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本文引用的文献

1
Synaptotagmin-Associated Endoplasmic Reticulum-Plasma Membrane Contact Sites Are Localized to Immobile ER Tubules.突触结合蛋白相关内质网-质膜接触位点定位于无运动的内质网小管。
Plant Physiol. 2018 Oct;178(2):641-653. doi: 10.1104/pp.18.00498. Epub 2018 Aug 20.
2
Stitching Organelles: Organization and Function of Specialized Membrane Contact Sites in Plants.缝合细胞器:植物中专门的膜接触位点的组织和功能。
Trends Cell Biol. 2016 Sep;26(9):705-717. doi: 10.1016/j.tcb.2016.05.007. Epub 2016 Jun 15.
3
Structure and function of ER membrane contact sites with other organelles.内质网与其他细胞器的膜接触位点的结构和功能。
Nat Rev Mol Cell Biol. 2016 Feb;17(2):69-82. doi: 10.1038/nrm.2015.8. Epub 2015 Dec 2.
4
Triggered Ca2+ influx is required for extended synaptotagmin 1-induced ER-plasma membrane tethering.扩展的突触结合蛋白1诱导内质网-质膜拴系需要触发的钙离子内流。
EMBO J. 2015 Sep 2;34(17):2291-305. doi: 10.15252/embj.201591565. Epub 2015 Jul 22.
5
Nucleocapsid protein from fig mosaic virus forms cytoplasmic agglomerates that are hauled by endoplasmic reticulum streaming.无花果花叶病毒的核衣壳蛋白形成细胞质聚集体,这些聚集体被内质网流运。
J Virol. 2015 Jan;89(1):480-91. doi: 10.1128/JVI.02527-14. Epub 2014 Oct 15.
6
Dynamics of vacuoles and H+-pyrophosphatase visualized by monomeric green fluorescent protein in Arabidopsis: artifactual bulbs and native intravacuolar spherical structures.拟南芥中通过单体绿色荧光蛋白观察到的液泡与H⁺-焦磷酸酶的动态变化:人为形成的球状体和天然液泡内球形结构
Plant Cell. 2014 Aug;26(8):3416-34. doi: 10.1105/tpc.114.127571. Epub 2014 Aug 12.
7
MAIGO5 functions in protein export from Golgi-associated endoplasmic reticulum exit sites in Arabidopsis.MAIGO5 在前体细胞蛋白输出复合体中作用于内质网-高尔基体间的蛋白运输。
Plant Cell. 2013 Nov;25(11):4658-75. doi: 10.1105/tpc.113.118158. Epub 2013 Nov 26.
8
PI(4,5)P(2)-dependent and Ca(2+)-regulated ER-PM interactions mediated by the extended synaptotagmins.由延伸突触结合蛋白介导的 PI(4,5)P(2)-依赖性和 Ca(2+)-调节的内质网-质膜相互作用。
Cell. 2013 Jun 20;153(7):1494-509. doi: 10.1016/j.cell.2013.05.026.
9
Qualitative difference between "bulb" membranes and other vacuolar membranes.“泡囊”膜与其他液泡膜之间的定性差异。
Plant Signal Behav. 2011 Dec;6(12):1914-7. doi: 10.4161/psb.6.12.18061.
10
Improved Gateway binary vectors: high-performance vectors for creation of fusion constructs in transgenic analysis of plants.改良的Gateway二元载体:用于植物转基因分析中创建融合构建体的高性能载体。
Biosci Biotechnol Biochem. 2007 Aug;71(8):2095-100. doi: 10.1271/bbb.70216. Epub 2007 Aug 7.

内质网-质膜锚定因子突触结合蛋白1的亚细胞定位受荧光蛋白融合的影响。

Subcellular localisation of an endoplasmic reticulum-plasma membrane tethering factor, SYNAPTOTAGMIN 1, is affected by fluorescent protein fusion.

作者信息

Ishikawa Kazuya, Tamura Kentaro, Shimada Tomoo

机构信息

a Department of Botany , Graduate School of Science, Kyoto University , Kyoto , Japan.

出版信息

Plant Signal Behav. 2018;13(12):e1547577. doi: 10.1080/15592324.2018.1547577. Epub 2018 Nov 16.

DOI:10.1080/15592324.2018.1547577
PMID:30445890
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC6296351/
Abstract

Membrane contact sites (MCS) have increasingly received attention because of their general role in a number of important cellular processes. SYNAPTOTAGMIN 1 (SYT1) is a tethering factor connecting the endoplasmic reticulum (ER) and the plasma membrane (PM) in plant cells. Confocal microscopy using fluorescent protein fusion is an indispensable tool for studying protein localisation and functions. However, several studies have reported that fluorescent protein dimerisation affects the subcellular localisation of proteins tagged by the fluorescent protein. Here, we investigate the effects of fluorescent protein dimerisation by comparing the subcellular localisation of SYT1 fused with a synthetic GFP (SYT1-sGFP) and SYT1 fused with a monomeric GFP (SYT1-mGFP). SYT1-mGFP was confined to specific domains in the ER, whereas SYT1-sGFP spread along the ER when transiently overexpressed. SYT1-localised regions were suggested to correspond to ER-PM contact sites because of its immobility. Similar results were obtained in the transgenic Arabidopsis, even though SYT1-sGFP and SYT1-mGFP were expressed at comparable levels. It is suggested that SYT1-mGFP more accurately reproduced SYT1 localisation in intact cells because the proportion of persistent area in the ER was more similar between the wild type and the plant expressing SYT1-mGFP than between the wild type and the plant expressing SYT1-sGFP. Taken together, these results suggest that the fusion of sGFP makes SYT1-sGFP form excessive ER-PM contact sites in the ER.

摘要

膜接触位点(MCS)因其在许多重要细胞过程中的普遍作用而越来越受到关注。突触结合蛋白1(SYT1)是植物细胞中连接内质网(ER)和质膜(PM)的一种拴系因子。使用荧光蛋白融合的共聚焦显微镜是研究蛋白质定位和功能不可或缺的工具。然而,多项研究报告称,荧光蛋白二聚化会影响由荧光蛋白标记的蛋白质的亚细胞定位。在这里,我们通过比较与合成绿色荧光蛋白(SYT1-sGFP)融合的SYT1和与单体绿色荧光蛋白(SYT1-mGFP)融合的SYT1的亚细胞定位,来研究荧光蛋白二聚化的影响。当瞬时过表达时,SYT1-mGFP局限于内质网中的特定区域,而SYT1-sGFP沿内质网扩散。由于SYT1的固定性,其定位区域被认为对应于内质网-质膜接触位点。在转基因拟南芥中也获得了类似的结果,尽管SYT1-sGFP和SYT1-mGFP的表达水平相当。有人认为,SYT1-mGFP更准确地再现了完整细胞中SYT1的定位,因为野生型与表达SYT1-mGFP的植物之间内质网中持续存在区域的比例比野生型与表达SYT1-sGFP的植物之间更相似。综上所述,这些结果表明,sGFP的融合使SYT1-sGFP在内质网中形成过多的内质网-质膜接触位点。