Elucidation of the Role of the Exocyst Subunit Sec6p in Exocytosis: A Dissertation

Brewer, Daniel Niron

23 November 2009

Trafficking of protein and lipid cargo through the secretory pathway in eukaryotic cells is mediated by membrane-bound vesicles. Secretory vesicles are targeted to sites of exocytosis on the plasma membrane in part by a conserved multi-subunit protein complex termed the exocyst. In addition to tethering vesicles to the plasma membrane, the exocyst complex and components therein may also add a layer of regulation by directly controlling assembly of the SNARE complex, which is required for membrane fusion, as well as other regulatory factors such as Sec1p. In the past, we have shown that Sec6p interacts with Sec9p in vivo and that that interaction retards binary SNARE complex formation in a SNARE assembly assay. Though many interactions have been mapped using in vitro methods, confirming them in vivoand placing them into the context of a complete model that accounts for all observed interactions (and lack of interactions) has proven difficult. In order to address these problems, I have studied the interactions between Sec6p and other factors involved in exocytosis at the plasma membrane via in vivo methods. My hypothesis was that Sec6p interaction with Sec9p and subsequent inhibition of SNARE complex assembly in vitro was an intermediate state and Sec6p was part of a set of cofactors that accelerated SNARE complex assembly in vivo. To test this hypothesis I showed that the interaction between the plasma membrane t-SNARE Sec9p and the yeast exocyst subunit Sec6p can be observed in vivoand designed point mutations to disrupt that interaction. Interestingly, I also showed that Sec6p:Sec9p interaction involves the free pool of Sec6p rather than the exocyst bound fraction of Sec6p. Point mutations in the N-terminal domain of Sec6p result in temperature sensitive growth and secretion defects, without loss of Sec6p-Sec9p interaction. However, at the non-permissive temperature, the exocyst subunits Sec5p, Sec10p and Sec15p are mislocalized and are absent from the exocyst complex. The resulting subcomplex, containing Sec3p, Sec8p, Exo70p and Exo84p, remains stably assembled and localized at sites of polarized secretion. This subcomplex is likely due to disruption of interaction between Sec6p and Sec5p, and may be similar to that observed at restrictive temperatures in the sec6-54temperature sensitive mutant. Additionally, one of the sec6 temperature sensitive mutants displays a loss of binding to the yeast regulatory protein Sec1p. In vitro binding studies indicate a direct interaction between Sec1p and the free pool of the wild-type Sec6p protein, suggesting close interplay between Sec6p and Sec1p in the regulation of SNARE complexes. A coherent model which incorporates all these interactions has continued to be elusive. However, the results I have found do suggest several hypotheses which should prove testable in the future.

SNARE Proteins

Vesicular Transport Proteins

Exocytosis

Amino Acids, Peptides, and Proteins

Cells

Genetic Phenomena

SNARE-Mediated Exocytosis of Atrial Natriuretic Peptide from Atrial Cardiac Myocytes

Peters, Christian G.

13 June 2007

No description available.

atrial natriuretic peptide

exocytosis

atrial myocytes

Ca2+ imaging

membrane capacitance

SNARE proteins

Úloha SNARE proteinu v biogenezi mitosomů Giardia intestinalis. / Role of a SNARE protein in the biogenesis of Giardia intestinalis mitosomes.

Voleman, Luboš

January 2011

SNARE proteins play essential role in most membrane fusions taking place in eukaryotic cell. They are responsible for all fusions that occur across endocytic and secretory pathways. Apart from these processes stand mitochondria and plastids. Fusion of these organelles is directed by specific protein machineries. In this work we review up-to-date information on SNARE mediated membrane fusion and fusion of outer and inner mitochondrial membranes with an emphasis on situation in flagellated protozoan parasite Giradia intestinalis. It was suggested that one of typical SNARE protein in Giardia (GiSec20) is localised to its highly reduced mitochondria called mitosomes. This protein is also essential for surviving of Giardia trophozoites. In this work we show that mitosomal localization of Gisec20 is caused by episomal expression however the protein is localised to endoplasmic reticulum under physiological conditions. Using GFP tag we were able to characterize its targeting signal which showed to be localised in transmembrane domain of GiSec20. This signal targets the protein to mitosomes of G. intestinalis and S. cerevisiae, respectively. Mitosomal localization was prevented by adding 3'UTR to gene sequence and its episomal expression. This suggests existence of targeting mechanism based on information...

The Exocyst Subunit Sec6 Interacts with Assembled Exocytic Snare Complexes: A Dissertation

Dubuke, Michelle L.

18 December 2015

In eukaryotic cells, membrane-bound vesicles carry cargo between intracellular compartments, to and from the cell surface, and to the extracellular environment. Many conserved families of proteins are required for properly localized vesicle fusion, including the multi-subunit tethering complexes and the SNARE complexes. These protein complexes work together to promote proper vesicle fusion in other trafficking pathways. Contrary to these other pathways, our lab previously suggested that the exocyst subunit Sec6, a component of the exocytosis-specific tethering complex, inhibited Sec9:Sso1 SNARE complex assembly due to interactions in vitro with the SNARE protein Sec9 (Sivaram et al., 2005). My goal for this project was to test the hypothesis that Sec6 inhibited SNARE complex assembly in vivo. I therefore chose to generate Sec6:Sec9 loss-of-binding mutants, and study their effect both in vitro and in vivo. I identified a patch of residues on Sec9 that, when mutated, are sufficient to disrupt the novel Sec6-SNARE interaction. Additionally, I found that the previous inhibitory role for Sec6 in SNARE assembly was due to a data mis-interpretation; my re-interpretation of the data shows that Sec6 has a mild, if any, inhibitory effect on SNARE assembly. My results suggest a potential positive role for Sec6 in SNARE complex assembly, similar to the role observed for other tether-SNARE interactions.

SNARE Proteins

Saccharomyces cerevisiae Proteins

Vesicular Transport Proteins

Exocysts

Exocyst Subunit Sec6

Dissertations, UMMS

Biochemistry

Cell and Developmental Biology

Molecular Biology

Biophysikalische und thermodynamische Charakterisierung der neuronalen SNARE-Komplexbildung / Biophysical and Thermodynamical Characterization of the Neuronal SNARE Complex Formation

Wiederhold, Katrin

30 April 2008

No description available.

570 Biowissenschaften, Biologie

Mathematics and Computer Science

Membranfusion

SNARE-Proteine

Komplexbildung

membrane fusion

SNARE proteins

complex assembly

35.73 Biochemische Reaktionen

Biophysical Characterization of SNARE Complex Disassembly Catalyzed by NSF and alphaSNAP

Winter, Ulrike

03 July 2008

No description available.

570 Biowissenschaften, Biologie

Mathematics and Computer Science

alphaSNAP

NSF

SNARE-Proteine

Membranfusion

SNARE-recycling

AAA-ATPasen

alphaSNAP

NSF

SNARE-Proteins

membrane fusion

SNARE-recycling

AAA-ATPases

42.12 Biophysik

WC

Zur Bedeutung von Zytoskelett-Membran-Verbindungen für die gerichtete HCI-Sekretion von Parietalzellen

Jöns, Thomas

16 May 2001

Die in der vorliegenden Habilitationsschrift zusammengefaßten Publikationen stellen Untersuchungen zu zwei Themenschwerpunkten dar: 1. Verankerungsmechanismen von Membranproteinen der basolateralen und der apikalen Plasmamembrandomäne der Parietalzellen mit dem Membranzytoskelett und 2. die regulierte Fusion von zytoplasmatischen Vesikeln mit der apikalen Plasmamembran dieser Zellen. Die strukturell und molekular sehr unterschiedlich gestaltete apikale und basolaterale Membrandomäne der Parietalzellen sollte funktionell charakterisiert und die Mechanismen der Membranumbauvorgänge aufgeklärt werden, die nach Aktivierung der Zellen im apikalen Membrankompartiment ablaufen. Für die strukturelle Stabilität der basolateralen Domäne spielt wahrscheinlich die Verankerung von AE2 über das Verknüpfungsprotein Ankyrin mit dem Membranzytoskelett eine wichtige Rolle. Die apikale Membrandomäne der Parietalzellen kann in drei Kompartimente unterteilt werden. Die freie apikale Membran, die canalikuläre Membran und die Membranen der tubulären Vesikel. Entlang der freien apikalen und der canaliculären Plasmamembran kommen wie auf der basolateralen Seite die Zytoskelett-Proteine Actin und Spectrin vor. Nach unseren Untersuchungen könnte es während der Sekretionsphase zu einer temporären Verbindung von H+,K+-ATPase Molekülen mit dem Membranzytoskelett kommen. Diese Verbindung wird wahrscheinlich durch das Verknüpfungsprotein Ezrin vermittelt. Der Mechanismus des Fusionsvorgangs der tubulären Vesikel mit der canaliculären Membran war bisher nicht bekannt. In Parietalzellen konnten die neuronalen SNARE-Proteine Synaptobrevin 2, Syntaxin 1 und SNAP25 sowie das zur Familie der kleinen G-Proteine gehörende Protein Rab3A und die Regulatorproteine NSF und alpha/beta SNAP nachgewiesen werden. Das in Parietalzellen gefundene Verteilungsmuster der SNARE-Proteine entspricht nicht der klassischen Vorstellung einer heterotypischen Membranfusion, vielmehr entspricht diese Verteilung einer homotypischen Fusion, wie sie für Vakuolen in Hefezellen beschrieben wurde. Die Bedeutung der SNARE-Proteine für die Fusion der tubulären Vesikel mit der canaliculären Membran und damit für die Steigerung der HCl-Sekretion konnte durch Inkubation der Zellen mit Tetanus Neurotoxin (TeNt) gezeigt werden. Die Behandlung der Parietalzellen mit TeNt führte zum vollständigen Ausbleiben der, nach Stimulation mit cAMP bei Kontrollzellen beobachteten Erhöhung, der Säuresekretion / The publications summarized here cover two topics: 1. the anchorage mechanism of membrane proteins of the basolateral and the apical plasma membrane with the membrane cytoskeleton of parietal cells and 2. the regulated fusion of cytoplasmic vesicles with the apical plasma membrane of these cells. It was the aim of these studies to characterize the structural and molecular differences between the apical and basolateral membrane domains in parietal cells. Moreover the mechanisms involved in membrane traffic within the apical membrane compartment following stimulation were investigated. We found that anchorage of AE2 with the membrane cytoskeleton through the linkage protein ankyrin seems to be important for the stability of the basolateral membrane. The apical membrane domain of parietal cells can be subdivided into three compartments. The free apical membrane, the canalicular membrane and the tubulovesicular membrane. The cytoskeletal proteins spectrin and actin can be found at the basolateral, the free apical and the canalicular membrane. We have shown that the H+K+-ATPase molecules appear to be temporary linked to the membrane cytoskeleton during acid-secretion. This contact is most likely mediated by the linker-protein ezrin. Until now the mechanism of fusion of the tubulovesicles with the canalicular membrane was unknown. In parietal cells the neuronal SNARE-proteins synaptobrevin 2, Syntaxin 1, SNAP25, the small G-protein rab3A, and the regulatory proteins NSF and alpha/beta-SNAP were detected. The subcellular distribution of these proteins does not support the notion of a neuron-like heterotypic fusion. Instead it shows similarity with the homotypic fusion process of vacuoles in yeast. The importance of SNARE-proteins for the fusion of tubulovesicles with the canalicular membrane and, by consequence also for the increase of acid-secretion was shown by incubation of the cells with tetanus neurotoxin (TeNt). The measurable increase of acid secretion by parietal cells after stimulation with c-AMP was inhibited completely through an incubation with TeNt.

Parietalzellen

Polarität

Membranzytoskelett

SNARE-Proteine

AE2

Ankyrin

Ezrin

Parietal cells

polarity

membrane cytoskeleton

SNARE-proteins

AE2

ankyrin

ezrin

610 Medizin

33 Medizin

WE 2600

ddc:610

Characterisation of Vti1b and Vti1a proteins and generation of knock-out mice. / Studies of endosomal transport proteins using targeted gene replacement of SNAREs in mouse. / Characterisierung von Vti1b und Vti1a Proteinen und Erzeugung von knockout Mäusen. / Untersuchungen von endosomalen Transportproteinen durch Genausschaltung von SNAREs in Maus.

Atlachkine, Vadim

20 June 2002

No description available.

570 Biowissenschaften, Biologie

Mathematics and Computer Science

SNARE Proteine

Vti1b

Vti1a

Knockout Mäuse

Proteintransport

späten Endosomen

Lysosomen

SNARE proteins

Vti1b

Vti1a

knockout mice

protein transport

late endosomes

lysosomes

WA

WH

WHC700

WHF800

Charakterisierung der endosomalen Qb-SNAREs Vti1a und Vti1b / Characterization of the endosomal Qb-SNAREs Vti1a and Vti1b

Kreykenbohm, Vera

03 November 2004

No description available.

570 Biowissenschaften, Biologie

Mathematics and Computer Science

SNARE-Proteine

Membrantransport

Endosomen

Lysosomen

Knockout-Mäuse

Vti1

Vti1a

Vti1b

SNARE proteins

membrane traffic

endosomes

lysosomes

knockout mice

Vti1

Vti1a

Vti1b

42.13 Molekularbiologie

42.15 Zellbiologie

35.70 Biochemie: Allgemeines

WA

WH

WHC100

WHC500

WHC700

WHF800

Charakterisierung von SNARE-Proteinen in der Hefe Saccharomyces cerevisiae / Characterization of SNARE proteins in the yeast Saccharomyces cerevisiae

Dilcher, Meik

30 January 2003

No description available.

570 Biowissenschaften, Biologie

Mathematics and Computer Science

SNARE-Proteine

Membrantransport

Saccharomyces cerevisiae

VTI1

VTS1

YKT6

USE1

SNARE proteins

membrane traffic

Saccharomyces cerevisiae

VTI1

VTS1

YKT6

USE1

42.15 Zellbiologie

42.13 Molekularbiologie

35.70 Biochemie

WA

WH

WHC700

WHF800