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多肽转运装置定位于内质网中含有核糖体结合蛋白和核糖体的区域。I. 对大鼠肝脏微粒体亚组分的功能测试。

Segregation of the polypeptide translocation apparatus to regions of the endoplasmic reticulum containing ribophorins and ribosomes. I. Functional tests on rat liver microsomal subfractions.

作者信息

Amar-Costesec A, Todd J A, Kreibich G

出版信息

J Cell Biol. 1984 Dec;99(6):2247-53. doi: 10.1083/jcb.99.6.2247.

DOI:10.1083/jcb.99.6.2247
PMID:6501423
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2113578/
Abstract

A preparation of rat liver microsomes containing 70% of the total cellular endoplasmic reticulum (ER) membranes was subfractionated by isopycnic density centrifugation. Twelve subfractions of different ribosome content ranging in density from 1.06 to 1.29 were obtained and analyzed with respect to marker enzymes, RNA, and protein content, as well as the capacity of these membranes to bind 80S ribosomes in vitro. After removal of native polysomes from these microsomal subfractions by puromycin in a buffer of high ionic strength their capacity to rebind 80S ribosomes approached levels found in the corresponding native membranes before ribosome stripping. This indicates that in vitro rebinding of ribosomes occurs to the same sites occupied in the cell by membrane-bound polysomes. Microsomes in the microsomal subfractions were also tested for their capacity to effect the translocation of nascent secretory proteins into the microsomal lumen utilizing a rabbit reticulocyte translation system programmed with mRNA coding for the precursor of human placental lactogen. Membranes from microsomes with the higher isopycnic density and a high ribosome content showed the highest translocation activity, whereas membranes derived from smooth microsomes had only a very low translocation activity. These results indicate the membranes of the rough and smooth portions of the endoplasmic reticulum are functionally differentiated so that sites for ribosome binding and the translocation of nascent polypeptides are segregated to the rough domain of the organelle.

摘要

通过等密度离心对含有70%的细胞内质网(ER)膜的大鼠肝微粒体进行亚分级分离。获得了密度范围从1.06至1.29的12个核糖体含量不同的亚分级,并针对标记酶、RNA和蛋白质含量,以及这些膜在体外结合80S核糖体的能力进行了分析。在高离子强度缓冲液中用嘌呤霉素从这些微粒体亚分级中去除天然多核糖体后,它们重新结合80S核糖体的能力接近核糖体去除前相应天然膜中的水平。这表明核糖体在体外重新结合到细胞中被膜结合多核糖体占据的相同位点。利用编码人胎盘催乳素前体的mRNA编程的兔网织红细胞翻译系统,还测试了微粒体亚分级中的微粒体将新生分泌蛋白转运到微粒体腔中的能力。具有较高等密度和高核糖体含量的微粒体膜显示出最高的转运活性,而来自光滑微粒体的膜只有非常低的转运活性。这些结果表明内质网粗糙和光滑部分的膜在功能上是有差异的,因此核糖体结合位点和新生多肽的转运被分隔到细胞器的粗糙区域。

相似文献

1
Segregation of the polypeptide translocation apparatus to regions of the endoplasmic reticulum containing ribophorins and ribosomes. I. Functional tests on rat liver microsomal subfractions.多肽转运装置定位于内质网中含有核糖体结合蛋白和核糖体的区域。I. 对大鼠肝脏微粒体亚组分的功能测试。
J Cell Biol. 1984 Dec;99(6):2247-53. doi: 10.1083/jcb.99.6.2247.
2
Segregation of the polypeptide translocation apparatus to regions of the endoplasmic reticulum containing ribophorins and ribosomes. II. Rat liver microsomal subfractions contain equimolar amounts of ribophorins and ribosomes.多肽转运装置定位于内质网中含有核糖体结合蛋白和核糖体的区域。II. 大鼠肝脏微粒体亚组分含有等摩尔量的核糖体结合蛋白和核糖体。
J Cell Biol. 1984 Dec;99(6):2254-9. doi: 10.1083/jcb.99.6.2254.
3
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J Supramol Struct. 1978;8(3):279-302. doi: 10.1002/jss.400080307.
4
Translocation and proteolytic processing of nascent secretory polypeptide chains: two functions associated with the ribosomal domain of the endoplasmic reticulum.新生分泌型多肽链的易位和蛋白水解加工:与内质网核糖体结构域相关的两种功能。
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5
Mobility of ribosomes bound to microsomal membranes. A freeze-etch and thin-section electron microscope study of the structure and fluidity of the rough endoplasmic reticulum.结合于微粒体膜的核糖体的移动性。粗面内质网结构与流动性的冷冻蚀刻及超薄切片电子显微镜研究。
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Recovery of ribophorins and ribosomes in "inverted rough" vesicles derived from rat liver rough microsomes.从大鼠肝脏粗面微粒体衍生的“反向粗面”囊泡中回收核糖体结合蛋白和核糖体
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Release of poly A(+) messenger RNA from rat liver rough microsomes upon disassembly of bound polysomes.结合多核糖体解体后大鼠肝脏粗面微粒体中多聚腺苷酸(+)信使核糖核酸的释放
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Characterization of secretory protein translocation: ribosome-membrane interaction in endoplasmic reticulum.分泌蛋白转运的特征:内质网中的核糖体 - 膜相互作用
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9
Proteins of rough microsomal membranes related to ribosome binding. I. Identification of ribophorins I and II, membrane proteins characteristics of rough microsomes.与核糖体结合相关的糙面微粒体膜蛋白。I. 核糖体结合蛋白I和II的鉴定,糙面微粒体的膜蛋白特性
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引用本文的文献

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J Cell Biol. 2000 Aug 7;150(3):461-74. doi: 10.1083/jcb.150.3.461.
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Localization of ribophorin II to the endoplasmic reticulum involves both its transmembrane and cytoplasmic domains.核糖体结合蛋白II定位于内质网涉及到它的跨膜结构域和胞质结构域。
Eur J Cell Biol. 2000 Apr;79(4):219-28. doi: 10.1078/S0171-9335(04)70025-4.
3
Segregation of the polypeptide translocation apparatus to regions of the endoplasmic reticulum containing ribophorins and ribosomes. II. Rat liver microsomal subfractions contain equimolar amounts of ribophorins and ribosomes.多肽转运装置定位于内质网中含有核糖体结合蛋白和核糖体的区域。II. 大鼠肝脏微粒体亚组分含有等摩尔量的核糖体结合蛋白和核糖体。
J Cell Biol. 1984 Dec;99(6):2254-9. doi: 10.1083/jcb.99.6.2254.
4
Anti-liver-kidney microsome antibody recognizes a 50,000 molecular weight protein of the endoplasmic reticulum.抗肝肾微粒体抗体识别内质网中一种分子量为50,000的蛋白质。
J Exp Med. 1985 May 1;161(5):1231-6. doi: 10.1084/jem.161.5.1231.
5
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本文引用的文献

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Protein measurement with the Folin phenol reagent.使用福林酚试剂进行蛋白质测定。
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ULTRACENTRIFUGAL STUDIES ON THE DISSOCIATION OF HEPATIC RIBOSOMES.肝脏核糖体解离的超速离心研究
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Translocation of proteins across the endoplasmic reticulum III. Signal recognition protein (SRP) causes signal sequence-dependent and site-specific arrest of chain elongation that is released by microsomal membranes.蛋白质在内质网上的转运III. 信号识别蛋白(SRP)导致依赖信号序列和位点特异性的链延伸停滞,这种停滞可被微粒体膜解除。
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Secretory protein translocation across membranes-the role of the "docking protein'.分泌蛋白跨膜转运——“对接蛋白”的作用
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8
Identification of ribophorins in rough microsomal membranes from different organs of several species.几种物种不同器官的粗面微粒体膜中核糖体结合蛋白的鉴定。
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Reconstitution of a tandem Co- and post-translational processing pathway with rat liver subcellular fractions.用大鼠肝脏亚细胞组分重建串联共翻译和翻译后加工途径。
J Biol Chem. 1982 Apr 25;257(8):4179-86.
10
Mechanisms for the incorporation of proteins in membranes and organelles.蛋白质整合到膜和细胞器中的机制。
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