Your search keyword '"Pancreatitis-Associated Proteins"' showing total 25 results

1. Lipopolysaccharide-induced cyclooxygenase-2 expression in human U937 macrophages is phosphatidic acid phosphohydrolase-1-dependent.

Author

Grkovich, Andrej, Johnson, Christina A, Buczynski, Matthew W, and Dennis, Edward A

Subjects

U937 Cells, Macrophages, Animals, Humans, Mice, Propranolol, Ethanol, Butanols, Pyrones, Naphthalenes, Phosphatidate Phosphatase, Lipopolysaccharides, Dinoprostone, Diglycerides, RNA, Messenger, Gene Expression Regulation, Enzymologic, Up-Regulation, Cytoprotection, Time Factors, Cyclooxygenase 2, Pancreatitis-Associated Proteins, RNA, Messenger, Gene Expression Regulation, Enzymologic, Chemical Sciences, Biological Sciences, Medical and Health Sciences, Biochemistry & Molecular Biology

Abstract

Cyclooxygenase (COX) has two isoforms, COX-1 and -2, which catalyze the key step in the conversion of cellular arachidonic acid into prostaglandins. In recent years, interest in COX-2 has significantly increased since it has been a target for the development of specific non-steroidal anti-inflammatory drugs. We report that COX-2 expression is up-regulated in phorbol ester (phorbol myristate acetate, PMA)-differentiated human U937 macrophage-like cells stimulated with lipopolysaccharide (LPS), whereas COX-1 is not up-regulated. We show that the LPS-induced up-regulation of COX-2 depends on the activity of the Mg(+2)-dependent phosphatidic acid phosphohydrolase 1 (PAP-1). Inhibition of PAP-1 by bromoenol lactone, propranolol, or ethanol resulted in a decrease in LPS-induced COX-2 mRNA transcript production, COX-2 protein expression, and prostaglandin E(2) release from U937 macrophages. To ensure that these results did not arise because of PMA treatment of the U937 cells, similar experiments were conducted with the P388D(1) cell line, which does not require PMA differentiation. LPS increased the levels of endogenous cellular diacylglycerol (DAG) within 2 min of stimulation. This increase was observed to be sensitive to the PAP-1 inhibitors. Furthermore, phosphatidic acid phosphohydrolase activity assays showed that the bromoenol lactone-sensitive PAP-1 activity was translocated from the cytosolic fraction to the membrane fraction within 2 min of LPS exposure. Finally, DAG add-back experiments demonstrate that LPS-induced COX-2 expression is enhanced by the addition of exogenous DAG.

Published

2006

2. Regulation of cyclooxygenase-2 expression by phosphatidate phosphohydrolase in human amnionic WISH cells.

Author

Johnson, CA, Balboa, MA, Balsinde, J, and Dennis, EA

Subjects

Amnion, Cell Line, Humans, Propranolol, Ethanol, Sulfonamides, Nitrobenzenes, Tetradecanoylphorbol Acetate, Pyrones, Naphthalenes, Phosphatidate Phosphatase, Isoenzymes, Arachidonic Acid, Dinoprostone, Membrane Proteins, Cyclooxygenase Inhibitors, Phosphodiesterase Inhibitors, Transcription, Genetic, Gene Expression Regulation, Enzymologic, Kinetics, Prostaglandin-Endoperoxide Synthases, Cyclooxygenase 2, Cyclooxygenase 2 Inhibitors, Pancreatitis-Associated Proteins, Transcription, Genetic, Gene Expression Regulation, Enzymologic, Chemical Sciences, Biological Sciences, Medical and Health Sciences, Biochemistry & Molecular Biology

Abstract

Prostaglandins are known to play a key role in the initiation of labor in humans, but the mechanisms governing their synthesis in amnion are largely unknown. In this study, we have examined the regulatory pathways for prostaglandin E(2) (PGE(2)) production during protein kinase C-dependent activation of human WISH cells. In these cells, PGE(2) synthesis appears to be limited not by free arachidonic acid availability but by the expression levels of cyclooxygenase-2 (COX-2). Concomitant with the cells being able to synthesize and secrete PGE(2), we detected significant elevations of both COX-2 protein and mRNA levels. Specific inhibition of COX-2 by NS-398 totally ablated PGE(2) synthesis. All of these responses were found to be strikingly dependent on an active phosphatidate phosphohydrolase 1 (PAP-1). Inhibition of PAP-1 activity by three different strategies (i.e. use of bromoenol lactone, propranolol, and ethanol) resulted in inhibition of COX-2 expression and hence of PGE(2) production. These data unveil a novel signaling mechanism for the regulation of PGE(2) production via regulation of COX-2 expression and implicate phosphatidate phosphohydrolase 1 as a key regulatory component of eicosanoid metabolic pathways in the amnion.

Published

1999

3. Regulation of C-type Lectin Antimicrobial Activity by a Flexible N-terminal Prosegment*S⃞

Author

Rebecca E. Lehotzky, Sohini Mukherjee, Carrie L. Partch, Charles L. Bevins, Cecilia V. Whitham, Kevin H. Gardner, Lora V. Hooper, and Hiutung Chu

Subjects

Pancreatitis-Associated Proteins, medicine.disease_cause, Biochemistry, Protein Structure, Secondary, Mice, C-type lectin, Antigens, Neoplasm, medicine, Biomarkers, Tumor, Animals, Homeostasis, Humans, Lectins, C-Type, Intestinal Mucosa, Molecular Biology, Nuclear Magnetic Resonance, Biomolecular, Mice, Knockout, Mutation, Innate immune system, biology, Protein Synthesis, Post-Translational Modification, and Degradation, Lectin, Proteins, Biological activity, Cell Biology, Trypsin, Immunity, Innate, Anti-Bacterial Agents, Protein Structure, Tertiary, Intestines, biology.protein, Antibacterial activity, medicine.drug

Abstract

Members of the RegIII family of intestinal C-type lectins are directly antibacterial proteins that play a vital role in maintaining host-bacterial homeostasis in the mammalian gut, yet little is known about the mechanisms that regulate their biological activity. Here we show that the antibacterial activities of mouse RegIIIgamma and its human ortholog, HIP/PAP, are tightly controlled by an inhibitory N-terminal prosegment that is removed by trypsin in vivo. NMR spectroscopy revealed a high degree of conformational flexibility in the HIP/PAP inhibitory prosegment, and mutation of either acidic prosegment residues or basic core protein residues disrupted prosegment inhibitory activity. NMR analyses of pro-HIP/PAP variants revealed distinctive colinear backbone amide chemical shift changes that correlated with antibacterial activity, suggesting that prosegment-HIP/PAP interactions are linked to a two-state conformational switch between biologically active and inactive protein states. These findings reveal a novel regulatory mechanism governing C-type lectin biological function and yield new insight into the control of intestinal innate immunity.

Published

2009

4. N-terminal cleaved pancreatitis-associated protein-III (PAP-III) serves as a scaffold for neurites and promotes neurite outgrowth

Author

Hiroyuki Konishi, Hiroshi Kiyama, Kazuhiko Namikawa, and Sakiko Matsumoto

Subjects

Male, Neurite, Proteolysis, medicine.medical_treatment, Nerve Tissue Proteins, Pancreatitis-Associated Proteins, Biology, Biochemistry, Protein filament, Neurobiology, Antigens, Neoplasm, medicine, Biomarkers, Tumor, Neurites, Animals, Lectins, C-Type, Rats, Wistar, Molecular Biology, Cells, Cultured, Protease, medicine.diagnostic_test, Sodium, Cell Biology, Anatomy, Nerve injury, Sciatic Nerve, In vitro, female genital diseases and pregnancy complications, Axons, Cell biology, Nerve Regeneration, Rats, Secretory protein, medicine.symptom, Axotomy

Abstract

Pancreatitis-associated protein (PAP)-III, also known as regenerating gene/regenerating islet-derived (Reg)-IIIγ, is a small secretory protein whose expression is substantially induced in injured nerves. Here, we found that PAP-III protein underwent proteolytic N-terminal processing by trypsin-like protease(s) in injured sciatic nerves after axotomy. In vitro studies demonstrated that the N terminus-truncated PAP-III (ΔN-PAP-III) polymerized into a filament with a relatively uniform diameter of 10-20 nm, and the filaments formed higher order structures in a Na(+) concentration-dependent manner. When the ΔN-PAP-III fibers were added to the culture media, the ΔN-PAP-III fibers were tightly attached to neurites and somata of primary cortical neurons in vitro. In contrast, little association with glial cells was observed. When dense matrices of ΔN-PAP-III fibers were sheeted on a culture dish, neurites preferentially adhered to the fibers, and neurite extension was enhanced. This neurite outgrowth activity was significantly suppressed by preincubation with antibodies against PAP-III. These results imply that the released PAP-III might be cleaved and forms ΔN-PAP-III fibers at the nerve injury sites. Consequently, these resulting fibers would provide regenerating axons with a platform for extension.

Published

2013

5. REF4 and RFR1, subunits of the transcriptional coregulatory complex mediator, are required for phenylpropanoid homeostasis in Arabidopsis

Author

Whitney L. Soltau, Jake Stout, Brendan L. Powers, Jing-Ke Weng, Michael R. Blatchley, Leslie A. Seals, Clint Chapple, Nicholas D. Bonawitz, and Anna K. Hurlock

Subjects

core promoters, Transcription, Genetic, Mutant, Arabidopsis, Plant Biology, RNA polymerase II, Pancreatitis-Associated Proteins, human health, Biochemistry, biosynthetic gene, Transcription (biology), Gene Expression Regulation, Plant, Homeostasis, Organic Chemicals, Phylogeny, Regulation of gene expression, Genetics, Phenylpropanoid, biology, food and beverages, Cell biology, Phenotype, anthocyanin accumulation, wild types, mediator complex, phenylpropanoids, mutant proteins, Mediator, metabolic pathways, phenylpropanoid pathways, RNA, Messenger, paralogs, Molecular Biology, Transcription factor, Cis-acting DNA, Arabidopsis thaliana mutant, Sequence Homology, Amino Acid, Arabidopsis Proteins, eukaryotic gene regulation, Membrane Proteins, Cell Biology, human needs, biology.organism_classification, binding partners, rational manipulation, Protein Subunits, Mutation, biology.protein

Abstract

The plant phenylpropanoid pathway produces an array of metabolites that impact human health and the utility of feed and fiber crops. We previously characterized several Arabidopsis thaliana mutants with dominant mutations in REDUCED EPIDERMAL FLUORESCENCE 4 (REF4) that cause dwarfing and decreased accumulation of phenylpropanoids. In contrast, ref4 null plants are of normal stature and have no apparent defect in phenylpropanoid biosynthesis. Here we show that disruption of both REF4 and its paralog, REF4-RELATED 1 (RFR1), results in enhanced expression of multiple phenylpropanoid biosynthetic genes, as well as increased accumulation of numerous downstream products. We also show that the dominant ref4-3 mutant protein interferes with the ability of the PAP1/MYB75 transcription factor to induce the expression of PAL1 and drive anthocyanin accumulation. Consistent with our experimental results, both REF4 and RFR1 have been shown to physically associate with the conserved transcriptional coregulatory complex, Mediator, which transduces information from cis-acting DNA elements to RNA polymerase II at the core promoter. Taken together, our data provide critical genetic support for a functional role of REF4 and RFR1 in the Mediator complex, and for Mediator in the maintenance of phenylpropanoid homeostasis. Finally, we show that wild-type RFR1 substantially mitigates the phenotype of the dominant ref4-3 mutant, suggesting that REF4 and RFR1 may compete with one another for common binding partners or for occupancy in Mediator. Determining the functions of diverse Mediator subunits is essential to understand eukaryotic gene regulation, and to facilitate rational manipulation of plant metabolic pathways to better suit human needs.

Published

2011

6. Evidence for a complex of transcription factor IIB with poly(A) polymerase and cleavage factor 1 subunits required for gene looping

Author

Scott Medler, Sarita Raghunayakula, Athar Ansari, Banupriya Mukundan, Ashley Aldea, and Nadra Al Husini

Subjects

Saccharomyces cerevisiae Proteins, Genes, Fungal, RNA polymerase II, Pancreatitis-Associated Proteins, Saccharomyces cerevisiae, Biology, Biochemistry, Chromatography, Affinity, Transcription (biology), Transcriptional regulation, Gene Regulation, DNA, Fungal, Molecular Biology, Transcription factor, 3' Untranslated Regions, mRNA Cleavage and Polyadenylation Factors, Polynucleotide Adenylyltransferase, Cell Biology, enzymes and coenzymes (carbohydrates), Multiprotein Complexes, Transcription preinitiation complex, Mutation, Transcription factor II H, biology.protein, Transcription Factor TFIIB, Myo-Inositol-1-Phosphate Synthase, RNA Polymerase II, Oxidoreductases, Transcription factor II B, Transcription factor II A

Abstract

Gene looping, defined as the interaction of the promoter and the terminator regions of a gene during transcription, requires transcription factor IIB (TFIIB). We have earlier demonstrated association of TFIIB with the distal ends of a gene in an activator-dependent manner (El Kaderi, B., Medler, S., Raghunayakula, S., and Ansari, A. (2009) J. Biol. Chem. 284, 25015–25025). The presence of TFIIB at the 3′ end of a gene required its interaction with cleavage factor 1 (CF1) 3′ end processing complex subunit Rna15. Here, employing affinity chromatography and glycerol gradient centrifugation, we show that TFIIB associates with poly(A) polymerase and the entire CF1 complex in yeast cells. The factors required for general transcription such as TATA-binding protein, RNA polymerase II, and TFIIH are not a component of the TFIIB complex. This holo-TFIIB complex was resistant to MNase digestion. The complex was observed only in the looping-competent strains, but not in the looping-defective sua7-1 strain. The requirement of Rna15 in gene looping has been demonstrated earlier. Here we provide evidence that poly(A) polymerase (Pap1) as well as CF1 subunits Rna14 and Pcf11 are also required for loop formation of MET16 and INO1 genes. Accordingly, cross-linking of TFIIB to the 3′ end of genes was abolished in the mutants of Pap1, Rna14, and Pcf11. We further show that in sua7-1 cells, where holo-TFIIB complex is not formed, the kinetics of activated transcription is altered. These results suggest that a complex of TFIIB, CF1 subunits, and Pap1 exists in yeast cells. Furthermore, TFIIB interaction with the CF1 complex and Pap1 is crucial for gene looping and transcriptional regulation.

Published

2011

7. Functions of Manduca sexta hemolymph proteinases HP6 and HP8 in two innate immune pathways

Author

Jun Ishibashi, Michael R. Kanost, Chunju An, Haobo Jiang, and Emily J. Ragan

Subjects

animal structures, Antimicrobial peptides, Immunoblotting, Gene Expression, Pancreatitis-Associated Proteins, Biochemistry, Models, Biological, Serine, Hemolymph, Manduca, Escherichia coli, Animals, Molecular Biology, Phylogeny, Enzyme Precursors, Innate immune system, Binding Sites, biology, Enzyme Catalysis and Regulation, Reverse Transcriptase Polymerase Chain Reaction, fungi, Serine Endopeptidases, Cell Biology, Prophenoloxidase, biology.organism_classification, Immunity, Innate, Recombinant Proteins, Isoenzymes, Cecropin, Manduca sexta, Larva, Host-Pathogen Interactions, Mutation, Insect Proteins, Catechol Oxidase, Antimicrobial Cationic Peptides, Signal Transduction

Abstract

Serine proteinases in insect plasma have been implicated in two types of immune responses; that is, activation of prophenoloxidase (proPO) and activation of cytokine-like proteins. We have identified more than 20 serine proteinases in hemolymph of the tobacco hornworm, Manduca sexta, but functions are known for only a few of them. We report here functions of two additional M. sexta proteinases, hemolymph proteinases 6 and 8 (HP6 and HP8). HP6 and HP8 are each composed of an amino-terminal clip domain and a carboxyl-terminal proteinase domain. HP6 is an apparent ortholog of Drosophila Persephone, whereas HP8 is most similar to Drosophila and Tenebrio spatzle-activating enzymes, all of which activate the Toll pathway. proHP6 and proHP8 are expressed constitutively in fat body and hemocytes and secreted into plasma, where they are activated by proteolytic cleavage in response to infection. To investigate activation and biological activity of HP6 and HP8, we purified recombinant proHP8, proHP6, and mutants of proHP6 in which the catalytic serine was replaced with alanine, and/or the activation site was changed to permit activation by bovine factor Xa. HP6 was found to activate proPO-activating proteinase (proPAP1) in vitro and induce proPO activation in plasma. HP6 was also determined to activate proHP8. Active HP6 or HP8 injected into larvae induced expression of antimicrobial peptides and proteins, including attacin, cecropin, gloverin, moricin, and lysozyme. Our results suggest that proHP6 becomes activated in response to microbial infection and participates in two immune pathways; activation of PAP1, which leads to proPO activation and melanin synthesis, and activation of HP8, which stimulates a Toll-like pathway.

Published

2009

8. Three mammalian lipins act as phosphatidate phosphatases with distinct tissue expression patterns

Author

Meltem Sariahmetoglu, Jay Dewald, David N. Brindley, Karen Reue, and Jimmy Donkor

Subjects

Protein family, Adipose Tissue, White, Phosphatase, Phosphatidate Phosphatase, Adipose tissue, Pancreatitis-Associated Proteins, Biology, Biochemistry, Cell Line, Phosphatidate, Mice, Adipose Tissue, Brown, Brown adipose tissue, medicine, Animals, Humans, Muscle, Skeletal, Molecular Biology, Mice, Inbred BALB C, Skeletal muscle, Nuclear Proteins, Proteins, Cell Biology, Phosphatidate phosphatase, medicine.disease, Mice, Mutant Strains, Fatty Liver, Mice, Inbred C57BL, medicine.anatomical_structure, Lipodystrophy, Glycolipids

Abstract

We previously identified mutations in the Lpin1 gene, encoding lipin-1, as the underlying cause of lipodystrophy in the fatty liver dystrophy (fld) mutant mouse. Lipin-1 is normally expressed at high levels in adipose tissue and skeletal muscle, and deficiency in the fld mouse causes impaired adipose tissue development, insulin resistance, and altered energy expenditure. We also identified two additional lipin protein family members of unknown function, lipin-2 and lipin-3. Han et al. (Han, G. S., Wu, W. I., and Carman, G. M. (2006) J. Biol. Chem. 281, 9210-9218) recently demonstrated that the single lipin homolog in yeast, Smp2, exhibits phosphatidate phosphatase type-1 (PAP1) activity, which has a key role in glycerolipid synthesis. Here we demonstrate that lipin-1 accounts for all of the PAP1 activity in white and brown adipose tissue and skeletal muscle. However, livers of lipin-1-deficient mice exhibited normal PAP1 activity, indicating that other members of the lipin protein family could have PAP1 activity. Consistent with this possibility, recombinant lipin-2 and lipin-3 possess PAP1 activity. Each of the three lipin family members showed Mg2+-dependent activity that was specific for phosphatidate under the conditions employed. The different lipins showed distinct tissue expression patterns. Our results establish the three mammalian lipin proteins as PAP1 enzymes and explain the biochemical basis for lipodystrophy in the lipin-1-deficient fld mouse.

Published

2006

9. Lipopolysaccharide-induced cyclooxygenase-2 expression in human U937 macrophages is phosphatidic acid phosphohydrolase-1-dependent

Author

Andrej Grkovich, Christina A. Johnson, Edward A. Dennis, and Matthew W. Buczynski

Subjects

Enzymologic, Lipopolysaccharides, Time Factors, Lipopolysaccharide, Butanols, Messenger, Endogeny, Pancreatitis-Associated Proteins, Biochemistry, Medical and Health Sciences, chemistry.chemical_compound, Mice, 2.1 Biological and endogenous factors, Prostaglandin E2, Aetiology, biology, U937 cell, U937 Cells, Biological Sciences, Propranolol, Up-Regulation, Arachidonic acid, lipids (amino acids, peptides, and proteins), medicine.drug, Biochemistry & Molecular Biology, Phosphatidate Phosphatase, Naphthalenes, Dinoprostone, Gene Expression Regulation, Enzymologic, Diglycerides, medicine, Animals, Humans, RNA, Messenger, Molecular Biology, Diacylglycerol kinase, Ethanol, Macrophages, Cell Biology, chemistry, Gene Expression Regulation, Cell culture, Cyclooxygenase 2, Cytoprotection, Pyrones, Chemical Sciences, biology.protein, RNA, Cyclooxygenase

Abstract

Cyclooxygenase (COX) has two isoforms, COX-1 and -2, which catalyze the key step in the conversion of cellular arachidonic acid into prostaglandins. In recent years, interest in COX-2 has significantly increased since it has been a target for the development of specific non-steroidal anti-inflammatory drugs. We report that COX-2 expression is up-regulated in phorbol ester (phorbol myristate acetate, PMA)-differentiated human U937 macrophage-like cells stimulated with lipopolysaccharide (LPS), whereas COX-1 is not up-regulated. We show that the LPS-induced up-regulation of COX-2 depends on the activity of the Mg(+2)-dependent phosphatidic acid phosphohydrolase 1 (PAP-1). Inhibition of PAP-1 by bromoenol lactone, propranolol, or ethanol resulted in a decrease in LPS-induced COX-2 mRNA transcript production, COX-2 protein expression, and prostaglandin E(2) release from U937 macrophages. To ensure that these results did not arise because of PMA treatment of the U937 cells, similar experiments were conducted with the P388D(1) cell line, which does not require PMA differentiation. LPS increased the levels of endogenous cellular diacylglycerol (DAG) within 2 min of stimulation. This increase was observed to be sensitive to the PAP-1 inhibitors. Furthermore, phosphatidic acid phosphohydrolase activity assays showed that the bromoenol lactone-sensitive PAP-1 activity was translocated from the cytosolic fraction to the membrane fraction within 2 min of LPS exposure. Finally, DAG add-back experiments demonstrate that LPS-induced COX-2 expression is enhanced by the addition of exogenous DAG.

Published

2006

10. Genetic requirements for growth of Escherichia coli K12 on methyl-alpha-D-glucopyranoside and the five alpha-D-glucosyl-D-fructose isomers of sucrose

Author

Bernhard Erni, John F. Thompson, Sonja Hess, Andreas Pikis, and Ingrid Arnold

Subjects

Sucrose, Molecular Sequence Data, Pancreatitis-Associated Proteins, Fructose, Biology, medicine.disease_cause, Biochemistry, Turanose, Substrate Specificity, Phosphotransferase, chemistry.chemical_compound, Transformation, Genetic, Isomerism, medicine, Amino Acid Sequence, Phosphoenolpyruvate Sugar Phosphotransferase System, Molecular Biology, Escherichia coli, Escherichia coli K12, Escherichia coli Proteins, Genetic Complementation Test, Methylglucosides, Glucose analog, alpha-Glucosidases, Cell Biology, PEP group translocation, Isomaltose, Complementation, Klebsiella pneumoniae, chemistry, Gene Deletion, Plasmids

Abstract

Strains of Escherichia coli K12, including MG-1655, accumulate methyl-alpha-D-glucopyranoside via the phosphoenolpyruvate-dependent glucose:phosphotransferase system (IICB(Glc)/IIA(Glc)). High concentrations of intracellular methyl-alpha-D-glucopyranoside 6-phosphate are toxic, and cell growth is prevented. However, transformation of E. coli MG-1655 with a plasmid (pAP1) encoding the gene aglB from Klebsiella pneumoniae resulted in excellent growth of the transformant MG-1655 (pAP1) on the glucose analog. AglB is an unusual NAD+/Mn2+-dependent phospho-alpha-glucosidase that promotes growth of MG-1655 (pAP1) by catalyzing the in vivo hydrolysis of methyl-alpha-D-glucopyranoside 6-phosphate to yield glucose 6-phosphate and methanol. When transformed with plasmid pAP2 encoding the K. pneumoniae genes aglB and aglA (an alpha-glucoside-specific transporter AglA (IICB(Agl))), strain MG-1655 (pAP2) metabolized a variety of other alpha-linked glucosides, including maltitol, isomaltose, and the following five isomers of sucrose: trehalulose alpha(1-->1), turanose alpha(1-->3), maltulose alpha(1-->4), leucrose alpha(1-->5), and palatinose alpha(1-->6). Remarkably, MG-1655 (pAP2) failed to metabolize sucrose alpha(1-->2). The E. coli K12 strain ZSC112L (ptsG::cat manXYZ nagE glk lac) can neither grow on glucose nor transport methyl-alpha-D-glucopyranoside. However, when transformed with pTSGH11 (encoding ptsG) or pAP2, this organism provided membranes that contained either the PtsG or AglA transporters, respectively. In vitro complementation of transporter-specific membranes with purified general phosphotransferase components showed that although PtsG and AglA recognized glucose and methyl-alpha-D-glucopyranoside, only AglA accepted other alpha-D-glucosides as substrates. Complementation experiments also revealed that IIA(Glc) was required for functional activity of both PtsG and AglA transporters. We conclude that AglA, AglB, and IIA(Glc) are necessary and sufficient for growth of E. coli K12 on methyl-alpha-D-glucoside and related alpha-D-glucopyranosides.

Published

2006

11. Methylglyoxal as a signal initiator for activation of the stress-activated protein kinase cascade in the fission yeast Schizosaccharomyces pombe

Author

Yoshiharu Inoue, Yoshifumi Takatsume, and Shingo Izawa

Subjects

Cell Cycle Proteins, Pancreatitis-Associated Proteins, Biochemistry, Fungal Proteins, Schizosaccharomyces, Phosphorylation, Protein kinase A, Molecular Biology, Cell Nucleus, biology, Kinase, Cell Biology, Hydrogen Peroxide, biology.organism_classification, Oxidants, Pyruvaldehyde, Response regulator, Basic-Leucine Zipper Transcription Factors, Schizosaccharomyces pombe, Cyclin-dependent kinase complex, Schizosaccharomyces pombe Proteins, Cyclin-dependent kinase 7, Signal Transduction

Abstract

Methylglyoxal (MG) is a typical 2-oxoaldehyde derived from glycolysis. We have recently found that MG activates transcription factors such as Yap1 and Msn2, and triggers a Hog1 mitogen-activated protein kinase cascade in Saccharomyces cerevisiae. Regarding the activation of Hog1 by MG, we found that Sln1, an osmosensor possessing histidine kinase activity, functions as a sensor of MG (Maeta, K., Izawa, S., and Inoue, Y. (2005) J. Biol. Chem. 280, 253-260). To gain further insight into the role of MG as a signal initiator, here we analyze the response of Schizosaccharomyces pombe to extracellular MG. Spc1, a stress-activated protein kinase (SAPK), was phosphorylated following the treatment with MG. No phosphorylation was observed in a wis1Delta mutant. The His-to-Asp phosphorelay system consisting of three histidine kinases (Phk1, Phk2, and Phk3), a phosphorelay protein (Spy1), and a response regulator (Mcs4) exists upstream of the Spc1-SAPK pathway. The phosphorylation of Spc1 following MG treatment was observed in phk1Deltaphk2Deltaphk3Delta and spy1Delta cells, but not in mcs4Delta cells. These results suggest that S. pombe has an alternative module(s) that directs the MG signal to the SAPK pathway via Mcs4. Additionally, we found that the transcription factor Pap1 is concentrated in the nucleus in response to MG, independent of the Spc1-SAPK pathway.

Published

2006

12. Oxidation of a eukaryotic 2-Cys peroxiredoxin is a molecular switch controlling the transcriptional response to increasing levels of hydrogen peroxide

Author

Jannine Cameron, Brian A. Morgan, Stephanie M. Bozonet, Victoria J. Findlay, Elizabeth A. Veal, and Alison M. Day

Subjects

Time Factors, Transcription, Genetic, Pancreatitis-Associated Proteins, Biochemistry, Peroxide, chemistry.chemical_compound, Gene Expression Regulation, Fungal, Oxidoreductases Acting on Sulfur Group Donors, Hydrogen peroxide, Fluorescent Antibody Technique, Indirect, Cell biology, Peroxides, DNA-Binding Proteins, Basic-Leucine Zipper Transcription Factors, Peroxidases, RNA, Viral, Electrophoresis, Polyacrylamide Gel, Thioredoxin, Mitogen-Activated Protein Kinases, Oxidoreductases, Oxidation-Reduction, Saccharomyces cerevisiae Proteins, Blotting, Western, Molecular Sequence Data, Active Transport, Cell Nucleus, Oxidative phosphorylation, Biology, Models, Biological, Catalysis, Fungal Proteins, Enzyme activator, Schizosaccharomyces, Immunoprecipitation, Amino Acid Sequence, Cysteine, Molecular Biology, Thioredoxin peroxidase activity, Cell Nucleus, Dose-Response Relationship, Drug, Cell Biology, Hydrogen Peroxide, Peroxiredoxins, Enzyme Activation, Oxygen, Sulfiredoxin, Oxidative Stress, chemistry, Schizosaccharomyces pombe Proteins, Peroxiredoxin

Abstract

Although activation of the AP-1-like transcription factor Pap1 in Schizosaccharomyces pombe is important for oxidative stress-induced gene expression, this activation is delayed at higher concentrations of peroxide. Here, we reveal that the 2-Cys peroxiredoxin (2-Cys Prx) Tpx1 is required for the peroxide-induced activation of Pap1. Tpx1, like other eukaryotic 2-Cys Prxs, is highly sensitive to oxidation, which inactivates its thioredoxin peroxidase activity. Our data suggest that the reduced thioredoxin peroxidase-active form of Tpx1 is required for the peroxide-induced oxidation and nuclear accumulation of Pap1. Indeed, in contrast to the previously described role for Tpx1 in the activation of the Sty1 stress-activated protein kinase by peroxide, we find that both catalytic cysteines of Tpx1 are required for Pap1 activation. Moreover, overexpression of the conserved sulfiredoxin Srx1, which interacts with and reduces Tpx1, allows rapid activation of Pap1 at higher concentrations of H(2)O(2). Conversely, loss of Srx1 prevents the reduction of oxidized Tpx1 and prolongs the inhibition of Pap1 activation. Collectively, these data suggest that redox regulation of the thioredoxin peroxidase activity of Tpx1 acts as a molecular switch controlling the transcriptional response to H(2)O(2). Furthermore, they reveal that a single eukaryotic 2-Cys Prx regulates peroxide signaling by multiple independent mechanisms.

Published

2005

13. Bromoenol lactone promotes cell death by a mechanism involving phosphatidate phosphohydrolase-1 rather than calcium-independent phospholipase A2

Author

Jesús Balsinde, Lucía Fuentes, Rebeca Pérez, María A. Balboa, and Maria de la O. Nieto

Subjects

T-Lymphocytes, Apoptosis, Pancreatitis-Associated Proteins, Biochemistry, Jurkat cells, Choline, Membrane Potentials, Phosphatidate, chemistry.chemical_compound, Mice, Magnesium, Annexin A5, Enzyme Inhibitors, Phospholipids, Enzyme Precursors, Phagocytes, Arachidonic Acid, Caspase 3, Propranolol, Caspase 9, Mitochondria, Caspases, Pituitary Gland, Poly(ADP-ribose) Polymerases, Programmed cell death, Phosphatidate Phosphatase, Biology, Naphthalenes, Phospholipases A, Cell Line, Phospholipase A2, Animals, Humans, Propidium iodide, DAPI, Molecular Biology, Triglycerides, Cell Nucleus, Macrophages, Cell Membrane, Cell Biology, Molecular biology, Phospholipases A2, chemistry, Cell culture, Pyrones, biology.protein, Calcium, DNA Damage

Abstract

Originally described as a serine protease inhibitor, bromoenol lactone (BEL) has recently been found to potently inhibit Group VI calcium-independent phospholipase A2 (iPLA2). Thus, BEL is widely used to define biological roles of iPLA2 in cells. However, BEL is also known to inhibit another key enzyme of phospholipid metabolism, namely the magnesium-dependent phosphatidate phosphohydrolase-1 (PAP-1). In this work we report that BEL is able to promote apoptosis in a variety of cell lines, including U937, THP-1, and MonoMac (human phagocyte), RAW264.7 (murine macrophage), Jurkat (human T lymphocyte), and GH3 (human pituitary). In these cells, long term treatment with BEL (up to 24 h) results in increased annexin-V binding to the cell surface and nuclear DNA damage, as detected by staining with both DAPI and propidium iodide. At earlier times (2 h), BEL induces the proteolysis of procaspase-9 and procaspase-3 and increases cleavage of poly(ADP-ribose) polymerase. These changes are preceded by variations in the mitochondrial membrane potential. All these effects of BEL are not mimicked by the iPLA2 inhibitor methylarachidonyl fluorophosphonate or by treating the cells with a specific iPLA2 antisense oligonucleotide. However, propranolol, a PAP-1 inhibitor, is able to reproduce these effects, suggesting that it is the inhibition of PAP-1 and not of iPLA2 that is involved in BEL-induced cell death. In support of this view, BEL-induced apoptosis is accompanied by a very strong inhibition of PAP-1-regulated events, such as incorporation of [3H]choline into phospholipids and de novo incorporation of [3H]arachidonic acid into triacylglycerol. Collectively, these results stress the role of PAP-1 as a key enzyme for cell integrity and survival and in turn caution against the use of BEL in studies involving long incubation times, due to the capacity of this drug to induce apoptosis in a variety of cells.

Published

2003

14. Schizosaccharomyces pombe cells lacking the Ran-binding protein Hba1 show a multidrug resistance phenotype due to constitutive nuclear accumulation of Pap1

Author

Elena Hidalgo, Ana Vivancos, Nic Jones, José Ayté, and Esther A. Castillo

Subjects

Antifungal Agents, Time Factors, Blotting, Western, Green Fluorescent Proteins, Pancreatitis-Associated Proteins, Biology, Protein Serine-Threonine Kinases, Biochemistry, Antioxidants, Fungal Proteins, chemistry.chemical_compound, Caffeine, Schizosaccharomyces, Nuclear export signal, Molecular Biology, Transcription factor, Cell Nucleus, Nucleoplasm, Brefeldin A, Microscopy, Confocal, Models, Genetic, Nuclear Proteins, Cell Biology, biology.organism_classification, Drug Resistance, Multiple, Cell biology, Protein Structure, Tertiary, DNA-Binding Proteins, Luminescent Proteins, Oxidative Stress, Basic-Leucine Zipper Transcription Factors, Phenotype, chemistry, Ran, Schizosaccharomyces pombe, RNA, Schizosaccharomyces pombe Proteins, Mitogen-Activated Protein Kinases, Nuclear localization sequence, Cell Division, Gene Deletion, Binding domain, Plasmids

Abstract

In Schizosaccharomyces pombe, the transcription factor Pap1, and the mitogen-activated protein kinase Sty1 are excluded from the nucleus in a Crm1-dependent manner under non-stressed conditions. Upon oxidant treatment, both Sty1 and Pap1 concentrate into the nucleus, due to an enhanced import or an impaired export. Hba1, a protein that when overexpressed confers brefeldin A resistance, contains a Ran binding domain. The purpose of this project was to understand at the molecular level the role of Hba1 in the S. pombe oxidative stress response. Fluorescent and confocal microscopy studies demonstrate that Hba1 is located at the nucleoplasm and not at the nuclear envelope. We also demonstrate that either multiple copies or deletion of the hba1 gene induces nuclear accumulation of Pap1 and Sty1. We propose that Hba1 assists Crm1 to export some nuclear export signal-containing proteins. Pap1 nuclear accumulation is sufficient for constitutive activation of its specific antioxidant response. On the contrary, constitutive nuclear localization of Sty1 in the Deltahba1 strain does not trigger the Sty1-specific, Atf1-dependent antioxidant response in the absence of stress. We conclude that the increased multidrug resistance of strains lacking or overexpressing Hba1 is due to the accumulation of Pap1 in the nucleus under non-stressed conditions.

Published

2003

15. Approaches to define antigen receptor-induced serine kinase signal transduction pathways

Author

Sandra Beer, Doreen A. Cantrell, Nick Totty, Denis R. Alexander, Emmanuelle Astoul, and Arian Laurence

Subjects

T-Lymphocytes, B-cell receptor, Amino Acid Motifs, Blotting, Western, Receptors, Antigen, T-Cell, Enzyme-Linked Immunosorbent Assay, Pancreatitis-Associated Proteins, Biology, Protein Serine-Threonine Kinases, Biochemistry, Binding, Competitive, Mass Spectrometry, src Homology Domains, Glycogen Synthase Kinase 3, Antigen, GSK-3, Proto-Oncogene Proteins, Serine, Humans, Phosphorylation, Pigment Epithelium of Eye, Molecular Biology, Chromatography, Binding Sites, Dose-Response Relationship, Drug, Antigen processing, T-cell receptor, Cell Biology, DNA, Protein Structure, Tertiary, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Signal transduction, Peptides, Proto-Oncogene Proteins c-akt, Proto-oncogene tyrosine-protein kinase Src, Protein Binding, Signal Transduction

Abstract

In the present report we describe the properties of a novel phospho-specific antiserum that has opened a route to the characterization of antigen receptor-activated serine kinase pathways in lymphocytes. The basis for the present work was that Ser-21 in glycogen synthase kinase 3α is robustly phosphorylated following antigen receptor triggering. We predicted accordingly that antigen receptors would also stimulate phosphorylation of other proteins with a similar sequence. To test this idea we raised an antibody against the phospho-peptide RARTSpSFAEP, where pS is a phospho-serine corresponding to the glycogen synthase kinase 3α Ser-21 sequence. The resulting antiserum was called phospho antibody for proteomics-1 (PAP-1). The present study describes the properties of PAP-1 and shows that it can reveal quite striking differences in the phospho-proteome of different cell types and is able to pinpoint new targets in important signal transduction pathways. PAP-1 was used to map protein phosphorylations regulated by the antigen receptor in T cells. One of these PAP-1-reactive proteins was purified and revealed to be a previously unrecognized target for antigen receptor signal transduction, namely an “orphan” adapter SLY (Src homology 3 (SH3) domain-containing protein expressed in lymphocytes). The use of sera detecting specific phosphorylation sites is thus proved as a powerful method for the discovery of novel downstream components of antigen receptor signals in T cells.

Published

2003

16. Prophenoloxidase-activating proteinase-2 from hemolymph of Manduca sexta. A bacteria-inducible serine proteinase containing two clip domains

Author

Haobo, Jiang, Yang, Wang, Xiao-Qiang, Yu, and Michael R, Kanost

Subjects

DNA, Complementary, Base Sequence, Molecular Sequence Data, Serine Endopeptidases, Pancreatitis-Associated Proteins, Bacterial Physiological Phenomena, Enzyme Activation, Enzyme Induction, Hemolymph, Manduca, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Animals, Amino Acid Sequence, Cloning, Molecular

Abstract

Proteolytic activation of prophenoloxidase in insects is a component of the host defense system against invading pathogens and parasites. We have purified from hemolymph of the tobacco hornworm, Manduca sexta, a new serine proteinase that cleaves prophenoloxidase. This enzyme, designated prophenoloxidase-activating proteinase-2 (PAP-2), differs from another PAP, previously isolated from integuments of the same insect (PAP-1). PAP-2 contains two clip domains at its amino terminus and a catalytic domain at its carboxyl terminus, whereas PAP-1 has only one clip domain. Purified PAP-2 cleaved prophenoloxidase at Arg(51) but yielded a product that has little phenoloxidase activity. However, in the presence of two serine proteinase homologs, active phenoloxidase was generated at a much higher level, and it formed covalently linked, high molecular weight oligomers. The serine proteinase homologs associate with a bacteria-binding lectin in M. sexta hemolymph, indicating that they may be important for ensuring that the activation of prophenoloxidase occurs only in the vicinity of invading microorganisms. PAP-2 mRNA was not detected in naive larval fat body or hemocytes, but it became abundant in these tissues after the insects were injected with bacteria.

Published

2002

17. A family of 16-kDa pancreatic secretory stress proteins form highly organized fibrillar structures upon tryptic activation

Author

Rolf Graf, Daniel Bimmler, George A. Scheele, Marc Schiesser, Thomas W. Frick, Klaus Marquardt, and Rudolf W. Ammann

Subjects

Gene isoform, Proteases, Genetic Vectors, Molecular Sequence Data, Nerve Tissue Proteins, Pancreatitis-Associated Proteins, Biology, Biochemistry, Pichia, Serine, 03 medical and health sciences, 0302 clinical medicine, Lithostathine, medicine, Extracellular, Animals, Protein Isoforms, Trypsin, Amino Acid Sequence, Cloning, Molecular, Molecular Biology, Pancreas, Heat-Shock Proteins, 030304 developmental biology, chemistry.chemical_classification, 0303 health sciences, Calcium-Binding Proteins, Cell Biology, Phosphoproteins, Peptide Fragments, Recombinant Proteins, Amino acid, Rats, Kinetics, Microscopy, Electron, chemistry, Pancreatic juice, 030211 gastroenterology & hepatology, Sequence Alignment, medicine.drug, Cysteine

Abstract

A group of 16-kDa proteins, synthesized and secreted by rat pancreatic acinar cells and composed of pancreatic stone protein (PSP/reg) and isoforms of pancreatitis-associated protein (PAP), show structural homologies, including conserved amino acid sequences, cysteine residues, and highly sensitive N-terminal trypsin cleavage sites, as well as conserved functional responses in conditions of pancreatic stress. Trypsin activation of recombinant stress proteins or counterparts contained in rat pancreatic juice (PSP/reg, PAP I and PAP III) resulted in conversion of 16-kDa soluble proteins into 14-kDa soluble isoforms (pancreatic thread protein and pancreatitis-associated thread protein, respectively) that rapidly polymerize into insoluble sedimenting structures. Activated thread proteins show long lived resistance to a wide spectrum of proteases contained in pancreatic juice, including serine proteases and metalloproteinases. In contrast, PAP II, following activation with trypsin or pancreatic juice, does not form insoluble structures and is rapidly digested by pancreatic proteases. Scanning and transmission electron microscopy indicate that activated thread proteins polymerize into highly organized fibrillar structures with helical configurations. Through bundling, branching, and extension processes, these fibrillar structures form dense matrices that span large topological surfaces. These findings suggest that PSP/reg and PAP I and III isoforms consist of a family of highly regulated soluble secretory stress proteins, which, upon trypsin activation, convert into a family of insoluble helical thread proteins. Dense extracellular matrices, composed of helical thread proteins organized into higher ordered matrix structures, may serve physiological functions within luminal compartments in the exocrine pancreas.

Published

2001

18. Regulation of cyclooxygenase-2 expression by phosphatidate phosphohydrolase in human amnionic WISH cells

Author

Christina A. Johnson, Edward A. Dennis, María A. Balboa, and Jesús Balsinde

Subjects

Enzymologic, Transcription, Genetic, Phosphodiesterase Inhibitors, medicine.medical_treatment, Pancreatitis-Associated Proteins, Biochemistry, Medical and Health Sciences, chemistry.chemical_compound, Sulfonamides, Arachidonic Acid, Amnion, biology, Biological Sciences, Propranolol, Isoenzymes, medicine.anatomical_structure, Tetradecanoylphorbol Acetate, Arachidonic acid, lipids (amino acids, peptides, and proteins), Transcription, Prostaglandin E, medicine.medical_specialty, Biochemistry & Molecular Biology, Phosphatidate Phosphatase, Naphthalenes, Dinoprostone, Gene Expression Regulation, Enzymologic, Cell Line, Genetic, Internal medicine, medicine, Humans, Secretion, Cyclooxygenase Inhibitors, Protein kinase A, Molecular Biology, Nitrobenzenes, Cyclooxygenase 2 Inhibitors, Ethanol, Membrane Proteins, Cell Biology, Metabolic pathway, Kinetics, Endocrinology, Eicosanoid, chemistry, Gene Expression Regulation, Cyclooxygenase 2, Prostaglandin-Endoperoxide Synthases, Pyrones, Chemical Sciences, biology.protein, Cyclooxygenase

Abstract

Prostaglandins are known to play a key role in the initiation of labor in humans, but the mechanisms governing their synthesis in amnion are largely unknown. In this study, we have examined the regulatory pathways for prostaglandin E(2) (PGE(2)) production during protein kinase C-dependent activation of human WISH cells. In these cells, PGE(2) synthesis appears to be limited not by free arachidonic acid availability but by the expression levels of cyclooxygenase-2 (COX-2). Concomitant with the cells being able to synthesize and secrete PGE(2), we detected significant elevations of both COX-2 protein and mRNA levels. Specific inhibition of COX-2 by NS-398 totally ablated PGE(2) synthesis. All of these responses were found to be strikingly dependent on an active phosphatidate phosphohydrolase 1 (PAP-1). Inhibition of PAP-1 activity by three different strategies (i.e. use of bromoenol lactone, propranolol, and ethanol) resulted in inhibition of COX-2 expression and hence of PGE(2) production. These data unveil a novel signaling mechanism for the regulation of PGE(2) production via regulation of COX-2 expression and implicate phosphatidate phosphohydrolase 1 as a key regulatory component of eicosanoid metabolic pathways in the amnion.

Published

1999

19. Acylation of naturally occurring and synthetic 1-deoxysphinganines by ceramide synthase. Formation of N-palmitoyl-aminopentol produces a toxic metabolite of hydrolyzed fumonisin, AP1, and a new category of ceramide synthase inhibitor

Author

H U, Humpf, E M, Schmelz, F I, Meredith, H, Vesper, T R, Vales, E, Wang, D S, Menaldino, D C, Liotta, and A H, Merrill

Subjects

Kinetics, Sphingosine, Acylation, Hydrolysis, Carboxylic Acids, Palmitic Acid, Humans, Pancreatitis-Associated Proteins, Mycotoxins, Oxidoreductases, Fumonisins

Abstract

Fumonisin B1 (FB1) is the predominant member of a family of mycotoxins produced by Fusarium moniliforme (Sheldon) and related fungi. Certain foods also contain the aminopentol backbone (AP1) that is formed upon base hydrolysis of the ester-linked tricarballylic acids of FB1. Both FB1 and, to a lesser extent, AP1 inhibit ceramide synthase due to structural similarities between fumonisins (as 1-deoxy-analogs of sphinganine) and sphingoid bases. To explore these structure-function relationships further, erythro- and threo-2-amino, 3-hydroxy- (and 3, 5-dihydroxy-) octadecanes were prepared by highly stereoselective syntheses. All of these analogs inhibit the acylation of sphingoid bases by ceramide synthase, and are themselves acylated with Vmax/Km of 40-125 for the erythro-isomers (compared with approximately 250 for D-erythro-sphinganine) and 4-6 for the threo-isomers. Ceramide synthase also acylates AP1 (but not FB1, under the conditions tested) to N-palmitoyl-AP1 (PAP1) with a Vmax/Km of approximately 1. The toxicity of PAP1 was evaluated using HT29 cells, a human colonic cell line. PAP1 was at least 10 times more toxic than FB1 or AP1 and caused sphinganine accumulation as an inhibitor of ceramide synthase. These studies demonstrate that: the 1-hydroxyl group is not required for sphingoid bases to be acylated; both erythro- and threo-isomers are acylated with the highest apparent Vmax/Km for the erythro-analogs; and AP1 is acylated to PAP1, a new category of ceramide synthase inhibitor as well as a toxic metabolite that may play a role in the diseases caused by fumonisins.

Published

1998

20. Isolation, expression, and regulation of the pgr1(+) gene encoding glutathione reductase absolutely required for the growth of Schizosaccharomyces pombe

Author

Jung-Hye Roe, Ian W. Dawes, and Joon Lee

Subjects

Transcription, Genetic, Saccharomyces cerevisiae, Glutathione reductase, Genes, Fungal, Molecular Sequence Data, Pancreatitis-Associated Proteins, Biology, Biochemistry, Fungal Proteins, chemistry.chemical_compound, Exon, Menadione, Gene Expression Regulation, Fungal, Gene expression, Schizosaccharomyces, Amino Acid Sequence, Molecular Biology, Gene, Genomic Library, Base Sequence, Glutathione Disulfide, Intron, Cell Biology, Sequence Analysis, DNA, biology.organism_classification, Molecular biology, Glutathione, Aerobiosis, Recombinant Proteins, DNA-Binding Proteins, Oxidative Stress, Basic-Leucine Zipper Transcription Factors, Glutathione Reductase, chemistry, Schizosaccharomyces pombe, Genes, Lethal, Schizosaccharomyces pombe Proteins

Abstract

The pgr1(+) gene encoding glutathione reductase (GR, EC 1.6.4.2) was isolated from Schizosaccharomyces pombe using a polymerase chain reaction fragment as a probe. The gene consists of two exons and an intron of 55 nucleotides, encoding a polypeptide of 465 amino acids (50,238 Da) with conserved residues characteristic of GR. The transcriptional start site was localized at 239 nucleotides upstream from the ATG initiation codon. The level of transcript as well as the GR enzyme activity increased more than 11-fold when the cloned pgr1(+) gene was expressed on a multicopy plasmid. This overexpression conferred on S. pombe cells more resistance against menadione, a redox cycling agent, but not against H2O2. The level of pgr1(+) transcripts increased by treatment with oxidants such as menadione, cumene hydroperoxide, and diamide. It also increased by treatment with high osmolarity, heat shock, or at the stationary growth phase. The deletion of the pap1(+) gene encoding an AP-1 homolog in S. pombe caused reduction in the pgr1(+) gene expression. Furthermore, Deltapap1 cells lost the inducibility of pgr1(+) gene expression by the above stresses, implying that Pap1 is involved in general stress-inducible gene expression. When the pgr1(+) gene was disrupted, the haploid spores were not viable. Repression of nmt1 promoter-driven pgr1(+) expression by thiamine caused cessation of growth, which was rescued by the episomal pgr1(+) gene. These results indicate that GR activity, which efficiently reduces GSSG, is essentially required for the growth of S. pombe, unlike in Saccharomyces cerevisiae or Escherichia coli.

Published

1997

21. Pancreatitis-associated protein I (PAP I), an acute phase protein induced by cytokines. Identification of two functional interleukin-6 response elements in the rat PAP I promoter region

Author

N J, Dusetti, E M, Ortiz, G V, Mallo, J C, Dagorn, and J L, Iovanna

Subjects

Binding Sites, Base Sequence, Interleukin-6, Tumor Necrosis Factor-alpha, DNA Mutational Analysis, Molecular Sequence Data, Gene Expression, Pancreatitis-Associated Proteins, Dexamethasone, Rats, Interferon-gamma, Structure-Activity Relationship, Oligodeoxyribonucleotides, Antigens, Neoplasm, Biomarkers, Tumor, Animals, Cytokines, Lectins, C-Type, RNA, Messenger, Promoter Regions, Genetic, Acute-Phase Proteins, Interleukin-1, Sequence Deletion

Abstract

Expression of the pancreatitis-associated protein I (PAP I), an exocrine pancreatic protein, increases rapidly and strongly in acinar cells during the acute phase of pancreatitis. This is reminiscent of the response to stress of acute phase proteins. We have previously demonstrated that serum factors from rats with acute pancreatitis, but not from healthy rats, could induce endogenous PAP I gene expression in the acinar cell line AR-42J (Dusetti, N., Mallo, G., Dagorn, J.-C., Iovanna, J. L. (1994) Biochem. Biophys. Res. Commun. 204, 238-243). In the present work, we have evaluated the influence of several mediators of inflammation on rat PAP I gene transcription in these cells. Tumor necrosis factor alpha induced an increase in PAP I mRNA expression, and interferon gamma caused an even greater increase in PAP I mRNA level. These stimulations were antagonized by dexamethasone. Interleukin (IL)-1, IL-6, or dexamethasone alone were ineffective. Combinations of IL-1 with IL-6 or dexamethasone were also ineffective. IL-6 and dexamethasone together induced a marked stimulation of PAP I gene transcription, and this effect was slightly attenuated by IL-1. To analyze the cis-regulatory elements responsible for the induction of transcription, we fused a 1.2-kilobase segment of the rat PAP I promoter to the chloramphenicol acetyltransferase (CAT) gene as reporter. The resultant chimeric DNA was transfected into AR-42J cells. Addition of IL-6 or dexamethasone was ineffective, whereas their mixture increased the CAT activity 12 times. Progressive deletions of the PAP I promoter were then fused to the CAT gene, and the constructs were transfected to AR-42J cells. A 12-fold increase in CAT activity was seen upon IL-6/dexamethasone treatment with constructs containing more than 274 base pairs upstream from the cap site. In that region, two sequences are similar to the canonical IL-6 response element. Site-directed mutagenesis of these regions strongly decreased induction, showing that they were functional. PAP I should therefore be classified among acute phase proteins of class 2, whose expression is increased by IL-6 acting in combination with glucocorticoids.

Published

1995

22. Brefeldin A sensitivity and resistance in Schizosaccharomyces pombe. Isolation of multiple genes conferring resistance

Author

T G, Turi, P, Webster, and J K, Rose

Subjects

Antifungal Agents, Brefeldin A, Sequence Homology, Amino Acid, Molecular Sequence Data, Golgi Apparatus, Receptors, Cytoplasmic and Nuclear, Drug Resistance, Microbial, Pancreatitis-Associated Proteins, Cyclopentanes, Saccharomyces cerevisiae, Karyopherins, Fungal Proteins, Phenotype, Mutation, Schizosaccharomyces, Amino Acid Sequence, Plasmids

Abstract

The fungal metabolite brefeldin A (BFA) causes the inhibition of protein secretion and the disruption of the structure and function of the Golgi complex in mammalian cells. Here we show that BFA has identical effects in the fission yeast Schizosaccharomyces pombe which normally contains a Golgi complex of stacked cisternae similar to the Golgi complexes in animal cells. After treatment with BFA, secretion was inhibited, Golgi complexes disappeared, and there was an accumulation of endoplasmic reticulum. These results indicate that the effects of BFA in fungi are very similar to those in mammalian cells and provide direct evidence for an effect of BFA on Golgi morphology in fungi. Five spontaneous BFA-resistant mutants were isolated. Genetic analysis showed that the mutations conferring BFA resistance were dominant and in two separate linkage groups. One of the BFA-resistant mutations was found to be allelic to crm1, a gene affecting chromatin structure. All BFA-resistant mutants overexpressed a 20-kDa protein, and the corresponding gene obr1 was isolated and sequenced. However, obr1 overexpression was not sufficient to confer BFA resistance. Plasmids capable of conferring BFA resistance to wild type cells were isolated from libraries constructed from the two BFA-resistant mutants. These plasmids contain six different genes capable of conferring resistance when present in high copy. One of these genes encoded the transcription factor pap1, a homolog of the mammalian AP1 protein. The overexpression of pap1 probably confers BFA resistance indirectly by inducing expression of one or more other proteins. The isolation of several genes conferring BFA resistance suggests several mechanisms are involved.

Published

1994

23. Structural organization of the gene encoding the rat pancreatitis-associated protein. Analysis of its evolutionary history reveals an ancient divergence from the other carbohydrate-recognition domain-containing genes

Author

N J, Dusetti, J M, Frigerio, V, Keim, J C, Dagorn, and J L, Iovanna

Subjects

Transcription, Genetic, Molecular Sequence Data, Gene Expression, Pancreatitis-Associated Proteins, Polymerase Chain Reaction, Antigens, Neoplasm, Lectins, Biomarkers, Tumor, Animals, Lectins, C-Type, Amino Acid Sequence, RNA, Messenger, Promoter Regions, Genetic, Base Sequence, Sequence Homology, Amino Acid, Genetic Variation, Proteins, Exons, Oligonucleotides, Antisense, Biological Evolution, Introns, Rats, Pancreatitis, Organ Specificity, Protein Biosynthesis, Acute Disease

Abstract

Rat pancreatitis-associated protein (PAP) mRNA is barely detectable in normal pancreas and overexpressed during acute pancreatitis (Iovanna, J., Orelle, B., Keim, V., and Dagorn J.-C. (1991) J. Biol. Chem. 266, 24664-24669). RNA amplification by reverse-transcriptase-coupled polymerase chain reaction showed that PAP mRNA was constitutively expressed in duodenum, jejunum, and ileum, at similar levels as in pancreas during the acute phase of pancreatitis. A weak expression was also detected in several other tissues. The rat PAP gene was isolated from a genomic library and characterized over 3.2 kilobases of gene sequence and 1.2 kilobases of 5'-flanking sequence. The 5' end of the coding sequence was determined by primer extension of the PAP transcript. Several potential regulatory elements were identified in the promoter region, including a pancreas-specific consensus sequence, two Pan1 (pancreas-specific) transcription activators, two IL-6 response elements, and one glucocorticoid response element. The PAP coding sequence spanned over six exons. The first three exons encoded the 5'-untranslated region of the mRNA, the signal peptide, and 39 amino acids of the NH2-terminal end of the mature protein, respectively. The other three exons encoded a domain of the protein with significant homology to the carbohydrate-recognition domain of animal lectins. Sequence comparison of the PAP gene with 13 carbohydrate-recognition domain-containing genes revealed that they derived from the same ancestor gene. Position of introns within the carbohydrate-recognition domain were different, however, suggesting that PAP belongs to a new group of lectins. These results support the hypothesis that genes encoding PAP and other lectins evolved from a common ancestor gene by intron gain.

Published

1993

24. Messenger RNA sequence and expression of rat pancreatitis-associated protein, a lectin-related protein overexpressed during acute experimental pancreatitis

Author

J, Iovanna, B, Orelle, V, Keim, and J C, Dagorn

Subjects

Base Sequence, Molecular Sequence Data, Proteins, Pancreatitis-Associated Proteins, DNA, Blotting, Northern, Bacterial Adhesion, Rats, Gene Expression Regulation, Pancreatitis, Antigens, Neoplasm, Lectins, Sequence Homology, Nucleic Acid, Acute Disease, Amylases, Biomarkers, Tumor, Animals, Lectins, C-Type, Amino Acid Sequence, RNA, Messenger, Sequence Alignment

Abstract

Rat pancreatitis-associated protein (PAP) is an additional protein appearing in pancreatic juice after induction of prancreatic inflammation. Its messenger RNA was cloned and sequenced from pancreas. The deduced amino acid sequence revealed that PAP was synthetized as a preprotein with, in its mature form, a predicted molecular weight of 16,630. A search in protein data bases revealed a marked homology with the carbohydrate binding region of animal lectins; no hemagglutination activity could be shown for PAP, but the protein induced extensive bacterial aggregation. In healthy rats, the very low level of PAP expression in pancreas could be increased up to 4-fold by physiological stimuli such as chronic hormonal or cholinergic stimulation of pancreatic secretion and adaptation of rats to a carbohydrate-rich diet. By contrast, induction of acute experimental pancreatitis by retrograde injection of sodium taurocholate resulted in dramatic overexpression. Pancreatic concentration of PAP mRNA increased more than 300 x within 12 h whereas concentrations of mRNAs encoding major secretory proteins such as amylase decreased. PAP overexpression persisted during the 2 days of the acute phase and then returned to the control level during pancreatic recovery. PAP mRNA could not be evidenced in liver, stomach, salivary glands, brain, kidney, or testis. Its pattern of expression during severe pancreatic aggression suggests that it might be a stress protein involved in the control of bacterial proliferation.

Published

1991

25. Characterization and purification of a mammalian osmoregulatory protein, aldose reductase, induced in renal medullary cells by high extracellular NaCl

Author

J J, Bedford, S M, Bagnasco, P F, Kador, H W, Harris, and M B, Burg

Subjects

Immunodiffusion, Kidney Medulla, Pancreatitis-Associated Proteins, Sodium Chloride, Epithelium, Cell Line, Substrate Specificity, Molecular Weight, Kinetics, Aldehyde Reductase, Enzyme Induction, Animals, Rabbits, Sugar Alcohol Dehydrogenases

Abstract

GRB-PAP1 is a continuous line of epithelial cells derived from a rabbit renal inner medulla. Elevation of the NaCl concentration in the medium bathing these cells strongly induced the expression of a soluble protein with an apparent molecular mass of 39 kDa. The protein, purified by affinity chromatography with Amicon Matrex Gel Orange A, had enzyme activity characteristic of aldose reductase (alditol:NADPH+ oxidoreductase, EC 1.1.1.21). Goat antiserum against this purified aldose reductase selected the 39-kDa band from immunoblots of cells grown in a medium containing high NaCl. When the osmolality of the medium was increased by adding NaCl, the amount of aldose reductase protein and the aldose reductase activity increased together from very low to sustained high levels over several days. The aldose reductase protein was more than 10% of the soluble cell protein when cells were propagated in medium made hyperosmotic by adding NaCl to increase medium osmolality to 600 mosm.kg-1.

Published

1987