Reconstitution of constitutive secretion using semi-intact cells: regulation by GTP but not calcium.

Regulated exocytosis in many permeabilized cells can be triggered by calcium and nonhydrolyzable GTP analogues. Here we examine the role of these effectors in exocytosis of constitutive vesicles using a system that reconstitutes transport between the trans-Golgi region and the plasma membrane. Transport is assayed by two independent methods: the movement of a transmembrane glycoprotein (vesicular stomatitis virus glycoprotein [VSV G protein]) to the cell surface; and the release of a soluble marker, sulfated glycosaminoglycan (GAG) chains, that have been synthesized and radiolabeled in the trans-Golgi. The plasma membrane of CHO cells was selectively perforated with the bacterial cytolysin streptolysin-O. These perforated cells allow exchange of ions and cytosolic proteins but retain intracellular organelles and transport vesicles. Incubation of the semi-intact cells with ATP and a cytosolic fraction results in transport of VSV G protein and GAG chains to the cell surface. The transport reaction is temperature dependent, requires hydrolyzable ATP, and is inhibited by N-ethylmaleimide. Nonhydrolyzable GTP analogs such as GTP gamma S, which stimulate the fusion of regulated secretory granules, completely abolish constitutive secretion. The rate and extent of constitutive transport between the trans-Golgi and the plasma membrane is independent of free Ca2+ concentrations. This is in marked contrast to fusion of regulated secretory granules with the plasma membrane, and transport between the ER and the cis-Golgi (Beckers, C. J. M., and W. E. Balch. 1989. J. Cell Biol. 108:1245-1256; Baker, D., L. Wuestehube, R. Schekman, and D. Botstein. 1990. Proc. Natl. Acad. Sci. USA. 87:355-359).

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N-glycosylation and topology of the human SLC26 family of anion transport membrane proteins

AJP Cell Physiology ◽

10.1152/ajpcell.00030.2014 ◽

2014 ◽

Vol 306 (10) ◽

pp. C943-C960 ◽

Cited By ~ 27

Author(s):

Jing Li ◽

Fan Xia ◽

Reinhart A. F. Reithmeier

Keyword(s):

Plasma Membrane ◽

Membrane Proteins ◽

Cell Surface ◽

Complex Form ◽

Cell Surface Expression ◽

Intact Cells ◽

Hek 293 ◽

Permeabilized Cells ◽

Glycosylation Sites ◽

High Mannose

The human solute carrier ( SLC26) family of anion transporters consists of 10 members ( SLCA1–11, SLCA10 being a pseudogene) that encode membrane proteins containing ∼12 transmembrane (TM) segments with putative N-glycosylation sites (-NXS/T-) in extracellular loops and a COOH-terminal cytosolic STAS domain. All 10 members of the human SLC26 family, FLAG-tagged at the NH2 terminus, were transiently expressed in HEK-293 cells. While most proteins were observed to contain both high-mannose and complex oligosaccharides, SLC26A2 was mainly in the complex form, SLC26A4 in the high-mannose form, and SLC26A8 was not N-glycosylated. Mutation of the putative N-glycosylation sites showed that most members contain multiple N-glycosylation sites in the second extracytosolic (EC) loop, except SLC26A11, which was N-glycosylated in EC loop 4. Immunofluorescence staining of permeabilized cells localized the proteins to the plasma membrane and the endoplasmic reticulum, with SLC26A2 highly localized to the plasma membrane. N-glycosylation was not a necessary requirement for cell surface expression as the localization of nonglycosylated proteins was similar to their wild-type counterparts, although a lower level of cell-surface biotinylation was observed. No immunostaining of intact cells was observed for any SLC26 members, demonstrating that the NH2-terminal FLAG tag was located in the cytosol. Topological models of the SLC26 proteins that contain an even number of transmembrane segments with both the NH2 and COOH termini located in the cytosol and utilized N-glycosylation sites defining the positions of two EC loops are presented.

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Transport of the membrane glycoprotein of vesicular stomatitis virus to the cell surface in two stages by clathrin-coated vesicles.

The Journal of Cell Biology ◽

10.1083/jcb.86.1.162 ◽

1980 ◽

Vol 86 (1) ◽

pp. 162-171 ◽

Cited By ~ 99

Author(s):

J E Rothman ◽

H Bursztyn-Pettegrew ◽

R E Fine

Keyword(s):

Endoplasmic Reticulum ◽

Plasma Membrane ◽

Golgi Apparatus ◽

Cell Surface ◽

G Protein ◽

Vesicular Stomatitis Virus ◽

Coated Vesicles ◽

Transmembrane Glycoprotein ◽

Vesicular Stomatitis ◽

Two Stages

The G protein of vesicular stomatitis virus is a transmembrane glycoprotein that is transported from its site of synthesis in the rough endoplasmic reticulum to the plasma membrane via the Golgi apparatus. Pulse-chase experiments suggest that G is transported to the cell surface in two successive waves of clathrin-coated vesicles. The oligosaccharides of G protein carried in the early wave are of the "high-mannose" (G1) form, whereas the oligosaccharides in the second, later wave are of the mature "complex" (G2) form. the early wave is therefore proposed to correspond to transport of G in coated vesicles from the endoplasmic reticulum to the Golgi apparatus, and the succeeding wave to transport from the Golgi apparatus to the plasma membrane. The G1- and G2-containing coated vesicles appear to be structurally distinct, as judged by their differential precipitation by anticoated vesicle serum.

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Intermediates in the constitutive and regulated secretory pathways released in vitro from semi-intact cells.

The Journal of Cell Biology ◽

10.1083/jcb.117.3.539 ◽

1992 ◽

Vol 117 (3) ◽

pp. 539-549 ◽

Cited By ~ 46

Author(s):

M Grimes ◽

R B Kelly

Keyword(s):

Secretory Granules ◽

Secretory Cells ◽

Intact Cells ◽

Secretory Pathways ◽

Permeabilized Cells ◽

Pheochromocytoma Cells ◽

Constitutive Secretion ◽

Granule Maturation ◽

Gamma S

Regulated secretory cells have two pathways that transport secreted proteins from the Golgi complex to the cell surface. To identify carrier vesicles involved in regulated and constitutive secretion, PC12 pheochromocytoma cells were labeled with [35S]sulfate to identify markers for the two secretory pathways, then mechanically permeabilized and incubated in vitro. Small constitutive secretory vesicles, containing mostly sulfated proteoglycans, accumulated during an in vitro incubation with ATP. In the presence of GTP gamma S, the constitutive vesicles became significantly more dense, suggesting that a coated intermediate was stabilized. Larger immature regulated secretory granules, enriched in sulfated secretogranin II, also escaped from the permeabilized cells in vitro. During granule maturation, their density increased and the amount of cofractionating proteoglycans diminished. The data suggest that sorting continues during secretory granule maturation.

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Insulin as a surface marker on isolated cells from rat pancreatic islets.

The Journal of Cell Biology ◽

10.1083/jcb.97.2.433 ◽

1983 ◽

Vol 97 (2) ◽

pp. 433-437 ◽

Cited By ~ 24

Author(s):

D R Kaplan ◽

J R Colca ◽

M L McDaniel

Keyword(s):

Plasma Membrane ◽

Cell Surface ◽

Islet Cells ◽

Secretory Granules ◽

Immunoreactive Insulin ◽

Isolated Cells ◽

Intact Cells ◽

Specific Receptors ◽

Specific Membrane ◽

Rat Pancreatic Islet

Immunoreactive insulin was shown to exist as a surface molecule in the plasma membrane of dispersed rat pancreatic islet cells. The intact cells were stained by immunofluorescence with a guinea pig antisera specific for insulin. The hormone on the cell surface could not be accounted for by insulin bound to specific receptors or nonspecifically absorbed to cells. Thus, surface insulin was demonstrated to be a specific membrane antigen for islet cells. Furthermore, the proportion of islet cells with insulin on the cell surface was directly correlated with insulin secretion in several different settings. This correspondence was demonstrated by varying the glucose concentration in the medium, by withholding Ca2+, which inhibits secretion, and by adding theophylline, which potentiates secretion. Consequently, these results suggested that insulin as a membrane protein was a marker for cells that actively secreted the hormone and may have been derived in the fusion process of secretory granules with the plasma membrane.

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Vesicular Transport Is Not Required for the Cytoplasmic Pool of Cholera Toxin To Interact with the Stimulatory Alpha Subunit of the Heterotrimeric G Protein

Infection and Immunity ◽

10.1128/iai.72.12.6826-6835.2004 ◽

2004 ◽

Vol 72 (12) ◽

pp. 6826-6835 ◽

Cited By ~ 13

Author(s):

Ken Teter ◽

Michael G. Jobling ◽

Randall K. Holmes

Keyword(s):

Plasma Membrane ◽

Cell Surface ◽

Cholera Toxin ◽

G Protein ◽

Vesicular Transport ◽

Cytotoxic Action ◽

Anterograde Transport ◽

Heterotrimeric G Protein ◽

Α Subunit ◽

Vesicular Traffic

ABSTRACT Cholera toxin (CT) moves from the cell surface to the endoplasmic reticulum (ER) by retrograde vesicular transport. The catalytic A1 polypeptide of CT (CTA1) then crosses the ER membrane, enters the cytosol, ADP-ribosylates the stimulatory α subunit of the heterotrimeric G protein (Gsα) at the cytoplasmic face of the plasma membrane, and activates adenylate cyclase. The cytosolic pool of CTA1 may reach the plasma membrane and its Gsα target by traveling on anterograde-directed transport vesicles. We examined this possibility with the use of a plasmid-based transfection system that directed newly synthesized CTA1 to either the ER lumen or the cytosol of CHO cells. Such a system allowed us to bypass the CT retrograde trafficking itinerary from the cell surface to the ER. Previous work has shown that the ER-localized pool of CTA1 is rapidly exported from the ER to the cytosol. Expression of CTA1 in either the ER or the cytosol led to the activation of Gsα, and Gsα activation was not inhibited in transfected cells exposed to drugs that inhibit vesicular traffic. Thus, anterograde transport from the ER to the plasma membrane is not required for the cytotoxic action of CTA1.

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Sorting of metabolic pathway flux by the plasma membrane in cerebrovascular smooth muscle cells

AJP Cell Physiology ◽

10.1152/ajpcell.2000.278.4.c803 ◽

2000 ◽

Vol 278 (4) ◽

pp. C803-C811 ◽

Cited By ~ 6

Author(s):

Pamela G. Lloyd ◽

Christopher D. Hardin

Keyword(s):

Smooth Muscle ◽

Plasma Membrane ◽

Major Product ◽

Intact Cells ◽

Glycolytic Intermediate ◽

Cerebral Microvessels ◽

Permeabilized Cells ◽

Direct Contrast ◽

Cerebrovascular Smooth Muscle Cells ◽

Fructose 1,6 Bisphosphate

We used β-escin-permeabilized pig cerebral microvessels (PCMV) to study the organization of carbohydrate metabolism in the cytoplasm of vascular smooth muscle (VSM) cells. We have previously demonstrated (Lloyd PG and Hardin CD. Am J Physiol Cell Physiol 277: C1250–C1262, 1999) that intact PCMV metabolize the glycolytic intermediate [1-13C]fructose 1,6-bisphosphate (FBP) to [1-13C]glucose with negligible production of [3-13C]lactate, while simultaneously metabolizing [2-13C]glucose to [2-13C]lactate. Thus gluconeogenic and glycolytic intermediates do not mix freely in intact VSM cells (compartmentation). Permeabilized PCMV retained the ability to metabolize [2-13C]glucose to [2-13C]lactate and to metabolize [1-13C]FBP to [1-13C]glucose. The continued existence of glycolytic and gluconeogenic activity in permeabilized cells suggests that the intermediates of these pathways are channeled (directly transferred) between enzymes. Both glycolytic and gluconeogenic flux in permeabilized PCMV were sensitive to the presence of exogenous ATP and NAD. It was most interesting that a major product of [1-13C]FBP metabolism in permeabilized PCMV was [3-13C]lactate, in direct contrast to our previous findings in intact PCMV. Thus disruption of the plasma membrane altered the distribution of substrates between the glycolytic and gluconeogenic pathways. These data suggest that organization of the plasma membrane into distinct microdomains plays an important role in sorting intermediates between the glycolytic and gluconeogenic pathways in intact cells.

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p180, a novel recycling transmembrane glycoprotein with restricted cell type expression.

Molecular and Cellular Biology ◽

10.1128/mcb.10.6.2606 ◽

1990 ◽

Vol 10 (6) ◽

pp. 2606-2618 ◽

Cited By ~ 44

Author(s):

C M Isacke ◽

P van der Geer ◽

T Hunter ◽

I S Trowbridge

Keyword(s):

Plasma Membrane ◽

Cell Surface ◽

Biochemical Characterization ◽

Surface Proteins ◽

Sequence Information ◽

Osteosarcoma Cell ◽

Binding Studies ◽

Coated Pits ◽

Transmembrane Glycoprotein ◽

Morphological Studies

A 180-kilodalton (kDa) protein (p180) was identified among the antigens for a panel of monoclonal antibodies raised against human fibroblast cell surface proteins. Binding studies with 125I-Fab' fragments of an anti-p180 monoclonal antibody demonstrated that 10 to 30% of p180 was located on the plasma membrane and that the remaining 70 to 90% was on intracellular membranes. p180 was rapidly internalized from the cell surface at 37 degrees C, and kinetic analyses indicated that this was a constitutive process followed by the recycling of p180 back to the plasma membrane. Morphological studies demonstrated that on the cell surface p180 was concentrated in coated pits, whereas inside the cell it was found in endosomes as suggested by its colocalization with the transferrin receptor. Immunoblot analysis with a polyclonal antiserum raised against purified human protein showed that p180 has a restricted distribution with expression at high levels in fibroblast cultures and in tissues containing cells of mesodermal origin. A biochemical characterization of p180 showed it to be a transmembrane glycoprotein with an extracellular domain, which consists of approximately 30 kDa of complex oligosaccharides attached to at least 45 kDa of the protein core. The cytoplasmic domain of p180 was found to contain a serine residue(s) that was phosphorylated both in vivo and in vitro by activated protein kinase C. p180 was purified by subjecting solubilized membrane proteins from a human osteosarcoma cell line to immunoaffinity chromatography and gel filtration. The N-terminal sequence information obtained from the purified protein showed no homology to other known proteins. It was concluded that p180 may be a novel recycling receptor which is highly restricted in its expression to fibroblastlike cells.

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Dynamic Regulation of a GPCR-Tetraspanin-G Protein Complex on Intact Cells: Central Role of CD81 in Facilitating GPR56-Gαq/11Association

Molecular Biology of the Cell ◽

10.1091/mbc.e03-12-0886 ◽

2004 ◽

Vol 15 (5) ◽

pp. 2375-2387 ◽

Cited By ~ 139

Author(s):

Kevin D. Little ◽

Martin E. Hemler ◽

Christopher S. Stipp

Keyword(s):

Cell Surface ◽

G Protein ◽

Cell Activation ◽

Surface Proteins ◽

Membrane Microdomains ◽

Cholesterol Depletion ◽

Scaffolding Proteins ◽

Intact Cells ◽

Heterotrimeric G Protein ◽

Vast Number

By means of a variety of intracellular scaffolding proteins, a vast number of heterotrimeric G protein–coupled receptors (GPCRs) may achieve specificity in signaling through a much smaller number of heterotrimeric G proteins. Members of the tetraspanin family organize extensive complexes of cell surface proteins and thus have the potential to act as GPCR scaffolds; however, tetraspanin-GPCR complexes had not previously been described. We now show that a GPCR, GPR56/TM7XN1, and heterotrimeric G protein subunits, Gαq, Gα11, and Gβ, associate specifically with tetraspanins and CD81, but not with other tetraspanins. CD9 Complexes of GPR56 with CD9 and CD81 remained intact when fully solubilized and were resistant to cholesterol depletion. Hence they do not depend on detergent-insoluble, raft-like membrane microdomains for stability. A central role for CD81 in promoting or stabilizing a GPR56-CD81-Gαq/11complex was revealed by CD81 immunodepletion and reexpression experiments. Finally, antibody engagement of cell surface CD81 or cell activation with phorbol ester revealed two distinct mechanisms by which GPR56-CD81-Gαq/11complexes can be dynamically regulated. These data reveal a potential role for tetraspanins CD9 and CD81 as GPCR scaffolding proteins.

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Microvillus-specific Mr 75,000 plasma membrane protein of human choriocarcinoma cells.

Journal of Histochemistry & Cytochemistry ◽

10.1177/35.8.3298422 ◽

1987 ◽

Vol 35 (8) ◽

pp. 809-816 ◽

Cited By ~ 40

Author(s):

R Pakkanen ◽

K Hedman ◽

O Turunen ◽

T Wahlström ◽

A Vaheri

Keyword(s):

Electron Microscopy ◽

Plasma Membrane ◽

Membrane Protein ◽

Cell Surface ◽

Polyclonal Antibodies ◽

Apical Cell ◽

Antigenic Site ◽

Electron Microscopic ◽

Permeabilized Cells ◽

Choriocarcinoma Cells

We have previously purified from cultured JEG-3 choriocarcinoma cells an Mr 75,000 protein, originally detected using antibodies to a retrovirus-related synthetic peptide. Using polyclonal antibodies, we have now localized this protein immunocytochemically in JEG-3 cells at both light and electron microscopic levels. In immunofluorescence microscopy of saponin-permeabilized cells, the antigen appeared as dots and short strands at the apical cell surface. In pre-embedding immunoperoxidase electron microscopy, the Mr 75,000 protein was specifically localized to microvilli on the apical cell surface. Immunoferritin electron microscopy was used to assess more quantitatively the antigen distribution in the plane of the plasma membrane, and to define the position of the antigenic site(s) with respect to the membrane. The immunoferritin results confirmed the microvillus specificity of the Mr 75,000 protein and showed that the antigenic portion of the protein is within a few nanometers from, and on the cytoplasmic side of, the lipid bilayer. In detergent extraction experiments, the Mr 75,000 antigen was highly enriched in the soluble fractions. These results demonstrate that the Mr 75,000 protein is a membrane protein highly specific for microvilli.

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Osmotically sensitive renin release from permeabilized juxtaglomerular cells

AJP Renal Physiology ◽

10.1152/ajprenal.1993.265.1.f87 ◽

1993 ◽

Vol 265 (1) ◽

pp. F87-F95 ◽

Cited By ~ 3

Author(s):

B. L. Jensen ◽

O. Skott

Keyword(s):

Secretory Granules ◽

Sucrose Concentration ◽

Proximal Tubules ◽

Renin Release ◽

Continuous Exposure ◽

Juxtaglomerular Cells ◽

Water Fluxes ◽

Intact Cells ◽

Permeabilized Cells ◽

Cellular Volume

Renin secretion from juxtaglomerular (JG) cells is sensitive to external osmolality in a way that has been suggested to depend either on cellular volume or on effects on secretory granules. To distinguish between these possibilities, a technique for permeabilization of JG cell membranes was developed. Rat glomeruli with attached JG cells were isolated and permeabilized by 20 microM digitonin for 12 min and followed by continuous exposure to 2 microM digitonin. Experiments on proximal tubules showed that cellular volume was unaffected by changes in external sucrose concentration after a similar permeabilization procedure. With permeabilized JG cells the following changes in osmolality were tested (in mM sucrose): +90 (n = 6), +60 (n = 5), +30 (n = 6), +15 (n = 6), -15 (n = 5), -30 (n = 6), -60 (n = 6), and -90 (n = 6). With nonpermeabilized cells similar experiments were done with changes of +90 (n = 7), +30 (n = 4), -30 (n = 4), and -90 (n = 6) mM sucrose. Increases in osmolality caused inhibition of renin release, whereas decreases stimulated secretion. Within +/- 10% variations in osmolality there were no differences between the responses in permeabilized and intact cells, whereas the responses with larger changes were less in the permeabilized cells. Increase or decrease in urea concentration by 30 mM did not affect renin release. Thus water fluxes can influence renin release by a mechanism that is independent of cell volume.

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