The Carboxy-Terminal Sequence of the Pestivirus Glycoprotein Erns Represents an Unusual Type of Membrane Anchor

ABSTRACT The Erns protein is a structural glycoprotein of pestiviruses that lacks a typical membrane anchor sequence and is known to be secreted from the infected cell. However, major amounts of the protein are retained within the cell and attached to the virion by a so far unknown mechanism. Transient-expression studies with cDNA constructs showed that in a steady-state situation, 16% of the protein is found in the supernatant of the transfected cells while 84% appears as intracellular protein. We show here that Erns represents a membrane-bound protein. Membrane binding occurs via the carboxy-terminal region of Erns. By fusion of this sequence to the carboxy terminus of green fluorescent protein (GFP), the subcellular localization of the reporter protein switched from cytosolic to membrane bound. A core sequence of 11 amino acids necessary for membrane binding was elicited in truncation experiments with GFP constructs. However, this peptide is not sufficient to confer membrane anchoring but needs either upstream or downstream accessory sequences. Analyses with different extraction procedures showed that Erns is neither easily stripped from the membrane, like a peripheral membrane protein, nor as tightly membrane bound as a transmembrane protein.

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Contribution of Membrane-Binding and Enzymatic Domains of Penicillin Binding Protein 5 to Maintenance of Uniform Cellular Morphology of Escherichia coli

Journal of Bacteriology ◽

10.1128/jb.184.13.3630-3639.2002 ◽

2002 ◽

Vol 184 (13) ◽

pp. 3630-3639 ◽

Cited By ~ 39

Author(s):

David E. Nelson ◽

Anindya S. Ghosh ◽

Avery L. Paulson ◽

Kevin D. Young

Keyword(s):

Escherichia Coli ◽

Site Directed Mutagenesis ◽

Outer Face ◽

Penicillin Binding Protein ◽

Membrane Anchor ◽

E Coli ◽

Membrane Bound ◽

Carboxy Terminal ◽

Membrane Anchoring ◽

Β Sheet

ABSTRACT Four low-molecular-weight penicillin binding proteins (LMW PBPs) of Escherichia coli are closely related and have similar dd-carboxypeptidase activities (PBPs 4, 5, and 6 and DacD). However, only one, PBP 5, has a demonstrated physiological function. In its absence, certain mutants of E. coli have altered diameters and lose their uniform outer contour, resulting in morphologically aberrant cells. To determine what differentiates the activities of these LMW PBPs, we constructed fusion proteins combining portions of PBP 5 with fragments of other dd-carboxypeptidases to see which hybrids restored normal morphology to a strain lacking PBP 5. Functional complementation occurred when truncated PBP 5 was combined with the terminal membrane anchor sequences of PBP 6 or DacD. However, complementation was not restored by the putative carboxy-terminal anchor of PBP 4 or by a transmembrane region of the osmosensor protein ProW, even though these hybrids were membrane bound. Site-directed mutagenesis of the carboxy terminus of PBP 5 indicated that complementation required a generalized amphipathic membrane anchor but that no specific residues in this region seemed to be required. A functional fusion protein was produced by combining the N-terminal enzymatic domain of PBP 5 with the C-terminal β-sheet domain of PBP 6. In contrast, the opposite hybrid of PBP 6 to PBP 5 was not functional. The results suggest that the mode of PBP 5 membrane anchoring is important, that the mechanism entails more than a simple mechanical tethering of the enzyme to the outer face of the inner membrane, and that the physiological differences among the LMW PBPs arise from structural differences in the dd-carboxypeptidase enzymatic core.

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Recruitment of the LIM protein hic-5 to focal contacts of human platelets

Journal of Cell Science ◽

10.1242/jcs.111.15.2181 ◽

1998 ◽

Vol 111 (15) ◽

pp. 2181-2188 ◽

Cited By ~ 1

Author(s):

J. Hagmann ◽

M. Grob ◽

A. Welman ◽

G. van Willigen ◽

M.M. Burger

Keyword(s):

Fluorescent Protein ◽

Human Platelets ◽

Gene Encoding ◽

Chain Reactions ◽

Amino Terminal ◽

Culture Cells ◽

Lim Domains ◽

Focal Contacts ◽

Green Fluorescent ◽

Carboxy Terminal

Platelets are anuclear, membrane-bounded fragments derived from megakaryocytes which, upon stimulation, assemble an actin skeleton including stress fibres and focal contacts. The focal contacts resemble those of tissue culture cells. However, they lack paxillin, a conspicuous component of these organelles. We found that instead of paxillin, platelets contain a related protein with a molecular mass of 55 kDa that crossreacts with a monoclonal antibody against paxillin. The gene for the 55 kDa protein was cloned from a bone marrow cDNA library and turned out to be identical to a recently discovered gene encoding hic-5. Like paxillin, hic-5 is a cytoskeletal protein containing four carboxy-terminal LIM domains and LD motifs in the amino-terminal half. The LIM domains of both hic-5 and paxillin are capable of targetting green fluorescent protein to focal contacts. In addition, GST-hic-5 precipitates the focal adhesion kinase pp125(FAK) and talin from platelet extracts. Only trace amounts of hic-5 occur in DAMI cells, a megakaryocytic cell line, and in megakaryocytes cultured from CD34+ cells obtained from umbilical cord blood. However, RT-polymerase chain reactions performed with RNA obtained from platelets gave a positive result when primers specific for hic-5 were used, but were negative with paxillin-specific primers, indicating that a switch from paxillin expression to hic-5 expression must occur late in the maturation of megakaryocytes into platelets.

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Na+-dependent phosphate transporters in the murine osteoclast: cellular distribution and protein interactions

AJP Cell Physiology ◽

10.1152/ajpcell.00580.2002 ◽

2003 ◽

Vol 284 (6) ◽

pp. C1633-C1644 ◽

Cited By ~ 37

Author(s):

Mohammed A. Khadeer ◽

Zhihui Tang ◽

Harriet S. Tenenhouse ◽

Maribeth V. Eiden ◽

Heini Murer ◽

...

Keyword(s):

Plasma Membrane ◽

Bone Resorption ◽

Protein Interactions ◽

Cellular Localization ◽

Fluorescent Protein ◽

Basolateral Membrane ◽

Atp Synthesis ◽

Cellular Distribution ◽

Green Fluorescent ◽

Carboxy Terminal

We previously demonstrated that inhibition of Na-dependent phosphate (Pi) transport in osteoclasts led to reduced ATP levels and diminished bone resorption. These findings suggested that Na/Picotransporters in the osteoclast plasma membrane provide Pifor ATP synthesis and that the osteoclast may utilize part of the Pireleased from bone resorption for this purpose. The present study was undertaken to define the cellular localization of Na/Picotransporters in the mouse osteoclast and to identify the proteins with which they interact. Using glutathione S-transferase (GST) fusion constructs, we demonstrate that the type IIa Na/Picotransporter (Npt2a) in osteoclast lysates interacts with the Na/H exchanger regulatory factor, NHERF-1, a PDZ protein that is essential for the regulation of various membrane transporters. In addition, NHERF-1 in osteoclast lysates interacts with Npt2a in spite of deletion of a putative PDZ-binding domain within the carboxy terminus of Npt2a. In contrast, deletion of the carboxy-terminal TRL amino acid motif of Npt2a significantly reduced its interaction with NHERF-1 in kidney lysates. Studies in osteoclasts transfected with green fluorescent protein-Npt2a constructs indicated that Npt2a colocalizes with NHERF-1 and actin at or near the plasma membrane of the osteoclast and associates with ezrin, a linker protein associated with the actin cytoskeleton, likely via NHERF-1. Furthermore, we demonstrate by RT/PCR of osteoclast RNA and in situ hybridization that the type III Na/Picotransporter, PiT-1, is also expressed in mouse osteoclasts. To examine the cellular distribution of PiT-1, we infected mouse osteoclasts with a retroviral vector encoding PiT-1 fused to an epitope tag. PiT-1 colocalizes with actin and is present on the basolateral membrane of the polarized osteoclast, similar to that previously reported for Npt2a. Taken together, our data suggest that association of Npt2a with NHERF-1, ezrin, and actin, and of PiT-1 with actin, may be responsible for membrane sorting and regulation of these Na/Picotransporters in the osteoclast.

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Two Point Mutations Produce Infectious Retrovirus Bearing a Green Fluorescent Protein-SU Fusion Protein

Journal of Virology ◽

10.1128/jvi.75.23.11881-11885.2001 ◽

2001 ◽

Vol 75 (23) ◽

pp. 11881-11885 ◽

Cited By ~ 6

Author(s):

Krishnakumar Kizhatil ◽

Adam Gromley ◽

Lorraine M. Albritton

Keyword(s):

Green Fluorescent Protein ◽

Envelope Protein ◽

Structural Changes ◽

Fluorescent Protein ◽

Fundamental Problem ◽

Transmembrane Protein ◽

Strong Association ◽

Slight Reduction ◽

Virus Envelope ◽

Green Fluorescent

ABSTRACT Two second-site mutations in Moloney murine leukemia virus envelope surface protein (SU) were previously shown to rescue infection of two different SU mutants, a fusion-defective point mutant and a fusion-defective modified SU that exhibits weak subunit association. We report here that they also rescue infection of a third defective SU, one modified by insertion of the green fluorescent protein (GFP) between serine 6 and proline 7. GFP-SU assembled into virions and showed a strong association with the transmembrane protein (TM). However, these virions were noninfectious. GFP-SU expression was not maintained within cells, suggesting that the protein was toxic. Addition of the second-site mutations rendered the GFP-SU virus infectious and resulted in prolonged expression of the modified envelope protein. This virus showed a slight reduction in receptor binding but not in envelope protein processing, suggesting that addition of the GFP sequences results in subtle structural changes. Extrapolating these data, we see that the fundamental problem with the GFP-SU envelope protein appears to be a folding problem, suggesting that the second-site mutations rescue GFP-SU primarily by a mechanism that involves stabilizing the envelope protein structure.

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Structural Determinants Required To Target Penicillin-Binding Protein 3 to the Septum of Escherichia coli

Journal of Bacteriology ◽

10.1128/jb.186.18.6110-6117.2004 ◽

2004 ◽

Vol 186 (18) ◽

pp. 6110-6117 ◽

Cited By ~ 44

Author(s):

André Piette ◽

Claudine Fraipont ◽

Tanneke den Blaauwen ◽

Mirjam E. G. Aarsman ◽

Soumya Pastoret ◽

...

Keyword(s):

Escherichia Coli ◽

Cell Division ◽

Fluorescent Protein ◽

Binding Protein ◽

Penicillin Binding Protein ◽

Structural Determinants ◽

Membrane Anchor ◽

Interaction Sites ◽

Division Site ◽

Green Fluorescent

ABSTRACT In Escherichia coli, cell division is mediated by the concerted action of about 12 proteins that assemble at the division site to presumably form a complex called the divisome. Among these essential division proteins, the multimodular class B penicillin-binding protein 3 (PBP3), which is specifically involved in septal peptidoglycan synthesis, consists of a short intracellular M1-R23 peptide fused to a F24-L39 membrane anchor that is linked via a G40-S70 peptide to an R71-I236 noncatalytic module itself linked to a D237-V577 catalytic penicillin-binding module. On the basis of localization analyses of PBP3 mutants fused to green fluorescent protein by fluorescence microscopy, it appears that the first 56 amino acid residues of PBP3 containing the membrane anchor and the G40-E56 peptide contain the structural determinants required to target the protein to the cell division site and that none of the putative protein interaction sites present in the noncatalytic module are essential for the positioning of the protein to the division site. Based on the effects of increasing production of FtsQ or FtsW on the division of cells expressing PBP3 mutants, it is suggested that these proteins could interact. We postulate that FtsQ could play a role in regulating the assembly of these division proteins at the division site and the activity of the peptidoglycan assembly machineries within the divisome.

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High Physiological Levels of LMP1 Result in Phosphorylation of eIF2α in Epstein-Barr Virus-Infected Cells

Journal of Virology ◽

10.1128/jvi.78.4.1657-1664.2004 ◽

2004 ◽

Vol 78 (4) ◽

pp. 1657-1664 ◽

Cited By ~ 48

Author(s):

Ngan Lam ◽

Mark L. Sandberg ◽

Bill Sugden

Keyword(s):

Gene Expression ◽

Epstein Barr Virus ◽

Fluorescent Protein ◽

Transmembrane Domain ◽

Barr Virus ◽

Signaling Domain ◽

Infected Cells ◽

Epstein Barr ◽

Green Fluorescent ◽

Carboxy Terminal

ABSTRACT LMP1 is an Epstein-Barr virus (EBV)-encoded membrane protein essential for the proliferation of EBV-infected lymphoblasts (E. Kilger, A. Kieser, M. Baumann, and W. Hammerschmidt, EMBO J. 17:1700-1709, 1998). LMP1 also inhibits gene expression and induces cytostasis in transfected cells when it is expressed at levels as little as twofold higher than the average for EBV-positive lymphoblasts (M. Sandberg, A. Kaykas, and B. Sugden, J. Virol. 74:9755-9761, 2000; A. Kaykas and B. Sugden, Oncogene 19:1400-1410, 2000). We have found that in three different clones of EBV-infected lymphoblasts the levels of expression of LMP1 in individual cells in each clone ranged over 100-fold. This difference is due to a difference in levels of the LMP1 transcript. In these clones, cells expressing high levels of LMP1 incorporated less BrdU. We also found that induction of expression of LMP1 or of a derivative of LMP1 with its transmembrane domain fused to green fluorescent protein instead of its carboxy-terminal signaling domain resulted in phosphorylation of eIF2α in EBV-negative Burkitt's lymphoma cells. This induction of phosphorylation of eIF2α was also detected in EBV-infected lymphoblasts, in which high levels of LMP1 correlated with high levels of phosphorylation of eIF2α. Our results indicate that inhibition of gene expression and of cell proliferation by LMP1 occurs normally in EBV-infected cells.

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Functional Analyses of a Putative, Membrane-Bound, Peroxisomal Protein Import Mechanism from the Apicomplexan Protozoan Toxoplasma gondii

Genes ◽

10.3390/genes9090434 ◽

2018 ◽

Vol 9 (9) ◽

pp. 434

Author(s):

Alison Mbekeani ◽

Will Stanley ◽

Vishal Kalel ◽

Noa Dahan ◽

Einat Zalckvar ◽

...

Keyword(s):

Toxoplasma Gondii ◽

Protein Import ◽

Fluorescent Protein ◽

Metabolic Energy ◽

Peroxisomal Protein ◽

Genes Encoding ◽

Peroxisomal Targeting ◽

Membrane Bound ◽

Green Fluorescent

Peroxisomes are central to eukaryotic metabolism, including the oxidation of fatty acids—which subsequently provide an important source of metabolic energy—and in the biosynthesis of cholesterol and plasmalogens. However, the presence and nature of peroxisomes in the parasitic apicomplexan protozoa remains controversial. A survey of the available genomes revealed that genes encoding peroxisome biogenesis factors, so-called peroxins (Pex), are only present in a subset of these parasites, the coccidia. The basic principle of peroxisomal protein import is evolutionarily conserved, proteins harbouring a peroxisomal-targeting signal 1 (PTS1) interact in the cytosol with the shuttling receptor Pex5 and are then imported into the peroxisome via the membrane-bound protein complex formed by Pex13 and Pex14. Surprisingly, whilst Pex5 is clearly identifiable, Pex13 and, perhaps, Pex14 are apparently absent from the coccidian genomes. To investigate the functionality of the PTS1 import mechanism in these parasites, expression of Pex5 from the model coccidian Toxoplasma gondii was shown to rescue the import defect of Pex5-deleted Saccharomyces cerevisiae. In support of these data, green fluorescent protein (GFP) bearing the enhanced (e)PTS1 known to efficiently localise to peroxisomes in yeast, localised to peroxisome-like bodies when expressed in Toxoplasma. Furthermore, the PTS1-binding domain of Pex5 and a PTS1 ligand from the putatively peroxisome-localised Toxoplasma sterol carrier protein (SCP2) were shown to interact in vitro. Taken together, these data demonstrate that the Pex5–PTS1 interaction is functional in the coccidia and indicate that a nonconventional peroxisomal import mechanism may operate in the absence of Pex13 and Pex14.

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Oligomerization of green fluorescent protein in the secretory pathway of endocrine cells

Biochemical Journal ◽

10.1042/bj3600645 ◽

2001 ◽

Vol 360 (3) ◽

pp. 645-649 ◽

Cited By ~ 43

Author(s):

Renu K. JAIN ◽

Paul B. M. JOYCE ◽

Miguel MOLINETE ◽

Philippe A. HALBAN ◽

Sven-Ulrik GORR

Keyword(s):

Green Fluorescent Protein ◽

Endocrine Cells ◽

Secretory Pathway ◽

Fluorescent Protein ◽

Secretory Granules ◽

Site Directed Mutagenesis ◽

Cysteine Residues ◽

Reporter Protein ◽

Regulated Secretory Pathway ◽

Green Fluorescent

Green fluorescent protein (GFP) is used extensively as a reporter protein to monitor cellular processes, including intracellular protein trafficking and secretion. In general, this approach depends on GFP acting as a passive reporter protein. However, it was recently noted that GFP oligomerizes in the secretory pathway of endocrine cells. To characterize this oligomerization and its potential role in GFP transport, cytosolic and secretory forms of enhanced GFP (EGFP) were expressed in GH4C1 and AtT-20 endocrine cells. Biochemical analysis showed that cytosolic EGFP existed as a 27kDa monomer, whereas secretory forms of EGFP formed disulphide-linked oligomers. EGFP contains two cysteine residues (Cys49 and Cys71), which could play a role in this oligomerization. Site-directed mutagenesis of Cys49 and Cys71 showed that both cysteine residues were involved in disulphide interactions. Substitution of either cysteine residue resulted in a reduction or loss of oligomers, although dimers of the secretory form of EGFP remained. Mutation of these residues did not adversely affect the fluorescence of EGFP. EGFP oligomers were stored in secretory granules and secreted by the regulated secretory pathway in endocrine AtT-20 cells. Similarly, the dimeric mutant forms of EGFP were still secreted via the regulated secretory pathway, indicating that the higher-order oligomers were not necessary for sorting in AtT-20 cells. These results suggest that the oligomerization of EGFP must be considered when the protein is used as a reporter molecule in the secretory pathway.

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Analysis of Proteasome-Dependent Proteolysis in Haloferax volcanii Cells, Using Short-Lived Green Fluorescent Proteins

Applied and Environmental Microbiology ◽

10.1128/aem.70.12.7530-7538.2004 ◽

2004 ◽

Vol 70 (12) ◽

pp. 7530-7538 ◽

Cited By ~ 55

Author(s):

Christopher J. Reuter ◽

Julie A. Maupin-Furlow

Keyword(s):

Fluorescent Protein ◽

Fluorescent Proteins ◽

Specific Inhibitor ◽

Haloferax Volcanii ◽

Reporter System ◽

Reporter Protein ◽

Protein Variant ◽

Fluorescent Reporter ◽

New Genes ◽

Green Fluorescent

ABSTRACT Proteasomes are energy-dependent proteases that are central to the quality control and regulated turnover of proteins in eukaryotic cells. Dissection of this proteolytic pathway in archaea, however, has been hampered by the lack of substrates that are easily detected in whole cells. In the present study, we developed a convenient reporter system by functional expression of a green fluorescent protein variant with C-terminal fusions in the haloarchaeon Haloferax volcanii. The levels of this reporter protein correlated with whole-cell fluorescence that was readily detected in culture. Accumulation of the reporter protein was dependent on the sequence of the C-terminal amino acid fusion, as well as the presence of an irreversible, proteasome-specific inhibitor (clasto-lactacystin β-lactone). This inhibitor was highly specific for H. volcanii 20S proteasomes, with a Ki of ∼40 nM. In contrast, phenylmethanesulfonyl fluoride did not influence the levels of fluorescent reporter protein or inhibit 20S proteasomes. Together, these findings provide a powerful tool for the elucidation of protein substrate recognition motifs and the identification of new genes which may be involved in the proteasome pathway of archaea.

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Characterization of a novel peroxisome membrane protein essential for conversion of isopenicillin N into cephalosporin C

Biochemical Journal ◽

10.1042/bj20100827 ◽

2010 ◽

Vol 432 (2) ◽

pp. 227-236 ◽

Cited By ~ 24

Author(s):

Ricardo V. Ullán ◽

Fernando Teijeira ◽

Susana M. Guerra ◽

Inmaculada Vaca ◽

Juan F. Martín

Keyword(s):

Membrane Protein ◽

Fluorescent Protein ◽

Transmembrane Protein ◽

Regulatory Gene ◽

Protein A ◽

Gene Replacement ◽

Cephalosporin C ◽

Peroxisomal Membrane ◽

Green Fluorescent ◽

Isopenicillin N

The mechanisms of compartmentalization of intermediates and secretion of penicillins and cephalosporins in β-lactam antibiotic-producing fungi are of great interest. In Acremonium chrysogenum, there is a compartmentalization of the central steps of the CPC (cephalosporin C) biosynthetic pathway. In the present study, we found in the ‘early’ CPC cluster a new gene named cefP encoding a putative transmembrane protein containing 11 transmembrane spanner. Targeted inactivation of cefP by gene replacement showed that it is essential for CPC biosynthesis. The disrupted mutant is unable to synthesize cephalosporins and secretes a significant amount of IPN (isopenicillin N), indicating that the mutant is blocked in the conversion of IPN into PenN (penicillin N). The production of cephalosporin in the disrupted mutant was restored by transformation with both cefP and cefR (a regulatory gene located upstream of cefP), but not with cefP alone. Fluorescence microscopy studies with an EGFP (enhanced green fluorescent protein)–SKL (Ser-Lys-Leu) protein (a peroxisomal-targeted marker) as a control showed that the red-fluorescence-labelled CefP protein co-localized in the peroxisomes with the control peroxisomal protein. In summary, CefP is a peroxisomal membrane protein probably involved in the import of IPN into the peroxisomes where it is converted into PenN by the two-component CefD1/CefD2 protein system.

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