Your search keyword '"Raufman JP"' showing total 7 results

1. Protein Kinase C Isoform Expression and Function in Transformed and Non-transformed Pancreatic Acinar Cell Lines

Author

Raufman Jp, Bao Ly, Nam J, Josef Michl, Robert D. Raffaniello, Cho I, and Junying Lin

Subjects

Gene isoform, Cell type, Protein Kinase C-alpha, Cellular differentiation, Biophysics, Biology, Biochemistry, Cell Line, Acinar cell, Animals, Enzyme Inhibitors, Pancreas, Molecular Biology, Protein Kinase C, Protein kinase C, Cell Line, Transformed, Acinar cell proliferation, Cell growth, Cell Biology, Molecular biology, Rats, Cell biology, Isoenzymes, Genes, ras, Cell culture, Cell Division, Subcellular Fractions

Abstract

Members of the protein kinase C (PKC) family of multifunctional serine/threonine phosphorylating enzymes are believed to play a role in regulating cellular differentiation and proliferation in many cell types. In the present study, we examined the expression of PKC isoforms in non-transformed (BMRPA.430) and transformed (TUC3) rat pancreatic acinar cell lines and compared this to PKC expression in freshly dispersed acini from rat pancreas. BMRPA.430 cells maintain characteristics of normal acini and are not tumorigenic, whereas TUC3 cells do not express tight junctions or polygonal morphology and are tumorigenic. As reported previously, PKC alpha, delta, epsilon, and zeta are expressed in freshly prepared acini. Likewise, these isoforms were detected in both the BMRPA.430 and TUC3 cell lines. In addition, PKC theta, a novel isoform, was detected in all three cell types at low levels. We used two PKC inhibitors to examine the role of PKC in acinar cell proliferation. CGP 41 251, a selective PKC inhibitor, and Go 6976, an agent which specifically inhibits calcium-dependent PKC isoforms, inhibited cell proliferation of both cell lines. Translocation of PKC alpha to the membrane was not observed in either cell line. Hence, our data indicate that ras-induced transformation does not alter PKC isoform expression in pancreatic acinar cells and that activation of PKC alpha is involved with acinar cell growth.

Published

1998

2. Muscarinic receptor agonists stimulate matrix metalloproteinase 1-dependent invasion of human colon cancer cells.

Author

Raufman JP, Cheng K, Saxena N, Chahdi A, Belo A, Khurana S, and Xie G

Subjects

Acetylcholine metabolism, Acetylcholine pharmacology, Cell Movement drug effects, Colonic Neoplasms enzymology, HT29 Cells, Humans, Matrix Metalloproteinase 1 genetics, Neoplasm Invasiveness, Taurodeoxycholic Acid pharmacology, Colonic Neoplasms pathology, Matrix Metalloproteinase 1 metabolism, Muscarinic Agonists pharmacology, Receptors, Muscarinic metabolism

Abstract

Mammalian matrix metalloproteinases (MMPs) which degrade extracellular matrix facilitate colon cancer cell invasion into the bloodstream and extra-colonic tissues; in particular, MMP1 expression correlates strongly with advanced colon cancer stage, hematogenous metastasis and poor prognosis. Likewise, muscarinic receptor signaling plays an important role in colon cancer; muscarinic receptors are over-expressed in colon cancer compared to normal colon epithelial cells. Muscarinic receptor activation stimulates proliferation, migration and invasion of human colon cancer cells. In mouse intestinal neoplasia models genetic ablation of muscarinic receptors attenuates carcinogenesis. In the present work, we sought to link these observations by showing that MMP1 expression and activation plays a mechanistic role in muscarinic receptor agonist-induced colon cancer cell invasion. We show that acetylcholine, which robustly increases MMP1 expression, stimulates invasion of HT29 and H508 human colon cancer cells into human umbilical vein endothelial cell monolayers - this was abolished by pre-incubation with atropine, a non-selective muscarinic receptor inhibitor, and by pre-incubation with anti-MMP1 neutralizing antibody. Similar results were obtained using a Matrigel chamber assay and deoxycholyltaurine (DCT), an amidated dihydroxy bile acid associated with colon neoplasia in animal models and humans, and previously shown to interact functionally with muscarinic receptors. DCT treatment of human colon cancer cells resulted in time-dependent, 10-fold increased MMP1 expression, and DCT-induced cell invasion was also blocked by pre-treatment with anti-MMP1 antibody. This study contributes to understanding mechanisms underlying muscarinic receptor agonist-induced promotion of colon cancer and, more importantly, indicates that blocking MMP1 expression and activation has therapeutic promise to stop or retard colon cancer invasion and dissemination., (Copyright © 2011 Elsevier Inc. All rights reserved.)

Published

2011

3. 3',5'-Cyclic diguanylic acid (c-di-GMP) inhibits basal and growth factor-stimulated human colon cancer cell proliferation.

Author

Karaolis DK, Cheng K, Lipsky M, Elnabawi A, Catalano J, Hyodo M, Hayakawa Y, and Raufman JP

Subjects

Acetylcholine metabolism, Animals, Cell Line, Cell Line, Tumor, Cell Proliferation, Colonic Neoplasms pathology, Dose-Response Relationship, Drug, Epidermal Growth Factor metabolism, Humans, Kidney cytology, Kidney metabolism, Models, Molecular, Neuroblastoma pathology, Rats, Staphylococcus aureus metabolism, Colonic Neoplasms metabolism, Cyclic GMP analogs & derivatives, Cyclic GMP metabolism, Growth Substances metabolism

Abstract

The novel cyclic dinucleotide, 3',5'-cyclic diguanylic acid, cGpGp (c-di-GMP), is a naturally occurring small molecule that regulates important signaling mechanisms in prokaryotes. Recently, we showed that c-di-GMP has "drug-like" properties and that c-di-GMP treatment might be a useful antimicrobial approach to attenuate the virulence and pathogenesis of Staphylococcus aureus and prevent or treat infection. In the present communication, we report that c-di-GMP (50 microM) has striking properties regarding inhibition of cancer cell proliferation in vitro. c-di-GMP inhibits both basal and growth factor (acetylcholine and epidermal growth factor)-induced cell proliferation of human colon cancer (H508) cells. Toxicity studies revealed that exposure of normal rat kidney cells and human neuroblastoma cells to c-di-GMP at biologically relevant doses showed no lethal cytotoxicity. Cyclic dinucleotides, such as c-di-GMP, represent an attractive and novel "drug-platform technology" that can be used not only to develop new antimicrobial agents, but also to develop novel therapeutic agents to prevent or treat cancer.

Published

2005

4. Protein kinase C isoform expression and function in transformed and non-transformed pancreatic acinar cell lines.

Author

Raffaniello RD, Nam J, Cho I, Lin J, Bao LY, Michl J, and Raufman JP

Subjects

Animals, Cell Division drug effects, Cell Line, Cell Line, Transformed, Enzyme Inhibitors pharmacology, Genes, ras, Isoenzymes antagonists & inhibitors, Pancreas cytology, Pancreas drug effects, Protein Kinase C antagonists & inhibitors, Protein Kinase C-alpha, Rats, Subcellular Fractions enzymology, Isoenzymes metabolism, Pancreas enzymology, Protein Kinase C metabolism

Abstract

Members of the protein kinase C (PKC) family of multifunctional serine/threonine phosphorylating enzymes are believed to play a role in regulating cellular differentiation and proliferation in many cell types. In the present study, we examined the expression of PKC isoforms in non-transformed (BMRPA.430) and transformed (TUC3) rat pancreatic acinar cell lines and compared this to PKC expression in freshly dispersed acini from rat pancreas. BMRPA.430 cells maintain characteristics of normal acini and are not tumorigenic, whereas TUC3 cells do not express tight junctions or polygonal morphology and are tumorigenic. As reported previously, PKC alpha, delta, epsilon, and zeta are expressed in freshly prepared acini. Likewise, these isoforms were detected in both the BMRPA.430 and TUC3 cell lines. In addition, PKC theta, a novel isoform, was detected in all three cell types at low levels. We used two PKC inhibitors to examine the role of PKC in acinar cell proliferation. CGP 41 251, a selective PKC inhibitor, and Go 6976, an agent which specifically inhibits calcium-dependent PKC isoforms, inhibited cell proliferation of both cell lines. Translocation of PKC alpha to the membrane was not observed in either cell line. Hence, our data indicate that ras-induced transformation does not alter PKC isoform expression in pancreatic acinar cells and that activation of PKC alpha is involved with acinar cell growth.

Published

1998

5. Actions and expression of RAB-GDP dissociation inhibitor in dispersed chief cells from guinea pig stomach.

Author

Raffaniello RD, Lin J, and Raufman JP

Subjects

Animals, Cells, Cultured, GTP-Binding Proteins biosynthesis, GTP-Binding Proteins isolation & purification, GTP-Binding Proteins metabolism, Gastric Mucosa drug effects, Guinea Pigs, Kinetics, Male, Nerve Tissue Proteins metabolism, Recombinant Fusion Proteins biosynthesis, Recombinant Fusion Proteins pharmacology, Subcellular Fractions metabolism, rab3 GTP-Binding Proteins, GTP-Binding Proteins physiology, Gastric Mucosa metabolism, Guanine Nucleotide Dissociation Inhibitors, Pepsinogens metabolism

Abstract

Rab proteins are a family of ras-like proteins that are involved in intracellular membrane trafficking. Rab-GDP dissociation inhibitor prevents dissociation of GDP from Rab proteins and extracts Rab proteins from cell membranes in vitro. In the present study, we examined the effects of recombinant rab-GDI on Rab proteins in gastric chief cells. Rab-GDI extracted GTP-binding proteins, including Rab3 and Rab5, from chief cell membranes in a dose-dependent manner. Maximal concentrations of rab-GDI (> or = 50 micrograms/ml) removed approx. 40% of membrane-associated Rab3. Moreover, preincubation of permeabilized chief cells with rab-GDI resulted in a 35% decrease in GTP gamma S(100 microM)-induced pepsinogen secretion, suggesting that membrane-associated Rab proteins are involved in the final stages of secretion. Immunostaining of chief cell cytosolic and membrane fractions with GDI-specific antisera revealed bands at 56 and 48 kDa, respectively, indicating that chief cells express two isoforms of rab-GDI. In gastric chief cells, regulation of Rab proteins by rab-GDI plays an important role in mediating exocytosis.

Published

1996

6. GTP gamma S-induced pepsinogen secretion from gastric chief cells does not require carboxyl methylation or translocation of low molecular weight (LMW) GTP-binding proteins.

Author

Raffaniello RD and Raufman JP

Subjects

Animals, Cell Membrane chemistry, Cell Membrane Permeability, Cytosol chemistry, Exocytosis drug effects, GTP-Binding Proteins isolation & purification, Gastric Mucosa drug effects, Guinea Pigs, Male, Methylation, Molecular Weight, GTP-Binding Proteins metabolism, Gastric Mucosa metabolism, Guanosine 5'-O-(3-Thiotriphosphate) pharmacology, Pepsinogens metabolism

Abstract

We identified at least four LMW GTP-binding proteins in membrane and cytosolic fractions from dispersed gastric chief cells. Extraction of membrane-bound GTP-binding proteins with various agents revealed that these proteins are intimately associated with chief cell membranes. Upon extraction with Triton X-114, the majority of GTP-binding proteins partitioned into the detergent phase, indicative of their hydrophobic nature. Although carboxyl methylation of LMW GTP-binding proteins has been shown to regulate their localization and function, inhibitors of carboxyl methylation had no effect on GTP gamma S-induced pepsinogen secretion. Moreover, pre-permeabilization of chief cells for up to 20 min did not alter GTP gamma S-induced secretion, suggesting that the guanine nucleotide analogue interacts with membrane-bound GTP-binding proteins to elicit a secretory response.

Published

1995

7. Increases in cellular calcium concentration stimulate pepsinogen secretion from dispersed chief cells.

Author

Raufman JP, Berger S, Cosowsky L, and Straus E

Subjects

Aminoquinolines, Animals, Calcimycin pharmacology, Cytoplasm metabolism, Dose-Response Relationship, Drug, Ethers pharmacology, Gastric Mucosa cytology, Guinea Pigs, Ionomycin, Male, Pepsin A analysis, Calcium physiology, Gastric Mucosa metabolism, Pepsinogens metabolism

Abstract

Intracellular calcium concentration ([Ca]i) and pepsinogen secretion from dispersed chief cells from guinea pig stomach were determined before and after stimulation with calcium ionophores. [Ca]i was measured using the fluorescent probe quin2. Basal [Ca]i was 105 +/- 4 nM. Pepsinogen secretion was measured with a new assay using 125I-albumin substrate. This assay is 1000-fold more sensitive than the widely-used spectrophotometric assay, technically easy to perform, rapid, and relatively inexpensive. The kinetics and stoichiometry of ionophore-induced changes in [Ca]i and pepsinogen secretion were similar. These data support a role for calcium as a cellular mediator of pepsinogen secretion.

Published

1986