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J Cell Biol. 1994 Nov;127(3):667-78. doi: 10.1083/jcb.127.3.667.
2
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3
Localization and targeting of the Saccharomyces cerevisiae Kre2p/Mnt1p alpha 1,2-mannosyltransferase to a medial-Golgi compartment.酿酒酵母Kre2p/Mnt1p α1,2-甘露糖基转移酶在内质网到高尔基体中间膜囊的定位与靶向运输
J Cell Biol. 1995 Nov;131(4):913-27. doi: 10.1083/jcb.131.4.913.
4
Retrograde transport of the mannosyltransferase Och1p to the early Golgi requires a component of the COG transport complex.甘露糖基转移酶Och1p向早期高尔基体的逆行运输需要COG运输复合体的一个组分。
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Role for Drs2p, a P-type ATPase and potential aminophospholipid translocase, in yeast late Golgi function.P型ATP酶及潜在氨基磷脂转位酶Drs2p在酵母晚期高尔基体功能中的作用。
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7
Mnt2p and Mnt3p of Saccharomyces cerevisiae are members of the Mnn1p family of alpha-1,3-mannosyltransferases responsible for adding the terminal mannose residues of O-linked oligosaccharides.酿酒酵母的Mnt2p和Mnt3p是Mnn1p家族α-1,3-甘露糖基转移酶的成员,负责添加O-连接寡糖的末端甘露糖残基。
Glycobiology. 1999 Oct;9(10):1045-51. doi: 10.1093/glycob/9.10.1045.
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Selective and immediate effects of clathrin heavy chain mutations on Golgi membrane protein retention in Saccharomyces cerevisiae.网格蛋白重链突变对酿酒酵母高尔基体膜蛋白保留的选择性和即时效应。
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Localization of a yeast early Golgi mannosyltransferase, Och1p, involves retrograde transport.酵母早期高尔基体甘露糖基转移酶Och1p的定位涉及逆向运输。
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10
Mannosyltransferase activities in membranes from various yeast strains.不同酵母菌株细胞膜中的甘露糖基转移酶活性。
Glycobiology. 1995 Oct;5(7):671-81. doi: 10.1093/glycob/5.7.671.

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Yeast vacuolar proenzymes are sorted in the late Golgi complex and transported to the vacuole via a prevacuolar endosome-like compartment.酵母液泡前体酶在高尔基体晚期复合体中进行分选,并通过类似前液泡内体的区室转运至液泡。
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Immunoisolation of Kex2p-containing organelles from yeast demonstrates colocalisation of three processing proteinases to a single Golgi compartment.从酵母中对含Kex2p的细胞器进行免疫分离,结果表明三种加工蛋白酶共定位于单个高尔基体区室。
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网格蛋白依赖性α1,3甘露糖基转移酶在酿酒酵母高尔基体复合体中的定位

Clathrin-dependent localization of alpha 1,3 mannosyltransferase to the Golgi complex of Saccharomyces cerevisiae.

作者信息

Graham T R, Seeger M, Payne G S, MacKay V L, Emr S D

机构信息

Department of Molecular Biology, Vanderbilt University, Nashville, Tennessee 37235.

出版信息

J Cell Biol. 1994 Nov;127(3):667-78. doi: 10.1083/jcb.127.3.667.

DOI:10.1083/jcb.127.3.667
PMID:7962051
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2120240/
Abstract

Posttranslational modification of yeast glycoproteins with alpha 1,3-linked mannose is initiated within a Golgi compartment analogous to the medial Golgi cisternae of higher eukaryotes. We have characterized the synthesis, posttranslational modification, and localization of the yeast alpha 1,3 mannosyltransferase (Mnn1p) using antibodies prepared against a segment of this protein expressed in bacteria. Mnn1p is initially synthesized as a 98.5-kD, type II integral membrane glycoprotein that is modified with both N- and O-linked oligosaccharides. It is subject to a slow, incremental increase in molecular mass that is dependent upon protein transport to the Golgi complex. Self-modification of Mnn1p with alpha 1,3 mannose epitopes, primarily on O-linked oligosaccharides, is at least partly responsible for the incremental increase in molecular mass. Mnn1p is a resident protein of the Golgi complex and colocalizes with guanosine diphosphatase to at least two physically distinct Golgi compartments by sucrose gradient fractionation, one of which may be a late Golgi compartment that also contains the Kex2 endopeptidase. Surprisingly, we found that a significant fraction of Mnn1p is mislocalized to the plasma membrane in a clathrin heavy chain temperature sensitive mutant while guanosine diphosphatase remains intracellular. A mutant Mnn1p that lacks the NH2-terminal cytoplasmic tail is properly localized to the Golgi complex, indicating that clathrin does not mediate Mnnlp Golgi retention by a direct interaction with the Mnn1p cytoplasmic tail. These results indicate that clathrin plays a broader role in the localization of Golgi proteins than anticipated.

摘要

酵母糖蛋白与α1,3 - 连接的甘露糖的翻译后修饰起始于一个类似于高等真核生物中高尔基中间膜囊的高尔基体区室。我们使用针对在细菌中表达的该蛋白片段制备的抗体,对酵母α1,3甘露糖基转移酶(Mnn1p)的合成、翻译后修饰及定位进行了表征。Mnn1p最初被合成为一种98.5-kD的II型整合膜糖蛋白,其同时被N - 连接和O - 连接寡糖修饰。它的分子量会缓慢、逐步增加,这取决于蛋白质向高尔基体复合体的转运。Mnn1p自身用α1,3甘露糖表位进行修饰,主要修饰O - 连接寡糖,这至少部分地导致了分子量的逐步增加。Mnn1p是高尔基体复合体的驻留蛋白,通过蔗糖梯度分级分离,它与鸟苷二磷酸酶共定位于至少两个物理上不同的高尔基体区室,其中一个可能是晚期高尔基体区室,该区域还含有Kex2内肽酶。令人惊讶的是,我们发现,在网格蛋白重链温度敏感突变体中,相当一部分Mnn1p错误定位于质膜,而鸟苷二磷酸酶仍保留在细胞内。缺乏NH2 - 末端细胞质尾巴的突变型Mnn1p能正确定位于高尔基体复合体,这表明网格蛋白并非通过与Mnn1p细胞质尾巴的直接相互作用来介导Mnn1p在高尔基体的保留。这些结果表明,网格蛋白在高尔基体蛋白定位中所起的作用比预期的更为广泛。