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高尔基糖基转移酶的非酶功能:通过与非肌肉肌球蛋白 IIA 的相互作用介导高尔基体碎片化。

A non-enzymatic function of Golgi glycosyltransferases: mediation of Golgi fragmentation by interaction with non-muscle myosin IIA.

机构信息

Department of Research Service, VA Nebraska-Western Iowa Health Care System, Omaha, NE 68105 USA.

出版信息

Glycobiology. 2013 Jun;23(6):690-708. doi: 10.1093/glycob/cwt009. Epub 2013 Feb 7.

Abstract

The Golgi apparatus undergoes morphological changes under stress or malignant transformation, but the precise mechanisms are not known. We recently showed that non-muscle myosin IIA (NMIIA) binds to the cytoplasmic tail of Core 2 N-acetylglucosaminyltransferase mucus-type (C2GnT-M) and transports it to the endoplasmic reticulum for recycling. Here, we report that Golgi fragmentation induced by brefeldin A (BFA) or coatomer protein (β-COP) knockdown (KD) in Panc1-bC2GnT-M (c-Myc) cells is accompanied by the increased association of NMIIA with C2GnT-M and its degradation by proteasomes. Golgi fragmentation is prevented by inhibition or KD of NMIIA. Using multiple approaches, we have shown that the speed of BFA-induced Golgi fragmentation is positively correlated with the levels of this enzyme in the Golgi. The observation is reproduced in LNCaP cells which express high levels of two endogenous glycosyltransferases--C2GnT-L and β-galactoside α2,3 sialyltransferase 1. NMIIA is found to form complexes with these two enzymes but not Golgi matrix proteins. The KD of both enzymes or the prevention of Golgi glycosyltransferases from exiting endoplasmic reticulum reduced Golgi-associated NMIIA and decreased the BFA-induced fragmentation. Interestingly, the fragmented Golgi detected in colon cancer HT-29 cells can be restored to a compact morphology after inhibition or KD of NMIIA. The Golgi disorganization induced by the microtubule or actin destructive agent is NMIIA-independent and does not affect the levels of glycosyltransferases. We conclude that NMIIA interacts with Golgi residential but not matrix proteins, and this interaction is responsible for Golgi fragmentation induced by β-COP KD or BFA treatment. This is a novel non-enzymatic function of Golgi glycosyltransferases.

摘要

高尔基复合体在应激或恶性转化下会发生形态变化,但确切的机制尚不清楚。我们最近表明,非肌肉肌球蛋白 IIA(NMIIA)与核心 2 N-乙酰葡萄糖胺基转移酶粘液型(C2GnT-M)的细胞质尾巴结合,并将其运输到内质网进行回收。在这里,我们报告说,在 Panc1-bC2GnT-M(c-Myc)细胞中,布雷菲德菌素 A(BFA)或衣壳蛋白(β-COP)敲低(KD)诱导的高尔基碎片化伴随着 NMIIA 与 C2GnT-M 的增加关联及其被蛋白酶体降解。NMIIA 的抑制或 KD 可防止高尔基碎片化。通过多种方法,我们已经表明,BFA 诱导的高尔基碎片化速度与该酶在高尔基中的水平呈正相关。这一观察结果在表达两种内源性糖基转移酶--C2GnT-L 和 β-半乳糖苷 α2,3 唾液酸转移酶 1 的 LNCaP 细胞中得到重现。NMIIA 被发现与这两种酶形成复合物,但不与高尔基基质蛋白形成复合物。两种酶的 KD 或防止高尔基糖基转移酶从内质网逸出会减少高尔基相关的 NMIIA,并减少 BFA 诱导的碎片化。有趣的是,在结肠癌细胞 HT-29 中检测到的碎片化高尔基在抑制或 KD NMIIA 后可以恢复到紧凑的形态。微管或肌动蛋白破坏剂诱导的高尔基紊乱与 NMIIA 无关,也不影响糖基转移酶的水平。我们得出结论,NMIIA 与高尔基驻留蛋白而不是基质蛋白相互作用,这种相互作用是由 β-COP KD 或 BFA 处理诱导的高尔基碎片化的原因。这是高尔基糖基转移酶的一种新的非酶功能。

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