Transport of a fluorescent phosphatidylcholine analog from the plasma membrane to the Golgi apparatus.

We have examined the internalization and degradation of a fluorescent analog of phosphatidylcholine after its insertion into the plasma membrane of cultured Chinese hamster fibroblasts. 1-acyl-2-(N-4-nitrobenzo-2-oxa-1,3-diazole)-aminocaproyl phosphatidylcholine (C6-NBD-PC) was incorporated into the cell surface by liposome-cell lipid transfer at 2 degrees C. The fluorescent lipid remained localized at the plasma membrane as long as the cells were kept at 2 degrees C; however, when the cells were warmed to 37 degrees C, internalization of some of the fluorescent lipid occurred. Most of the internalized C6-NBD-PC accumulated in the Golgi apparatus although a small amount was found randomly distributed throughout the cytoplasm in punctate fluorescent structures. Internalization of the fluorescent lipid at 37 degrees C was blocked by the presence of inhibitors of endocytosis. Incubation of cells containing C6-NBD-PC at 37 degrees C resulted in a rapid degradation of the fluorescent lipid. This degradation occurred predominantly at the plasma membrane. The degradation of C6-NBD-PC resulted in the release of NBD-fatty acid into the medium. We have compared the internalization of the fluorescent lipid with that of a fluorescent protein bound to the cell surface. Both fluorescent lipid and protein remained at the plasma membrane at 2 degrees C and neither were internalized at 37 degrees C in the presence of inhibitors of endocytosis. However, when incubated at 37 degrees C under conditions that permit endocytosis, the two fluorescent species appeared at different intracellular sites. Our data suggest that there is no transmembrane movement of C6-NBD-PC and that the fluorescent probe reflects the internalization of the outer leaflet of the plasma membrane lipid bilayer. The results are consistent with the Golgi apparatus as being the primary delivery site of phospholipid by bulk membrane movement from the plasma membrane.

Download Full-text

Internalization of Monomeric Lipopolysaccharide Occurs after Transfer Out of Cell Surface Cd14

Journal of Experimental Medicine ◽

10.1084/jem.190.4.509 ◽

1999 ◽

Vol 190 (4) ◽

pp. 509-522 ◽

Cited By ~ 58

Author(s):

Thierry Vasselon ◽

Eric Hailman ◽

Rolf Thieringer ◽

Patricia A. Detmers

Keyword(s):

Plasma Membrane ◽

Green Fluorescent Protein ◽

Golgi Apparatus ◽

Cell Surface ◽

Enhanced Green Fluorescent Protein ◽

Fluorescent Protein ◽

Soluble Cd14 ◽

Stable Transfectants ◽

Intracellular Vesicles ◽

Green Fluorescent

Lipopolysaccharide (LPS) fluorescently labeled with boron dipyrromethane (BODIPY) first binds to the plasma membrane of CD14-expressing cells and is subsequently internalized. Intracellular LPS appears in small vesicles near the cell surface and later in larger, punctate structures identified as the Golgi apparatus. To determine if membrane (m)CD14 directs the movement of LPS to the Golgi apparatus, an mCD14 chimera containing enhanced green fluorescent protein (mCD14–EGFP) was used to follow trafficking of mCD14 and BODIPY–LPS in stable transfectants. The chimera was expressed strongly on the cell surface and also in a Golgi complex–like structure. mCD14–EGFP was functional in mediating binding of and responses to LPS. BODIPY–LPS presented to the transfectants as complexes with soluble CD14 first colocalized with mCD14–EGFP on the cell surface. However, within 5–10 min, the BODIPY–LPS distributed to intracellular vesicles that did not contain mCD14–EGFP, indicating that mCD14 did not accompany LPS during endocytic movement. These results suggest that monomeric LPS is transferred out of mCD14 at the plasma membrane and traffics within the cell independently of mCD14. In contrast, aggregates of LPS were internalized in association with mCD14, suggesting that LPS clearance occurs via a pathway distinct from that which leads to signaling via monomeric LPS.

Download Full-text

Truncations of the C-terminal cytoplasmic domain of MG160, a medial Golgi sialoglycoprotein, result in its partial transport to the plasma membrane and filopodia

Journal of Cell Science ◽

10.1242/jcs.111.2.249 ◽

1998 ◽

Vol 111 (2) ◽

pp. 249-260 ◽

Cited By ~ 2

Author(s):

J.O. Gonatas ◽

Y.J. Chen ◽

A. Stieber ◽

Z. Mourelatos ◽

N.K. Gonatas

Keyword(s):

Amino Acids ◽

Plasma Membrane ◽

Golgi Apparatus ◽

Cell Surface ◽

Chinese Hamster Ovary Cells ◽

Chinese Hamster ◽

Growth Factor Receptor ◽

Cytoplasmic Domain ◽

Type I ◽

Ovary Cells

MG160, a type I cysteine-rich membrane sialoglycoprotein residing in the medial cisternae of the rat Golgi apparatus, is highly homologous to CFR, a fibroblast growth factor receptor, and ESL-1, an E-selectin ligand located at the cell surface of mouse myeloid cells and recently detected in the Golgi apparatus as well. The mechanism for the transport of MG160 from the Golgi apparatus to the cell surface is unknown. In this study we found that differential processing of the carboxy-terminal cytoplasmic domain (CD), consisting of amino acids Arg1159 Ile Thr Lys Arg Val Thr Arg Glu Leu Lys Asp Arg1171, resulted in the partial transport of the protein to the plasma membrane and filopodia. In Chinese hamster ovary cells (CHO), stably transfected with the entire cDNA encoding MG160, the protein was localized in the Golgi apparatus. However, when the terminal Arg1171 or up to nine distal amino acids were deleted, the protein was distributed to the plasma membrane and filopodia as well as the Golgi apparatus. This report shows that the CD of an endogenous type I Golgi protein is important for its efficient retention and identifies a unique residue preference in this process. Cleavage within the CD of MG160 may constitute a regulatory mechanism for the partial export of the protein from the Golgi apparatus to the plasma membrane and filopodia.

Download Full-text

Lipid recycling between the plasma membrane and intracellular compartments: transport and metabolism of fluorescent sphingomyelin analogues in cultured fibroblasts.

The Journal of Cell Biology ◽

10.1083/jcb.108.6.2169 ◽

1989 ◽

Vol 108 (6) ◽

pp. 2169-2181 ◽

Cited By ~ 141

Author(s):

M Koval ◽

R E Pagano

Keyword(s):

Plasma Membrane ◽

Intracellular Transport ◽

Chinese Hamster ◽

Membrane Lipid ◽

Cell Periphery ◽

Perinuclear Region ◽

Cultured Fibroblasts ◽

Plasma Membrane Lipid ◽

Intracellular Compartments ◽

Fluorescent Lipid

We examined the metabolism and intracellular transport of the D-erythro and L-threo stereoisomers of a fluorescent analogue of sphingomyelin, N-(N-[6-[(7-nitrobenz-2-oxa-1,3-diazol-4-yl)amino] caproyl])-sphingosylphosphorylcholine (C6-NBD-SM), in Chinese hamster ovary (CHO-K1) fibroblast monolayers. C6-NBD-SM was integrated into the plasma membrane bilayer by transfer of C6-NBD-SM monomers from liposomes to cells at 7 degrees C. The cells were washed, and within 10-15 min of being warmed to 37 degrees C, C6-NBD-SM was internalized from the plasma membrane to a perinuclear location that colocalized with the centriole and was distinct from the lysosomes and the Golgi apparatus. This perinuclear region was also labeled by internalized rhodamine-conjugated transferrin. C6-NBD-SM endocytosis was not inhibited when the microtubules were disrupted with nocodazole; rather, the fluorescent lipid was distributed in vesicles throughout the cell periphery instead of being internalized to the perinuclear region of the cell. The metabolism of C6-NBD-SM to other fluorescent sphingolipids at 37 degrees C and its effect on C6-NBD-SM transport was also examined. To study plasma membrane lipid recycling, C6-NBD-SM was first inserted into the plasma membrane of CHO-K1 cells and then allowed to be internalized by the cells at 37 degrees C. Any C6-NBD-SM remaining at the plasma membrane was then removed by incubation with nonfluorescent liposomes at 7 degrees C, leaving cells containing only internalized fluorescent lipid. The return of C6-NBD-SM to the plasma membrane from intracellular compartments upon further 37 degrees C incubation was then observed. The half-time for a complete round C6-NBD-SM recycling between the plasma membrane and intracellular compartments was approximately 40 min. Pretreatment of cells with either monensin or nocodazole did not inhibit C6-NBD-SM recycling.

Download Full-text

Direct visualization of Ras proteins in spatially distinct cell surface microdomains

The Journal of Cell Biology ◽

10.1083/jcb.200209091 ◽

2003 ◽

Vol 160 (2) ◽

pp. 165-170 ◽

Cited By ~ 514

Author(s):

Ian A. Prior ◽

Cornelia Muncke ◽

Robert G. Parton ◽

John F. Hancock

Keyword(s):

Plasma Membrane ◽

Cell Surface ◽

Lipid Rafts ◽

Membrane Lipid ◽

Point Pattern Analysis ◽

Immunogold Electron Microscopy ◽

Point Pattern ◽

Ras Proteins ◽

Outer Leaflet ◽

Spatial Point Pattern Analysis

Localization of signaling complexes to specific microdomains coordinates signal transduction at the plasma membrane. Using immunogold electron microscopy of plasma membrane sheets coupled with spatial point pattern analysis, we have visualized morphologically featureless microdomains, including lipid rafts, in situ and at high resolution. We find that an inner-plasma membrane lipid raft marker displays cholesterol-dependent clustering in microdomains with a mean diameter of 44 nm that occupy 35% of the cell surface. Cross-linking an outer-leaflet raft protein results in the redistribution of inner leaflet rafts, but they retain their modular structure. Analysis of Ras microlocalization shows that inactive H-ras is distributed between lipid rafts and a cholesterol-independent microdomain. Conversely, activated H-ras and K-ras reside predominantly in nonoverlapping, cholesterol-independent microdomains. Galectin-1 stabilizes the association of activated H-ras with these nonraft microdomains, whereas K-ras clustering is supported by farnesylation, but not geranylgeranylation. These results illustrate that the inner plasma membrane comprises a complex mosaic of discrete microdomains. Differential spatial localization within this framework can likely account for the distinct signal outputs from the highly homologous Ras proteins.

Download Full-text

Intracellular translocation of fluorescent sphingolipids in cultured fibroblasts: endogenously synthesized sphingomyelin and glucocerebroside analogues pass through the Golgi apparatus en route to the plasma membrane.

The Journal of Cell Biology ◽

10.1083/jcb.100.1.27 ◽

1985 ◽

Vol 100 (1) ◽

pp. 27-34 ◽

Cited By ~ 200

Author(s):

N G Lipsky ◽

R E Pagano

Keyword(s):

Plasma Membrane ◽

Golgi Apparatus ◽

Cell Surface ◽

Chinese Hamster ◽

Fluorescent Labeling ◽

Lung Fibroblasts ◽

Cultured Fibroblasts ◽

Back Exchange ◽

Pass Through ◽

Intracellular Translocation

When monolayer cultures of Chinese hamster lung fibroblasts are briefly incubated at 2 degrees C with the fluorescent sphingolipid analogue, C6-NBD-ceramide (N- [7-(4-nitrobenzo-2-oxa-1,3-diazole)] aminocaproyl sphingosine), fluorescent labeling of the mitochondria, endoplasmic reticulum, and nuclear envelope occur. During further incubation at 37 degrees C, the Golgi apparatus, and later the plasma membrane, become intensely fluorescent. Within this period, the C6-NBD-ceramide is converted to equal amounts of fluorescent sphingomyelin and glucocerebroside (Lipsky, N. G., and R. E. Pagano, 1983, Proc. Natl. Acad. Sci. USA., 80:2608-2612). In the present study, the intracellular translocation of these metabolites and their subsequent appearance at the plasma membrane were investigated by fluorescence microscopy, the addition of the ionophore monensin, and the technique of "back exchange," in which the amounts and types of fluorescent lipids present at the cell surface are identified after their transfer from the cell surface into recipient vesicles. In control cells, the amount of fluorescent glucocerebroside and sphingomyelin that could be removed from the cell surface by back exchange increased during incubation at 37 degrees C, correlating with the increased fluorescence of the plasma membrane observed by microscopy. In the presence of 10 microM monensin, visible labeling of the plasma membrane was greatly diminished, whereas the Golgi apparatus became highly fluorescent and distended. The ability to remove fluorescent metabolites from the cell surface by back exchange was significantly but reversibly inhibited by monensin. Monensin also increased the total amount of fluorescent sphingomyelin, but not the glucocerebroside found in cells. Subcellular fractions were assayed for their ability to convert radiolabeled and fluorescent ceramides to the corresponding sphingomyelins and glucocerebrosides. The activities of parallel fractions coincided, suggesting that the presence of the NBD moiety did not affect the cellular metabolism of ceramide. Furthermore, the major peak of sphingomyelin- and glucocerebroside-synthesizing activity appeared to coincide with an enriched Golgi fraction. These results strongly suggest that fluorescent sphingomyelin was not synthesized at the plasma membrane as has recently been suggested for endogenous sphingomyelin. Rather, both the sphingomyelin and glucocerebroside analogues were synthesized intracellularly from C6-NBD-ceramide and translocated through the Golgi apparatus to the cell surface.

Download Full-text

Specific Retrieval of the Exocytic SNARE Snc1p from Early Yeast Endosomes

Molecular Biology of the Cell ◽

10.1091/mbc.11.1.23 ◽

2000 ◽

Vol 11 (1) ◽

pp. 23-38 ◽

Cited By ~ 250

Author(s):

Michael J. Lewis ◽

Benjamin J. Nichols ◽

Cristina Prescianotto-Baschong ◽

Howard Riezman ◽

Hugh R. B. Pelham

Keyword(s):

Plasma Membrane ◽

Green Fluorescent Protein ◽

Golgi Apparatus ◽

Cell Surface ◽

Immunoelectron Microscopy ◽

Fluorescent Protein ◽

Transmembrane Domain ◽

Early Endosomes ◽

Internal Structures ◽

Green Fluorescent

Many endocytosed proteins in yeast travel to the vacuole, but some are recycled to the plasma membrane. We have investigated the recycling of chimeras containing green fluorescent protein (GFP) and the exocytic SNARE Snc1p. GFP-Snc1p moves from the cell surface to internal structures when Golgi function or exocytosis is blocked, suggesting continuous recycling via the Golgi. Internalization is mediated by a conserved cytoplasmic signal, whereas diversion from the vacuolar pathway requires sequences within and adjacent to the transmembrane domain. Delivery from the Golgi to the surface is also influenced by the transmembrane domain, but the requirements are much less specific. Recycling requires the syntaxins Tlg1p and Tlg2p but not Pep12p or proteins such as Vps4p and Vps5p that have been implicated in late endosome–Golgi traffic. Subtle changes to the recycling signal cause GFP-Snc1p to accumulate preferentially in punctate internal structures, although it continues to recycle to the surface. The internal GFP-Snc1p colocalizes with Tlg1p, and immunofluorescence and immunoelectron microscopy reveal structures that contain Tlg1p, Tlg2p, and Kex2p but lack Pep12p and Sec7p. We propose that these represent early endosomes in which sorting of Snc1p and late Golgi proteins occurs, and that transport can occur directly from them to the Golgi apparatus.

Download Full-text

Transport of (Glyco)Sphingolipids in and Between Cellular Membranes; Multidrug Transporters and Lateral Domains

Bioscience Reports ◽

10.1023/a:1020506726480 ◽

1999 ◽

Vol 19 (4) ◽

pp. 327-333 ◽

Cited By ~ 8

Author(s):

Gerrit van Meer ◽

Dan Sillence ◽

Hein Sprong ◽

Nanette Kälin ◽

René Raggers

Keyword(s):

Plasma Membrane ◽

Cancer Cells ◽

Lipid Bilayer ◽

Membrane Lipid ◽

Golgi Membrane ◽

Cellular Membranes ◽

Multidrug Transporters ◽

Outer Leaflet ◽

Plasma Membrane Lipid ◽

Membrane Lipid Bilayer

Sphingolipids are highly enriched in the outer leaflet of the plasma membrane lipid bilayer. However, the first glycolipid, glucosylceramide, is synthesized in the opposite, cytosolic leaflet of the Golgi membrane. This has led us to experiments which suggest that the level of glucosylceramide in the cytosolic surface is carefully regulated both by the balance between synthesis and hydrolysis and by transport away from this surface through translocators, multidrug transporters, the same molecules that make cancer cells resistant to chemotherapy. Our data suggest a role for newly synthesized glucosylceramide not only in the formation of domains in the luminal leaflet of the Golgi but also on the cytosolic surface of this organelle.

Download Full-text

Time-Course of Changes in the Plasma–Membrane Lipid Bilayer and Cellular Ultrastructure Induced by Tumour Necrosis Factor-α in K 562 and Daudi Cells

Journal of International Medical Research ◽

10.1177/030006059502300405 ◽

1995 ◽

Vol 23 (4) ◽

pp. 254-263 ◽

Cited By ~ 1

Author(s):

M Marutaka ◽

H Iwagaki ◽

K Mizukawa ◽

N Tanaka ◽

K Orita

Keyword(s):

Plasma Membrane ◽

Cell Membrane ◽

Membrane Fluidity ◽

Time Course ◽

Membrane Lipid ◽

Plasma Membrane Lipid ◽

Membrane Lipid Bilayer ◽

Cell Membrane Fluidity ◽

K 562 Cells ◽

Factor Α

The time-course of changes in the plasma-membrane lipid bilayer induced by tumour necrosis factor-α (TNF) were investigated in cultured cells using spin-label electron-spin-resonance techniques. Treatment of K 562 cells, a human chronic myelocytic leukaemia cell line, in suspension culture with TNF for up to 6 h caused an initial increase in cell-membrane fluidity, which returned to the control level after 12 h of treatment. After 24 h of treatment, the cell-membrane fluidity had decreased and this decrease was maintained after 48 h of treatment. In Daudi cells, a human malignant lymphoma cell line, TNF, did not induce any changes in cell-membrane fluidity, indicating that the effect of TNF on membrane structure is cell-specific. The early and transient change in membrane fluidity in K 562 cells is probably related to signal generation, while the later, persistent change may reflect the phenotype of TNF-treated cells, in particular, changes in the plasma membrane-cytoplasmic complex. Histochemical electron microscopic studies indicated that the membrane fluidity changes induced by TNF have an ultrastructural correlate.

Download Full-text

Molecular architecture and dynamics of the plasma membrane lipid bilayer: The red blood cell as a model

Infection ◽

10.1007/bf01644035 ◽

1991 ◽

Vol 19 (S4) ◽

pp. S206-S209 ◽

Cited By ~ 10

Author(s):

B. Roelofsen

Keyword(s):

Plasma Membrane ◽

Blood Cell ◽

Lipid Bilayer ◽

Red Blood Cell ◽

Membrane Lipid ◽

Molecular Architecture ◽

Plasma Membrane Lipid ◽

Membrane Lipid Bilayer

Download Full-text

Disruption of dynamic cell surface architecture of NIH3T3 fibroblasts by the N-terminal domains of moesin and ezrin: in vivo imaging with GFP fusion proteins

Journal of Cell Science ◽

10.1242/jcs.112.1.111 ◽

1999 ◽

Vol 112 (1) ◽

pp. 111-125 ◽

Cited By ~ 7

Author(s):

M.R. Amieva ◽

P. Litman ◽

L. Huang ◽

E. Ichimaru ◽

H. Furthmayr

Keyword(s):

Plasma Membrane ◽

Cell Surface ◽

Fluorescent Protein ◽

Cultured Cells ◽

Full Length ◽

Cell Behavior ◽

Amino Terminal ◽

Terminal Domain ◽

Carboxy Terminal Domain ◽

Carboxy Terminal

Lamellipodia, filopodia, microspikes and retraction fibers are characteristic features of a dynamic and continuously changing cell surface architecture and moesin, ezrin and radixin are thought to function in these microextensions as reversible links between plasma membrane proteins and actin microfilaments. Full-length and truncated domains of the three proteins were fused to green fluorescent protein (GFP), expressed in NIH3T3 cells, and distribution and behaviour of cells were analysed by using digitally enhanced differential interference contrast (DIC) and fluorescence video microscopy. The amino-terminal (N-)domains of all three proteins localize to the plasma membrane and fluorescence recordings parallel the dynamic changes in cell surface morphology observed by DIC microscopy of cultured cells. Expression of this domain, however, significantly affects cell surface architecture by the formation of abnormally long and fragile filopodia that poorly attach and retract abnormally. Even more striking are abundant irregular, branched and motionless membraneous structures that accumulate during retraction of lamellipodia. These are devoid of actin, endogenous moesin, ezrin and radixin, but contain the GFP-labeled domain. While a large proportion of endogenous proteins can be extracted with non-ionic detergents as in untransfected control cells, >90% of N-moesin and >60% of N-ezrin and N-radixin remain insoluble. The minimal size of the domain of moesin required for membrane localization and change in behavior includes residues 1–320. Deletions of amino acid residues from either end result in diffuse intracellular distribution, but also in normal cell behavior. Expression of GFP-fusions of full-length moesin or its carboxy-terminal domain has no effect on cell behavior during the observation period of 6–8 hours. The data suggest that, in the absence of the carboxy-terminal domain, N-moesin, -ezrin and -radixin interact tightly with the plasma membrane and interfere with normal functions of endogeneous proteins mainly during retraction.

Download Full-text