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GnTI 的高尔基定位需要其跨膜结构域内的一个极性氨基酸残基。

The Golgi Localization of GnTI Requires a Polar Amino Acid Residue within Its Transmembrane Domain.

机构信息

Department of Applied Genetics and Cell Biology, University of Natural Resources and Life Sciences, Muthgasse 18, A-1190 Vienna, Austria.

Department of Chemistry, University of Natural Resources and Life Sciences, Muthgasse 18, A-1190 Vienna, Austria.

出版信息

Plant Physiol. 2019 Jun;180(2):859-873. doi: 10.1104/pp.19.00310. Epub 2019 Apr 10.

DOI:10.1104/pp.19.00310
PMID:30971450
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC6548254/
Abstract

The Golgi apparatus consists of stacked cisternae filled with enzymes that facilitate the sequential and highly controlled modification of glycans from proteins that transit through the organelle. Although the glycan processing pathways have been extensively studied, the underlying mechanisms that concentrate Golgi-resident glycosyltransferases and glycosidases in distinct Golgi compartments are poorly understood. The single-pass transmembrane domain (TMD) of n-acetylglucosaminyltransferaseI (GnTI) accounts for its steady-state distribution in the cis/medial-Golgi. Here, we investigated the contribution of individual amino acid residues within the TMD of Arabidopsis () and GnTI toward Golgi localization and n-glycan processing. Conserved sequence motifs within the TMD were replaced with those from the established trans-Golgi enzyme α2,6-sialyltransferase and site-directed mutagenesis was used to exchange individual amino acid residues. Subsequent subcellular localization of fluorescent fusion proteins and n-glycan profiling revealed that a conserved Gln residue in the GnTI TMD is essential for its cis/medial-Golgi localization. Substitution of the crucial Gln residue with other amino acids resulted in mislocalization to the vacuole and impaired n-glycan processing in vivo. Our results suggest that sequence-specific features of the GnTI TMD are required for its interaction with a Golgi-resident adaptor protein or a specific lipid environment that likely promotes coat protein complexI-mediated retrograde transport, thus maintaining the steady-state distribution of GnTI in the cis/medial-Golgi of plants.

摘要

高尔基氏体由堆叠的潴泡组成,充满了酶,这些酶有助于从穿过细胞器的蛋白质中顺序且高度受控地修饰聚糖。尽管糖基化途径已被广泛研究,但将高尔基体驻留的糖基转移酶和糖苷酶集中在不同的高尔基体隔室中的基本机制仍知之甚少。N-乙酰氨基葡萄糖基转移酶 I(GnTI)的单次跨膜结构域(TMD)解释了其在顺面/中间高尔基体内的稳定分布。在这里,我们研究了拟南芥()和 GnTI 的 TMD 中单个氨基酸残基对高尔基体定位和 n-糖基化加工的贡献。TMD 中的保守序列基序被来自已建立的跨高尔基酶 α2,6-唾液酸转移酶的序列基序取代,并用定点突变法交换单个氨基酸残基。随后对荧光融合蛋白的亚细胞定位和 n-糖基化分析表明,GnTI TMD 中的保守 Gln 残基对于其顺面/中间高尔基体内的定位是必不可少的。用其他氨基酸替代关键的 Gln 残基会导致错误定位到液泡,并在体内损害 n-糖基化加工。我们的结果表明,GnTI TMD 的序列特异性特征是其与高尔基体驻留衔接蛋白或特定脂质环境相互作用所必需的,这可能促进了衣壳蛋白复合物 I 介导的逆行运输,从而维持 GnTI 在植物顺面/中间高尔基体内的稳定分布。

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本文引用的文献

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Recycling of Golgi glycosyltransferases requires direct binding to coatomer.高尔基糖基转移酶的回收需要直接结合衣被蛋白。
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The glycan-dependent ERAD machinery degrades topologically diverse misfolded proteins.糖基依赖的内质网相关降解机制可降解拓扑结构多样的错误折叠蛋白。
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