Your search keyword '"Coated Vesicles chemistry"' showing total 9 results

1. Transport of axl2p depends on erv14p, an ER-vesicle protein related to the Drosophila cornichon gene product.

Author

Powers J and Barlowe C

Subjects

Amino Acid Sequence, Animals, Biological Transport physiology, Cell Fractionation, Cell Polarity physiology, Coated Vesicles chemistry, Drosophila physiology, Endoplasmic Reticulum chemistry, Fluorescent Antibody Technique, Golgi Apparatus chemistry, Immunohistochemistry, Insect Proteins chemistry, Molecular Sequence Data, Mutation genetics, Sequence Analysis, Sequence Homology, Amino Acid, Spores chemistry, Fungal Proteins chemistry, Membrane Proteins chemistry, Saccharomyces cerevisiae physiology

Abstract

COPII-coated ER-derived transport vesicles from Saccharomyces cerevisiae contain a distinct set of membrane-bound polypeptides. One of these polypeptides, termed Erv14p (ER-vesicle protein of 14 kD), corresponds to an open reading frame on yeast chromosome VII that is predicted to encode an integral membrane protein and shares sequence identity with the Drosophila cornichon gene product. Experiments with an epitope-tagged version of Erv14p indicate that this protein localizes to the ER and is selectively packaged into COPII-coated vesicles. Haploid cells that lack Erv14p are viable but display a modest defect in bud site selection because a transmembrane secretory protein, Axl2p, is not efficiently delivered to the cell surface. Axl2p is required for selection of axial growth sites and normally localizes to nascent bud tips or the mother bud neck. In erv14Delta strains, Axl2p accumulates in the ER while other secretory proteins are transported at wild-type rates. We propose that Erv14p is required for the export of specific secretory cargo from the ER. The polarity defect of erv14Delta yeast cells is reminiscent of cornichon mutants, in which egg chambers fail to establish proper asymmetry during early stages of oogenesis. These results suggest an unforeseen conservation in mechanisms producing cell polarity shared between yeast and Drosophila.

Published

1998

2. A major transmembrane protein of Golgi-derived COPI-coated vesicles involved in coatomer binding.

Author

Sohn K, Orci L, Ravazzola M, Amherdt M, Bremser M, Lottspeich F, Fiedler K, Helms JB, and Wieland FT

Subjects

Amino Acid Sequence, Animals, CHO Cells, Cloning, Molecular, Coated Vesicles metabolism, Coatomer Protein, Cricetinae, DNA, Complementary genetics, Fluorescent Antibody Technique, Golgi Apparatus metabolism, Membrane Proteins analysis, Membrane Proteins chemistry, Membrane Proteins isolation & purification, Microscopy, Immunoelectron, Molecular Sequence Data, Molecular Weight, Coated Vesicles chemistry, Golgi Apparatus chemistry, Membrane Proteins metabolism, Receptors, Cytoplasmic and Nuclear

Abstract

Formation of non-clathrin-coated vesicles requires the recruitment of several cytosolic factors to the Golgi membrane. To identify membrane proteins involved in this budding process, a highly abundant type I transmembrane protein (p23) was isolated from mammalian Golgi-derived COPI-coated vesicles, and its cDNA was cloned and sequenced. It belongs to the p24 family of proteins involved in the budding of transport vesicles (Stamnes, M.A., M.W. Craighead, M.H. Hoe, N. Lampen, S. Geromanos, P. Tempst, and J.E. Rothman. 1995. Proc. Natl. Acad. Sci. USA. 92:8011-8015). p23 consists of a large NH2-terminal luminal domain and a short COOH-terminal cytoplasmic tail (-LRRFFKAKKLIE-CO2-) that shows similarity, but not identity, with the sequence motif-KKXX-CO2-, known as a signal for retrieval of escaped ER-resident membrane proteins (Jackson, M.R., T. Nilsson, and P.A. Peterson. 1990. EMBO (Eur. Mol. Biol. Organ.) J. 9:3153-3162; Nilsson, T., M. Jackson, and P.A. Peterson. 1989. Cell. 58:707-718). The cytoplasmic tail of p23 binds to coatomer with similar efficiency as known KKXX motifs. However, the p23 tail differs from the KKXX motif in having an additional motif needed for binding of coatomer. p23 is localized to Golgi cisternae and, during vesicle formation, it concentrates into COPI-coated buds and vesicles. Biochemical analysis revealed that p23 is enriched in vesicles by a factor of approximately 20, as compared with the donor Golgi fraction, and is present in amounts stoichiometric to the small GTP-binding protein ADP-ribosylation factor (ARF) and coatomer. From these data we conclude that p23 represents a Golgi-specific receptor for coatomer involved in the formation of COPI-coated vesicles.

Published

1996

3. AP-2-containing clathrin coats assemble on mature lysosomes.

Author

Traub LM, Bannykh SI, Rodel JE, Aridor M, Balch WE, and Kornfeld S

Subjects

Animals, Antigens, CD analysis, Antigens, CD metabolism, Brain cytology, Cell Membrane Permeability, Cells, Cultured chemistry, Cells, Cultured metabolism, Cells, Cultured ultrastructure, Coated Vesicles ultrastructure, DNA-Binding Proteins metabolism, Fluorescent Antibody Technique, Freeze Etching, Kidney cytology, Liver cytology, Lysosomal Membrane Proteins, Lysosomes chemistry, Lysosomes ultrastructure, Membrane Glycoproteins analysis, Membrane Glycoproteins metabolism, Membrane Proteins analysis, Microscopy, Electron, Rats, Transcription Factor AP-2, Transcription Factors metabolism, Clathrin analysis, Coated Vesicles chemistry, DNA-Binding Proteins analysis, Lysosomes metabolism, Transcription Factors analysis

Abstract

Coat proteins appear to play a general role in intracellular protein trafficking by coordinating a membrane budding event with cargo selection. Here we show that the AP-2 adaptor, a clathrin-associated coat-protein complex that nucleates clathrin-coated vesicle formation at the cell surface, can also initiate the assembly of normal polyhedral clathrin coats on dense lysosomes under physiological conditions in vitro. Clathrin coat formation on lysosomes is temperature dependent, displays an absolute requirement for ATP, and occurs in both semi-intact cells and on purified lysosomes, suggesting that clathrin-coated vesicles might regulate retrograde membrane traffic out of the lysosomal compartment.

Published

1996

4. COPII vesicles derived from mammalian endoplasmic reticulum microsomes recruit COPI.

Author

Rowe T, Aridor M, McCaffery JM, Plutner H, Nuoffer C, and Balch WE

Subjects

ADP-Ribosylation Factor 1, ADP-Ribosylation Factors, Animals, Biological Transport physiology, Carrier Proteins genetics, Carrier Proteins metabolism, Cells, Cultured metabolism, Cells, Cultured ultrastructure, Coated Vesicles metabolism, Coatomer Protein, Endoplasmic Reticulum metabolism, Endoplasmic Reticulum ultrastructure, GTP-Binding Proteins genetics, GTP-Binding Proteins metabolism, Genetic Complementation Test, Golgi Apparatus chemistry, Golgi Apparatus metabolism, Guanosine Diphosphate metabolism, Immunomagnetic Separation, Kidney cytology, Mammals, Membrane Proteins analysis, Microscopy, Electron, Microsomes metabolism, Microsomes ultrastructure, Mutation physiology, Rabbits, Rats, Receptors, Cytoplasmic and Nuclear isolation & purification, Receptors, Cytoplasmic and Nuclear metabolism, Vesicular Transport Proteins, Lamin B Receptor, Coated Vesicles chemistry, Endoplasmic Reticulum chemistry, Membrane Proteins metabolism, Microsomes chemistry, Monomeric GTP-Binding Proteins, Saccharomyces cerevisiae Proteins

Abstract

ER to Golgi transport requires the function of two distinct vesicle coat complexes, termed COPI (coatomer) and COPII, whose assembly is regulated by the small GTPases ADP-ribosylation factor 1 (ARF1) and Sar1, respectively. To address their individual roles in transport, we have developed a new assay using mammalian microsomes that reconstitute the formation of ER-derived vesicular carriers. Vesicles released from the ER were found to contain the cargo molecule vesicular stomatitis virus glycoprotein (VSV-G) and p58, an endogenous protein that continuously recycles between the ER and pre-Golgi intermediates. Cargo was efficiently sorted from resident ER proteins during vesicle formation in vitro. Export of VSV-G and p58 were found to be exclusively mediated by COPII. Subsequent movement of ER-derived carriers to the Golgi stack was blocked by a trans-dominant ARF1 mutant restricted to the GDP-bound state, which is known to prevent COPI recruitment. To establish the initial site of coatomer assembly after export from the ER, we immunoisolated the vesicular intermediates and tested their ability to recruit COPI. Vesicles bound coatomer in a physiological fashion requiring an ARF1-guanine nucleotide exchange activity. These results suggest that coat exchange is an early event preceding the targeting of ER-derived vesicles to pre-Golgi intermediates.

Published

1996

5. The organization of endoplasmic reticulum export complexes.

Author

Bannykh SI, Rowe T, and Balch WE

Subjects

Animals, Biological Transport, Cell Line, Coated Vesicles chemistry, Coated Vesicles metabolism, Endoplasmic Reticulum chemistry, Endoplasmic Reticulum metabolism, Freeze Etching methods, GTP-Binding Proteins genetics, GTP-Binding Proteins physiology, Golgi Apparatus ultrastructure, Guanosine 5'-O-(3-Thiotriphosphate), Kidney, Leukemia, Basophilic, Acute, Membrane Proteins analysis, Mutation, Nuclear Envelope ultrastructure, Rats, Tumor Cells, Cultured, Vesicular Transport Proteins, Vesicular stomatitis Indiana virus, Viral Envelope Proteins metabolism, Coated Vesicles ultrastructure, Endoplasmic Reticulum ultrastructure, Membrane Glycoproteins, Monomeric GTP-Binding Proteins, Saccharomyces cerevisiae Proteins

Abstract

Export of cargo from the ER occurs through the formation of 60-70nm COPII-coated vesicular carriers. We have applied serial-thin sectioning and stereology to quantitatively characterize the three-dimensional organization of ER export sites in vivo and in vitro. We find that ER buds in vivo are nonrandomly distributed, being concentrated in regional foci we refer to as export complexes. The basic organization of an export complex can be divided into an active COPII-containing budding zone on a single ER cisterna, which is adjacent to budding zones found on distantly connected ER cisternae. These budding foci surround and face a central cluster of morphologically independent vesicular-tubular elements that contain COPI coats involved in retrograde transport. Vesicles within these export complexes contain concentrated cargo molecules. The structure of vesicular-tubular clusters in export complexes is particularly striking in replicas generated using a quick-freeze, deep-etch approach to visualize for the first time their three-dimensional organization and cargo composition. We conclude that budding from the ER through recruitment of COPII is confined to highly specialized export complexes that topologically restrict anterograde transport to regional foci to facilitate efficient coupling to retrograde recycling by COPI.

Published

1996

6. Architecture of coatomer: molecular characterization of delta-COP and protein interactions within the complex.

Author

Faulstich D, Auerbach S, Orci L, Ravazzola M, Wegchingel S, Lottspeich F, Stenbeck G, Harter C, Wieland FT, and Tschochner H

Subjects

Amino Acid Sequence, Animals, Brain, Cattle, Cloning, Molecular, Coated Vesicles chemistry, Coatomer Protein, DNA, Complementary genetics, Gene Expression, Genes, Lethal genetics, Golgi Apparatus chemistry, Liver, Membrane Proteins analysis, Molecular Sequence Data, Precipitin Tests, Rats, Recombinant Fusion Proteins metabolism, Sequence Analysis, DNA, Sequence Homology, Amino Acid, Membrane Proteins genetics, Membrane Proteins metabolism

Abstract

Coatomer is a cytosolic protein complex that forms the coat of COP I-coated transport vesicles. In our attempt to analyze the physical and functional interactions between its seven subunits (coat proteins, [COPs] alpha-zeta), we engaged in a program to clone and characterize the individual coatomer subunits. We have now cloned, sequenced, and overexpressed bovine alpha-COP, the 135-kD subunit of coatomer as well as delta-COP, the 57-kD subunit and have identified a yeast homolog of delta-COP by cDNA sequence comparison and by NH2-terminal peptide sequencing. delta-COP shows homologies to subunits of the clathrin adaptor complexes AP1 and AP2. We show that in Golgi-enriched membrane fractions, the protein is predominantly found in COP I-coated transport vesicles and in the budding regions of the Golgi membranes. A knock-out of the delta-COP gene in yeast is lethal. Immunoprecipitation, as well as analysis exploiting the two-hybrid system in a complete COP screen, showed physical interactions between alpha- and epsilon-COPs and between beta- and delta-COPs. Moreover, the two-hybrid system indicates interactions between gamma- and zeta-COPs as well as between alpha- and beta' COPs. We propose that these interactions reflect in vivo associations of those subunits and thus play a functional role in the assembly of coatomer and/or serve to maintain the molecular architecture of the complex.

Published

1996

7. A v-SNARE implicated in intra-Golgi transport.

Author

Nagahama M, Orci L, Ravazzola M, Amherdt M, Lacomis L, Tempst P, Rothman JE, and Söllner TH

Subjects

Amino Acid Sequence, Animals, Antibody Specificity, Base Sequence, Binding, Competitive physiology, Biological Transport physiology, CHO Cells chemistry, CHO Cells metabolism, CHO Cells ultrastructure, Carrier Proteins immunology, Carrier Proteins metabolism, Cell Fractionation, Coated Vesicles chemistry, Cricetinae, Cytoplasm chemistry, Golgi Apparatus chemistry, Golgi Apparatus ultrastructure, Intracellular Membranes chemistry, Membrane Proteins immunology, Membrane Proteins isolation & purification, Microscopy, Immunoelectron, Molecular Sequence Data, Nerve Tissue Proteins isolation & purification, Nerve Tissue Proteins metabolism, SNARE Proteins, Soluble N-Ethylmaleimide-Sensitive Factor Attachment Proteins, Golgi Apparatus metabolism, Membrane Proteins metabolism, Vesicular Transport Proteins

Abstract

We report the identification of a putative v-SNARE (GOS-28), localized primarily to transport vesicles at the terminal rims of Golgi stacks. In vitro, GOS-28, A Golgi SNARE of 28 kD, is efficiently packaged into Golgi-derived vesicles, which are most likely COPI coated. Antibodies directed against GOS-28 block its ability to bind alpha-SNAP, partially inhibit transport from the cis to the medial cisternae, and do not inhibit budding of COP-coated vesicles, but do accumulate docked uncoated vesicles.

Published

1996

8. Targeting signals and subunit interactions in coated vesicle adaptor complexes.

Author

Page LJ and Robinson MS

Subjects

Adaptor Protein Complex alpha Subunits, Adaptor Protein Complex beta Subunits, Adaptor Protein Complex gamma Subunits, Adaptor Proteins, Vesicular Transport, Animals, Cell Membrane physiology, Fibroblasts cytology, Fluorescent Antibody Technique, Golgi Apparatus physiology, Membrane Proteins analysis, Rats, Recombinant Fusion Proteins physiology, Recombinant Fusion Proteins ultrastructure, Adaptor Protein Complex 1, Adaptor Protein Complex 2, Adaptor Protein Complex mu Subunits, Adaptor Protein Complex sigma Subunits, Coated Vesicles chemistry, Coated Vesicles physiology

Abstract

There are two clathrin-coated vesicle adaptor complexes in the cell, one associated with the plasma membrane and one associated with the TGN. The subunit composition of the plasma membrane adaptor complex is alpha-adaptin, beta-adaptin, AP50, and AP17; while that of the TGN adaptor complex is gamma-adaptin, beta'-adaptin, AP47, and AP19. To search for adaptor targeting signals, we have constructed chimeras between alpha-adaptin and gamma-adaptin within their NH2-terminal domains. We have identified stretches of sequence in the two proteins between amino acids approximately 130 and 330-350 that are essential for targeting. Immunoprecipitation reveals that this region determines whether a construct coassemblies with AP50 and AP17, or with AP47 and AP19. These observations suggest that these other subunits may play an important role in targeting. In contrast, beta- and beta'-adaptins are clearly not involved in this event. Chimeras between the alpha- and gamma-adaptin COOH-terminal domains reveal the presence of a second targeting signal. We have further investigated the interactions between the adaptor subunits using the yeast two-hybrid system. Interactions can be detected between the beta/beta'-adaptins and the alpha/gamma-adaptins, between the beta/beta'-adaptins and the AP50/AP47 subunits, between alpha-adaptin and AP17, and between gamma-adaptin and AP19. These results indicate that the adaptor subunits act in concert to target the complex to the appropriate membrane.

Published

1995

9. The t-SNAREs syntaxin 1 and SNAP-25 are present on organelles that participate in synaptic vesicle recycling.

Author

Walch-Solimena C, Blasi J, Edelmann L, Chapman ER, von Mollard GF, and Jahn R

Subjects

Animals, Antigens, Surface genetics, Antigens, Surface isolation & purification, Botulinum Toxins pharmacology, Brain cytology, Brain metabolism, Calcium Channels, Cell Fractionation, Clathrin, Coated Vesicles chemistry, Coated Vesicles metabolism, GTP-Binding Proteins isolation & purification, Immunohistochemistry, Inositol 1,4,5-Trisphosphate Receptors, Membrane Glycoproteins isolation & purification, Membrane Proteins genetics, Membrane Proteins isolation & purification, Microscopy, Immunoelectron, Nerve Tissue Proteins genetics, Nerve Tissue Proteins isolation & purification, Neurotoxins pharmacology, Organelles chemistry, Qa-SNARE Proteins, R-SNARE Proteins, Rats, Receptors, Cytoplasmic and Nuclear, Recombinant Proteins metabolism, Sodium-Potassium-Exchanging ATPase isolation & purification, Synaptic Vesicles drug effects, Synaptophysin isolation & purification, Synaptosomal-Associated Protein 25, Synaptotagmins, Syntaxin 1, rab3 GTP-Binding Proteins, Antigens, Surface metabolism, Calcium-Binding Proteins, Membrane Proteins metabolism, Nerve Tissue Proteins metabolism, Organelles metabolism, Synaptic Vesicles metabolism

Abstract

Syntaxin 1 and synaptosome-associated protein of 25 kD (SNAP-25) are neuronal plasmalemma proteins that appear to be essential for exocytosis of synaptic vesicles (SVs). Both proteins form a complex with synaptobrevin, an intrinsic membrane protein of SVs. This binding is thought to be responsible for vesicle docking and apparently precedes membrane fusion. According to the current concept, syntaxin 1 and SNAP-25 are members of larger protein families, collectively designated as target-SNAP receptors (t-SNAREs), whose specific localization to subcellular membranes define where transport vesicles bind and fuse. Here we demonstrate that major pools of syntaxin 1 and SNAP-25 recycle with SVs. Both proteins cofractionate with SVs and clathrin-coated vesicles upon subcellular fractionation. Using recombinant proteins as standards for quantitation, we found that syntaxin 1 and SNAP-25 each comprise approximately 3% of the total protein in highly purified SVs. Thus, both proteins are significant components of SVs although less abundant than synaptobrevin (8.7% of the total protein). Immunoisolation of vesicles using synaptophysin and syntaxin specific antibodies revealed that most SVs contain syntaxin 1. The widespread distribution of both syntaxin 1 and SNAP-25 on SVs was further confirmed by immunogold electron microscopy. Botulinum neurotoxin C1, a toxin that blocks exocytosis by proteolyzing syntaxin 1, preferentially cleaves vesicular syntaxin 1. We conclude that t-SNAREs participate in SV recycling in what may be functionally distinct forms.

Published

1995