Faculty Opinions recommendation of Binding of the cytoplasmic domain of CD28 to the plasma membrane inhibits Lck recruitment and signaling.

We have compared the lateral diffusion of intact transmembrane proteins, wild-type H-2Ld antigens, with that of mutants truncated in the cytoplasmic domain. Diffusion coefficients and mobile fractions were similar for all molecules examined, from wild-type Ld antigens with 31 residues on the cytoplasmic side of the plasma membrane to mutants with only four residues in the cytoplasmic domain. This result limits ways in which the lateral diffusion of a major histocompatibility antigen, a transmembrane protein, can be constrained by interactions with other molecules.

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TGN38 recycles basolaterally in polarized Madin-Darby canine kidney cells.

Molecular Biology of the Cell ◽

10.1091/mbc.5.10.1093 ◽

1994 ◽

Vol 5 (10) ◽

pp. 1093-1103 ◽

Cited By ~ 37

Author(s):

A K Rajasekaran ◽

J S Humphrey ◽

M Wagner ◽

G Miesenböck ◽

A Le Bivic ◽

...

Keyword(s):

Plasma Membrane ◽

Mdck Cells ◽

Protein Localization ◽

Evolutionary Relationship ◽

Cytoplasmic Domain ◽

Chimeric Proteins ◽

Madin Darby Canine Kidney ◽

Surface Domains ◽

Darby Canine Kidney ◽

Canine Kidney

Sorting of newly synthesized plasma membrane proteins to the apical or basolateral surface domains of polarized cells is currently thought to take place within the trans-Golgi network (TGN). To explore the relationship between protein localization to the TGN and sorting to the plasma membrane in polarized epithelial cells, we have expressed constructs encoding the TGN marker, TGN38, in Madin-Darby canine kidney (MDCK) cells. We report that TGN38 is predominantly localized to the TGN of these cells and recycles via the basolateral membrane. Analyses of the distribution of Tac-TGN38 chimeric proteins in MDCK cells suggest that the cytoplasmic domain of TGN38 has information leading to both TGN localization and cycling through the basolateral surface. Mutations of the cytoplasmic domain that disrupt TGN localization also lead to nonpolarized delivery of the chimeric proteins to both surface domains. These results demonstrate an apparent equivalence of basolateral and TGN localization determinants and support an evolutionary relationship between TGN and plasma membrane sorting processes.

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Identification of a di-leucine motif within the C terminus domain of the Menkes disease protein that mediates endocytosis from the plasma membrane

Journal of Cell Science ◽

10.1242/jcs.112.11.1721 ◽

1999 ◽

Vol 112 (11) ◽

pp. 1721-1732 ◽

Cited By ~ 2

Author(s):

M.J. Francis ◽

E.E. Jones ◽

E.R. Levy ◽

R.L. Martin ◽

S. Ponnambalam ◽

...

Keyword(s):

Plasma Membrane ◽

Golgi Apparatus ◽

Transmembrane Domain ◽

Menkes Disease ◽

Cytoplasmic Domain ◽

Endocytic Pathway ◽

Site Directed Mutagenesis ◽

Trans Golgi Network ◽

C Terminus ◽

Golgi Network

The protein encoded by the Menkes disease gene (MNK) is localised to the Golgi apparatus and cycles between the trans-Golgi network and the plasma membrane in cultured cells on addition and removal of copper to the growth medium. This suggests that MNK protein contains active signals that are involved in the retention of the protein to the trans-Golgi network and retrieval of the protein from the plasma membrane. Previous studies have identified a signal involved in Golgi retention within transmembrane domain 3 of MNK. To identify a motif sufficient for retrieval of MNK from the plasma membrane, we analysed the cytoplasmic domain, downstream of transmembrane domain 7 and 8. Chimeric constructs containing this cytoplasmic domain fused to the reporter molecule CD8 localised the retrieval signal(s) to 62 amino acids at the C terminus. Further studies were performed on putative internalisation motifs, using site-directed mutagenesis, protein expression, chemical treatment and immunofluorescence. We observed that a di-leucine motif (L1487L1488) was essential for rapid internalisation of chimeric CD8 proteins and the full-length Menkes cDNA from the plasma membrane. We suggest that this motif mediates the retrieval of MNK from the plasma membrane into the endocytic pathway, via the recycling endosomes, but is not sufficient on its own to return the protein to the Golgi apparatus. These studies provide a basis with which to identify other motifs important in the sorting and delivery of MNK from the plasma membrane to the Golgi apparatus.

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Cytoplasmic domains of cellular and viral integral membrane proteins substitute for the cytoplasmic domain of the vesicular stomatitis virus glycoprotein in transport to the plasma membrane.

The Journal of Cell Biology ◽

10.1083/jcb.102.6.2147 ◽

1986 ◽

Vol 102 (6) ◽

pp. 2147-2157 ◽

Cited By ~ 24

Author(s):

L Puddington ◽

C E Machamer ◽

J K Rose

Keyword(s):

Plasma Membrane ◽

G Protein ◽

Vesicular Stomatitis Virus ◽

Heavy Chain ◽

Cytoplasmic Domain ◽

Integral Membrane Proteins ◽

Vesicular Stomatitis Virus Glycoprotein ◽

Hybrid Proteins ◽

Vesicular Stomatitis ◽

Immunoglobulin Mu

Oligonucleotide-directed mutagenesis was used to construct chimeric cDNAs that encode the extracellular and transmembrane domains of the vesicular stomatitis virus glycoprotein (G) linked to the cytoplasmic domain of either the immunoglobulin mu membrane heavy chain, the hemagglutinin glycoprotein of influenza virus, or the small glycoprotein (p23) of infectious bronchitis virus. Biochemical analyses and immunofluorescence microscopy demonstrated that these hybrid genes were correctly expressed in eukaryotic cells and that the hybrid proteins were transported to the plasma membrane. The rate of transport to the Golgi complex of G protein with an immunoglobulin mu membrane cytoplasmic domain was approximately sixfold slower than G protein with its normal cytoplasmic domain. However, this rate was virtually identical to the rate of transport of micron heavy chain molecules measured in the B cell line WEHI 231. The rate of transport of G protein with a hemagglutinin cytoplasmic domain was threefold slower than wild type G protein and G protein with a p23 cytoplasmic domain, which were transported at similar rates. The combined results underscore the importance of the amino acid sequence in the cytoplasmic domain for efficient transport of G protein to the cell surface. Also, normal cytoplasmic domains from other transmembrane glycoproteins can substitute for the G protein cytoplasmic domain in transport of G protein to the plasma membrane. The method of constructing precise hybrid proteins described here will be useful in defining functions of specific domains of viral and cellular integral membrane proteins.

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Role of the Varicella-Zoster Virus gB Cytoplasmic Domain in gB Transport and Viral Egress

Journal of Virology ◽

10.1128/jvi.76.2.591-599.2002 ◽

2002 ◽

Vol 76 (2) ◽

pp. 591-599 ◽

Cited By ~ 31

Author(s):

Thomas C. Heineman ◽

Susan L. Hall

Keyword(s):

Amino Acids ◽

Plasma Membrane ◽

Amino Acid ◽

Varicella Zoster Virus ◽

Cultured Cells ◽

Signal Sequence ◽

Cytoplasmic Domain ◽

Varicella Zoster ◽

Golgi Transport ◽

Viral Egress

ABSTRACT To study the function of the varicella-zoster virus (VZV) gB cytoplasmic domain during viral infection, we produced a VZV recombinant virus that expresses a truncated form of gB lacking the C-terminal 36 amino acids of its cytoplasmic domain (VZV gB-36). VZV gB-36 replicates in noncomplementing cells and grows at a rate similar to that of native VZV. However, cells infected with VZVgB-36 form extensive syncytia compared to the relatively small syncytia formed during native VZV infection. In addition, electron microscopy shows that very little virus is present on the surfaces of cells infected with VZV gB-36, while cells infected with native VZV exhibit abundant virions on the cell surface. The C-terminal 36 amino acids of the gB cytoplasmic domain have been shown in transfection-based experiments to contain both an endoplasmic reticulum-to-Golgi transport signal (the C-terminal 17 amino acids) and a consensus YXXφ (where Y is tyrosine, X is any amino acid, and φ is any bulky hydrophobic amino acid) signal sequence (YSRV) that mediates the internalization of gB from the plasma membrane. As predicted based on these data, gB-36 expressed during the infection of cultured cells is transported inefficiently to the Golgi. Despite lacking the YSRV signal sequence, gB-36 is internalized from the plasma membrane; however, in contrast to native gB, it fails to localize to the Golgi. Therefore, the C-terminal 36 amino acids of the VZV gB cytoplasmic domain are required for normal viral egress and for both the pre- and post-Golgi transport of gB.

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Retention of a cell adhesion complex at the paranodal junction requires the cytoplasmic region of Caspr

The Journal of Cell Biology ◽

10.1083/jcb.200203050 ◽

2002 ◽

Vol 157 (7) ◽

pp. 1247-1256 ◽

Cited By ~ 57

Author(s):

Leora Gollan ◽

Helena Sabanay ◽

Sebastian Poliak ◽

Erik O. Berglund ◽

Barbara Ranscht ◽

...

Keyword(s):

Plasma Membrane ◽

Cell Adhesion ◽

Cell Surface ◽

Cell Adhesion Molecules ◽

Cytoplasmic Domain ◽

Short Sequence ◽

Extracellular Region ◽

A Cell ◽

Adhesion Complex ◽

Protein 4.1B

An axonal complex of cell adhesion molecules consisting of Caspr and contactin has been found to be essential for the generation of the paranodal axo-glial junctions flanking the nodes of Ranvier. Here we report that although the extracellular region of Caspr was sufficient for directing it to the paranodes in transgenic mice, retention of the Caspr–contactin complex at the junction depended on the presence of an intact cytoplasmic domain of Caspr. Using immunoelectron microscopy, we found that a Caspr mutant lacking its intracellular domain was often found within the axon instead of the junctional axolemma. We further show that a short sequence in the cytoplasmic domain of Caspr mediated its binding to the cytoskeleton-associated protein 4.1B. Clustering of contactin on the cell surface induced coclustering of Caspr and immobilized protein 4.1B at the plasma membrane. Furthermore, deletion of the protein 4.1B binding site accelerated the internalization of a Caspr–contactin chimera from the cell surface. These results suggest that Caspr serves as a “transmembrane scaffold” that stabilizes the Caspr/contactin adhesion complex at the paranodal junction by connecting it to cytoskeletal components within the axon.

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The VE-cadherin cytoplasmic domain undergoes proteolytic processing during endocytosis

Molecular Biology of the Cell ◽

10.1091/mbc.e16-09-0658 ◽

2017 ◽

Vol 28 (1) ◽

pp. 76-84 ◽

Cited By ~ 18

Author(s):

Wenji Su ◽

Andrew P. Kowalczyk

Keyword(s):

Plasma Membrane ◽

Adhesion Strength ◽

Turnover Rate ◽

Cytoplasmic Tail ◽

Cytoplasmic Domain ◽

Proteolytic Processing ◽

Endocytic Pathway ◽

Cytoplasmic Domains ◽

P120 Catenin ◽

Binding Domains

VE-cadherin trafficking to and from the plasma membrane has emerged as a critical mechanism for regulating cadherin surface levels and adhesion strength. In addition, proteolytic processing of cadherin extracellular and cytoplasmic domains has been reported to regulate cadherin adhesion and signaling. Here we provide evidence that VE-cadherin is cleaved by calpain upon entry into clathrin-enriched domains. This cleavage event occurs between the β-catenin and p120-binding domains within the cadherin cytoplasmic tail. Of interest, VE-cadherin mutants that are resistant to endocytosis are similarly resistant to cleavage. Furthermore, p120-catenin overexpression blocks cadherin internalization and cleavage, coupling entry into the endocytic pathway with proteolytic processing. Of importance, the cleavage of the VE-cadherin tail alters the postendocytic trafficking itinerary of the cadherin, resulting in a higher turnover rate due to decreased recycling and increased degradation. In conclusion, this study identifies a novel proteolytic event that regulates the trafficking of VE-cadherin after endocytosis.

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Role of Cytoplasmic Domain Serines in Intracellular Trafficking of Furin

Molecular Biology of the Cell ◽

10.1091/mbc.e03-09-0653 ◽

2004 ◽

Vol 15 (6) ◽

pp. 2884-2894 ◽

Cited By ~ 27

Author(s):

Florencia B. Schapiro ◽

Thwe Thwe Soe ◽

William G. Mallet ◽

Frederick R. Maxfield

Keyword(s):

Plasma Membrane ◽

Steady State ◽

Transmembrane Protein ◽

Interleukin 2 ◽

Chimeric Protein ◽

Cytoplasmic Domain ◽

Serine Phosphorylation ◽

Endocytic Recycling ◽

Late Endosomes

Furin is a transmembrane protein that cycles between the plasma membrane, endosomes, and the trans-Golgi network, maintaining a predominant distribution in the latter. It has been shown previously that Tac-furin, a chimeric protein expressing the extracellular and transmembrane domains of the interleukin-2 receptor α chain (Tac) and the cytoplasmic domain of furin, is delivered from the plasma membrane to the TGN through late endosomes, bypassing the endocytic recycling compartment. Tac-furin also recycles in a loop between the TGN and late endosomes. Localization of furin to the TGN is modulated by a six-amino acid acidic cluster that contains two phosphorylatable serines (SDSEED). We investigated the role of these serines in the trafficking of Tac-furin by using a mutant chimera in which the SDS sequence was replaced by the nonphosphorylatable sequence ADA (Tac-furin/ADA). Although the mutant construct is internalized and delivered to the TGN, both the postendocytic trafficking and the steady-state distribution were found to differ from the wild-type. In contrast with Tac-furin, Tac-furin/ADA does not enter late endosomes after being internalized. Instead, it traffics with transferrin to the endocytic recycling compartment, and from there it is delivered to the TGN. As with Tac-furin, Tac-furin/ADA is sorted from the TGN into late endosomes at steady state, but its retrieval from the late endosomes to the TGN is inhibited. These results suggest that serine phosphorylation plays an important role in at least two steps of Tac-furin trafficking, acting as an active sorting signal that mediates the selective sorting of Tac-furin into late endosomes after internalization, as well as its retrieval from late endosomes back to the TGN.

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Rat ovarian lutropin receptor is a transmembrane protein. Evidence for an Mr-20,000 cytoplasmic domain

Biochemical Journal ◽

10.1042/bj2390083 ◽

1986 ◽

Vol 239 (1) ◽

pp. 83-87 ◽

Cited By ~ 7

Author(s):

K P Keinänen ◽

H J Rajaniemi

Keyword(s):

Plasma Membrane ◽

Transmembrane Protein ◽

Membrane Vesicles ◽

Cytoplasmic Domain ◽

Proteolytic Digestion ◽

Plasma Membrane Vesicles ◽

Human Choriogonadotropin ◽

Lutropin Receptor ◽

Membrane Bound ◽

Inside Out

Membrane topography of the rat ovarian lutropin receptor was studied by two different approaches. Ovarian membrane preparation, labelled with 125I-labelled human choriogonadotropin in vivo, was subjected to extensive chymotryptic digestion. The soluble and membrane-bound radioactive complexes were cross-linked with glutaraldehyde, and analysed by SDS/polyacrylamide-gel electrophoresis and autoradiography. Chymotrypsin solubilized 70-75% of the radioactivity as Mr-96,000, Mr-74,000 and Mr-61,000 complexes, and decreased the size of the membrane-bound 125I-labelled human choriogonadotropin-receptor complex from Mr 130,000 to Mr 110,000. The Mr-110,000 complex was not observed when 0.1% Triton X-100 was present in the proteolytic digestion. Enrichment of inside-out-oriented plasma-membrane vesicles by concanavalin A affinity chromatography increased by 70% the fraction of radioactivity that remained in the membrane fraction after chymotrypsin treatment. Chymotrypsin also diminished the size of the membrane-bound unoccupied receptor from Mr 90,000 to Mr 70,000, as detected by ligand (125I-labelled human choriogonadotropin) blotting. These results suggest that the lutropin receptor is a transmembrane protein with a cytoplasmic domain of Mr 20,000 that is sensitive to proteolytic digestion in the inside-out-oriented plasma-membrane vesicles.

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Syntaxin 8 has two functionally distinct di-leucine-based motifs

Cellular & Molecular Biology Letters ◽

10.2478/s11658-007-0043-9 ◽

2008 ◽

Vol 13 (1) ◽

Cited By ~ 6

Author(s):

Kazuo Kasai ◽

Kei Suga ◽

Tetsuro Izumi ◽

Kimio Akagawa

Keyword(s):

Plasma Membrane ◽

Intracellular Localization ◽

Cytoplasmic Domain ◽

Snare Complex ◽

Transport Pathways ◽

First Report ◽

Late Endosomes

AbstractSyntaxin 8 has been shown to form the SNARE complex with syntaxin 7, vti1b and endobrevin. These have been shown to function as the machinery for the homotypic fusion of late endosomes. Recently, we showed that syntaxins 7 and 8 cycle through the plasma membrane, and that the di-leucine-based motifs in the cytoplasmic domain of syntaxins 7 and 8 respectively function in their endocytic and exocytic processes. However, we could not elucidate the mechanism by which syntaxin 8 cycles through the plasma membrane. In this study, we constructed several different syntaxin 8 molecules by mutating putative di-leucine-based motifs, and analyzed their intracellular localization and trafficking. We found a di-leucine-based motif in the cytoplasmic domain of syntaxin 8. It is similar to that of syntaxin 7, and functions in its endocytosis. These results suggest that in the cytoplasmic domain, syntaxin 8 has two functionally distinct di-leucine-based motifs that act independently in its endocytic and exocytic processes. This is the first report on two di-leucine-based motifs in the same molecule acting independently in distinct transport pathways.

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