磷酸化在内的翻译后修饰调节,但其 CerK 蛋白的细胞命运及其在神经元功能中的作用尚未明确阐明。因此,我们在 PC12 细胞中研究了这些问题。用神经生长因子(NGF)处理 6 小时增加了 C1P 的形成,但不增加 CerK mRNA 的形成。CerK 的敲低和 HA 标记的 CerK 的过表达分别下调和上调了 C1P 的形成。在 PC12-CerK-HA 细胞中,血清剥夺导致 CerK-HA 蛋白的泛素化,并在 6 小时内下调 CerK-HA 蛋白和 C1P 的形成,这些下调作用被 NGF 或蛋白酶体抑制剂如 MG132 和 clasto-lactacystin 的共同处理所消除。显微镜分析显示,用蛋白酶体抑制剂处理会增加细胞中 CerK-HA 在穿刺结构中的含量,这些结构可能是内体和/或囊泡。用溶酶体抑制剂处理会减少血清剥夺诱导的 CerK-HA 蛋白下调,但不会减少 C1P 的形成。当 CerK 被敲低或过表达时,Ca2+诱导的[H]去甲肾上腺素释放分别减少或增强,但神经突延伸没有改变。在 NGF 和 clasto-lactacystin 处理的细胞中,去甲肾上腺素释放与 C1P 和/或 CerK-HA 水平之间存在正相关。这些结果表明,CerK 水平通过泛素/蛋白酶体和溶酶体途径下调,并且 CerK 的前一种途径敏感池与 PC12 细胞中的胞吐作用有关。

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