ER Import Sites and Their Relationship to ER Exit Sites: A New Model for Bidirectional ER-Golgi Transport in Higher Plants

Per definition, ER exit sites are COPII vesiculation events at the surface of the ER and in higher plants are only visualizable in the electron microscope through cryofixation techniques. Fluorescent COPII labeling moves with Golgi stacks and locates to the interface between the ER and the Golgi. In...

Descripción completa

Detalles Bibliográficos
Autores principales: Lerich, Alexander, Hillmer, Stefan, Langhans, Markus, Scheuring, David, van Bentum, Paulien, Robinson, David G.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Frontiers Research Foundation 2012
Materias:
Plant Science
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3410614/
https://www.ncbi.nlm.nih.gov/pubmed/22876251
http://dx.doi.org/10.3389/fpls.2012.00143
_version_ 1782239742705795072
author Lerich, Alexander
Hillmer, Stefan
Langhans, Markus
Scheuring, David
van Bentum, Paulien
Robinson, David G.
author_facet Lerich, Alexander
Hillmer, Stefan
Langhans, Markus
Scheuring, David
van Bentum, Paulien
Robinson, David G.
author_sort Lerich, Alexander
collection PubMed
description Per definition, ER exit sites are COPII vesiculation events at the surface of the ER and in higher plants are only visualizable in the electron microscope through cryofixation techniques. Fluorescent COPII labeling moves with Golgi stacks and locates to the interface between the ER and the Golgi. In contrast, the domain of the ER where retrograde COPI vesicles fuse, i.e., ER import sites (ERIS), has remained unclear. To identify ERIS we have employed ER-located SNAREs and tethering factors. We screened several SNAREs (SYP81, the SYP7 family, and USE1) to find a SNARE whose overexpression did not disrupt ER-Golgi traffic and which gave rise to discrete fluorescent punctae when expressed with an XFP tag. Only the Qc-SNARE SYP72 fulfilled these criteria. When coexpressed with SYP72-YFP, both the type I-membrane protein RFP-p24δ5 and the luminal marker CFP-HDEL whose ER localization are due to an efficient COPI-mediated recycling, form nodules along the tubular ER network. SYP72-YFP colocalizes with these nodules which are not seen when RFP-p24δ5 or CFP-HDEL is expressed alone or when SYP72-YFP is coexpressed with a mutant form of RFP-p24δ5 that cannot exit the ER. SYP72-YFP does not colocalize with Golgi markers, except when the Golgi stacks are immobilized through actin depolymerization. Endogenous SYP7 SNAREs, also colocalize with immobilized COPII/Golgi. In contrast, XFP-tagged versions of plant homologs to TIP20 of the Dsl1 COPI-tethering factor complex, and the COPII-tethering factor p115 colocalize perfectly with Golgi stacks irrespective of the motile status. These data suggest that COPI vesicle fusion with the ER is restricted to periods when Golgi stacks are stationary, but that when moving both COPII and COPI vesicles are tethered and collect in the ER-Golgi interface. Thus, the Golgi stack and an associated domain of the ER thereby constitute a mobile secretory and recycling unit: a unique feature in eukaryotic cells.
format Online
Article
Text
id pubmed-3410614
institution National Center for Biotechnology Information
language English
publishDate 2012
publisher Frontiers Research Foundation
record_format MEDLINE/PubMed
spelling pubmed-34106142012-08-08 ER Import Sites and Their Relationship to ER Exit Sites: A New Model for Bidirectional ER-Golgi Transport in Higher Plants Lerich, Alexander Hillmer, Stefan Langhans, Markus Scheuring, David van Bentum, Paulien Robinson, David G. Front Plant Sci Plant Science Per definition, ER exit sites are COPII vesiculation events at the surface of the ER and in higher plants are only visualizable in the electron microscope through cryofixation techniques. Fluorescent COPII labeling moves with Golgi stacks and locates to the interface between the ER and the Golgi. In contrast, the domain of the ER where retrograde COPI vesicles fuse, i.e., ER import sites (ERIS), has remained unclear. To identify ERIS we have employed ER-located SNAREs and tethering factors. We screened several SNAREs (SYP81, the SYP7 family, and USE1) to find a SNARE whose overexpression did not disrupt ER-Golgi traffic and which gave rise to discrete fluorescent punctae when expressed with an XFP tag. Only the Qc-SNARE SYP72 fulfilled these criteria. When coexpressed with SYP72-YFP, both the type I-membrane protein RFP-p24δ5 and the luminal marker CFP-HDEL whose ER localization are due to an efficient COPI-mediated recycling, form nodules along the tubular ER network. SYP72-YFP colocalizes with these nodules which are not seen when RFP-p24δ5 or CFP-HDEL is expressed alone or when SYP72-YFP is coexpressed with a mutant form of RFP-p24δ5 that cannot exit the ER. SYP72-YFP does not colocalize with Golgi markers, except when the Golgi stacks are immobilized through actin depolymerization. Endogenous SYP7 SNAREs, also colocalize with immobilized COPII/Golgi. In contrast, XFP-tagged versions of plant homologs to TIP20 of the Dsl1 COPI-tethering factor complex, and the COPII-tethering factor p115 colocalize perfectly with Golgi stacks irrespective of the motile status. These data suggest that COPI vesicle fusion with the ER is restricted to periods when Golgi stacks are stationary, but that when moving both COPII and COPI vesicles are tethered and collect in the ER-Golgi interface. Thus, the Golgi stack and an associated domain of the ER thereby constitute a mobile secretory and recycling unit: a unique feature in eukaryotic cells. Frontiers Research Foundation 2012-07-02 /pmc/articles/PMC3410614/ /pubmed/22876251 http://dx.doi.org/10.3389/fpls.2012.00143 Text en Copyright © 2012 Lerich, Hillmer, Langhans, Scheuring, van Bentum and Robinson. http://www.frontiersin.org/licenseagreement This is an open-access article distributed under the terms of the Creative Commons Attribution Non Commercial License, which permits non-commercial use, distribution, and reproduction in other forums, provided the original authors and source are credited.
spellingShingle Plant Science
Lerich, Alexander
Hillmer, Stefan
Langhans, Markus
Scheuring, David
van Bentum, Paulien
Robinson, David G.
ER Import Sites and Their Relationship to ER Exit Sites: A New Model for Bidirectional ER-Golgi Transport in Higher Plants
title ER Import Sites and Their Relationship to ER Exit Sites: A New Model for Bidirectional ER-Golgi Transport in Higher Plants
title_full ER Import Sites and Their Relationship to ER Exit Sites: A New Model for Bidirectional ER-Golgi Transport in Higher Plants
title_fullStr ER Import Sites and Their Relationship to ER Exit Sites: A New Model for Bidirectional ER-Golgi Transport in Higher Plants
title_full_unstemmed ER Import Sites and Their Relationship to ER Exit Sites: A New Model for Bidirectional ER-Golgi Transport in Higher Plants
title_short ER Import Sites and Their Relationship to ER Exit Sites: A New Model for Bidirectional ER-Golgi Transport in Higher Plants
title_sort er import sites and their relationship to er exit sites: a new model for bidirectional er-golgi transport in higher plants
topic Plant Science
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3410614/
https://www.ncbi.nlm.nih.gov/pubmed/22876251
http://dx.doi.org/10.3389/fpls.2012.00143
work_keys_str_mv AT lerichalexander erimportsitesandtheirrelationshiptoerexitsitesanewmodelforbidirectionalergolgitransportinhigherplants
AT hillmerstefan erimportsitesandtheirrelationshiptoerexitsitesanewmodelforbidirectionalergolgitransportinhigherplants
AT langhansmarkus erimportsitesandtheirrelationshiptoerexitsitesanewmodelforbidirectionalergolgitransportinhigherplants
AT scheuringdavid erimportsitesandtheirrelationshiptoerexitsitesanewmodelforbidirectionalergolgitransportinhigherplants
AT vanbentumpaulien erimportsitesandtheirrelationshiptoerexitsitesanewmodelforbidirectionalergolgitransportinhigherplants
AT robinsondavidg erimportsitesandtheirrelationshiptoerexitsitesanewmodelforbidirectionalergolgitransportinhigherplants

Ejemplares similares