Your search keyword '"Garfield SH"' showing total 43 results

1. Exosomes released by k562 chronic myeloid leukemia cells promote endothelial cell tubular differentiation through uptake and cell-to-cell transfer

Author

MINEO, Marco, TAVERNA, Simona, FLUGY PAPE', Anna Maria, DE LEO, Giacomo, ALESSANDRO, Riccardo, Garfield, SH, Kohn, EC, Mineo, M, Garfield, SH, Taverna, S, Flugy Pape', AM, De Leo, G, Alessandro, R, and Kohn, EC

Subjects

Exosomes, Nanotubes, Chronic myeloid leukemia, Endothelial cells, Tyrosine kinase inhibitors

Abstract

Exosomes, microvesicles of endocytic origin released by normal and tumor cells, play an important role in cell-to-cell ommunication. Angiogenesis has been shown to regulate progression of chronic myeloid leukemia (CML). The mechanism through which this happens has not been elucidated. We isolated and characterized exosomes from K562 CML cells and evaluated their effects on human umbilical endothelial cells (HUVECs). Fluorescent-labeled exosomes were nternalized by HUVECs during tubular differentiation on Matrigel. Exosome localization was perinuclear early in differentiation, moving peripherally in cells undergoing elongation and connection. Exosomes move within and between nanotubular structures connecting the remodeling endothelial cells. They stimulated angiotube formation over a serum/growth factor-limited medium control,doubling total cumulative tube length (P = 0.003). Treatment of K562 cells with two clinically active tyrosine kinase inhibitors, imatinib and dasatinib, reduced their total exosome release (P\0.009); equivalent concentrations of drug-treated exosomes induced a similar extent of tubular differentiation. However, dasatinib treatment of HUVECs markedly inhibited HUVEC response to drug control CML exosomes (P\0.002). In an in vivo mouse matrigel plug model angiogenesis was induced by K562 exosomes and abrogated by oral dasatinib treatment (P\0.01). K562 exosomes induced dasatinib-sensitive Src phosphorylation and activation of downstream Src pathway proteins in HUVECs. Imatinib was minimally active against exosome stimulation of HUVEC cell differentiation and signaling. Thus, CML cell-derived exosomes induce angiogenic activity in HUVEC cells. The inhibitory effect of dasatinib on exosome production and vascular differentiation and signaling reveals a key role for Src in both the leukemia and its microenvironment.

Published

2012

2. Exosomes released by K562 chronic myeloid leukemia cells promote angiogenesis in a Src-dependent fashion

Author

Mineo, M, Garfield, Sh, Taverna, Simona, Flugy, A, De Leo, G, Alessandro, R, and Kohn, E. C.

Published

2011

3. A function-blocking CD47 antibody suppresses stem cell and EGF signaling in triple-negative breast cancer.

Author

Kaur S, Elkahloun AG, Singh SP, Chen QR, Meerzaman DM, Song T, Manu N, Wu W, Mannan P, Garfield SH, and Roberts DD

Subjects

Antibodies, Blocking immunology, Antigens, Differentiation genetics, Antigens, Differentiation metabolism, Blotting, Western, CD47 Antigen genetics, CD47 Antigen immunology, Cell Line, Cell Line, Tumor, Cell Proliferation drug effects, Cell Proliferation genetics, Epidermal Growth Factor genetics, Epidermal Growth Factor metabolism, Epidermal Growth Factor pharmacology, ErbB Receptors genetics, Female, Gene Expression Profiling methods, Gene Expression Regulation, Neoplastic genetics, Humans, Kruppel-Like Factor 4, MCF-7 Cells, MicroRNAs genetics, Microscopy, Confocal, Neoplastic Stem Cells metabolism, Neoplastic Stem Cells pathology, Phosphorylation drug effects, Receptors, Immunologic genetics, Receptors, Immunologic metabolism, Reverse Transcriptase Polymerase Chain Reaction, Signal Transduction genetics, Thrombospondin 1 genetics, Thrombospondin 1 metabolism, Triple Negative Breast Neoplasms genetics, Triple Negative Breast Neoplasms metabolism, Triple Negative Breast Neoplasms pathology, Antibodies, Blocking pharmacology, CD47 Antigen metabolism, ErbB Receptors metabolism, Neoplastic Stem Cells drug effects, Signal Transduction drug effects

Abstract

CD47 is a signaling receptor for thrombospondin-1 and the counter-receptor for signal-regulatory protein-α (SIRPα). By inducing inhibitory SIRPα signaling, elevated CD47 expression by some cancers prevents macrophage phagocytosis. The anti-human CD47 antibody B6H12 inhibits tumor growth in several xenograft models, presumably by preventing SIRPα engagement. However, CD47 signaling in nontransformed and some malignant cells regulates self-renewal, suggesting that CD47 antibodies may therapeutically target cancer stem cells (CSCs). Treatment of MDA-MB-231 breast CSCs with B6H12 decreased proliferation and asymmetric cell division. Similar effects were observed in T47D CSCs but not in MCF7 breast carcinoma or MCF10A breast epithelial cells. Gene expression analysis in breast CSCs treated with B6H12 showed decreased expression of epidermal growth factor receptor (EGFR) and the stem cell transcription factor KLF4. EGFR and KLF4 mRNAs are known targets of microRNA-7, and B6H12 treatment correspondingly enhanced microRNA-7 expression in breast CSCs. B6H12 treatment also acutely inhibited EGF-induced EGFR tyrosine phosphorylation. Expression of B6H12-responsive genes correlated with CD47 mRNA expression in human breast cancers, suggesting that the CD47 signaling pathways identified in breast CSCs are functional in vivo. These data reveal a novel SIRPα-independent mechanism by which therapeutic CD47 antibodies could control tumor growth by autonomously forcing differentiation of CSC.

Published

2016

4. Variations in Glycogen Synthesis in Human Pluripotent Stem Cells with Altered Pluripotent States.

Author

Chen RJ, Zhang G, Garfield SH, Shi YJ, Chen KG, Robey PG, and Leapman RD

Subjects

Bone Morphogenetic Protein 4 metabolism, Cell Differentiation, Cell Line, Cell Proliferation, Glycogen Synthase metabolism, Glycogen Synthase Kinase 3 metabolism, Humans, Induced Pluripotent Stem Cells cytology, Induced Pluripotent Stem Cells metabolism, Glycogen metabolism, Pluripotent Stem Cells cytology, Pluripotent Stem Cells metabolism

Abstract

Human pluripotent stem cells (hPSCs) represent very promising resources for cell-based regenerative medicine. It is essential to determine the biological implications of some fundamental physiological processes (such as glycogen metabolism) in these stem cells. In this report, we employ electron, immunofluorescence microscopy, and biochemical methods to study glycogen synthesis in hPSCs. Our results indicate that there is a high level of glycogen synthesis (0.28 to 0.62 μg/μg proteins) in undifferentiated human embryonic stem cells (hESCs) compared with the glycogen levels (0 to 0.25 μg/μg proteins) reported in human cancer cell lines. Moreover, we found that glycogen synthesis was regulated by bone morphogenetic protein 4 (BMP-4) and the glycogen synthase kinase 3 (GSK-3) pathway. Our observation of glycogen bodies and sustained expression of the pluripotent factor Oct-4 mediated by the potent GSK-3 inhibitor CHIR-99021 reveals an altered pluripotent state in hPSC culture. We further confirmed glycogen variations under different naïve pluripotent cell growth conditions based on the addition of the GSK-3 inhibitor BIO. Our data suggest that primed hPSCs treated with naïve growth conditions acquire altered pluripotent states, similar to those naïve-like hPSCs, with increased glycogen synthesis. Furthermore, we found that suppression of phosphorylated glycogen synthase was an underlying mechanism responsible for altered glycogen synthesis. Thus, our novel findings regarding the dynamic changes in glycogen metabolism provide new markers to assess the energetic and various pluripotent states in hPSCs. The components of glycogen metabolic pathways offer new assays to delineate previously unrecognized properties of hPSCs under different growth conditions.

Published

2015

5. CD47 signaling regulates the immunosuppressive activity of VEGF in T cells.

Author

Kaur S, Chang T, Singh SP, Lim L, Mannan P, Garfield SH, Pendrak ML, Soto-Pantoja DR, Rosenberg AZ, Jin S, and Roberts DD

Subjects

Animals, CD47 Antigen biosynthesis, CD47 Antigen genetics, CD8-Positive T-Lymphocytes immunology, Cell Communication immunology, Cell Line, Tumor, Cell Proliferation, Humans, Jurkat Cells, Lymphocyte Activation immunology, Mice, Mice, Knockout, Neovascularization, Pathologic immunology, Phosphorylation, Receptors, Antigen, T-Cell immunology, Signal Transduction immunology, Up-Regulation, Vascular Endothelial Growth Factor A biosynthesis, Vascular Endothelial Growth Factor Receptor-2 biosynthesis, src-Family Kinases metabolism, CD4-Positive T-Lymphocytes immunology, CD47 Antigen immunology, Immune Tolerance, Thrombospondin 1 immunology, Vascular Endothelial Growth Factor A immunology, Vascular Endothelial Growth Factor Receptor-2 metabolism

Abstract

Thrombospondin-1 (TSP1) inhibits angiogenesis, in part, by interacting with the ubiquitous cell-surface receptor CD47. In endothelial cells, CD47 interacts directly with vascular endothelial growth factor receptor (VEGFR)-2, and TSP1 inhibits VEGFR2 phosphorylation and signaling by disrupting this association. We show that CD47 similarly associates with and regulates VEGFR2 in T cells. TSP1 inhibits phosphorylation of VEGFR2 and its downstream target Src in wild type but not in CD47-deficient human Jurkat and primary murine T cells. VEGFR2 signaling inhibits proliferation and TCR signaling in wild type T cells. However, ligation of CD47 by TSP1 or loss of CD47 expression reverses some inhibitory effects of VEGF on proliferation and T cell activation. We further found that VEGF and VEGFR2 expression are upregulated in CD47-deficient murine CD4(+) and human Jurkat T cells, and the resulting autocrine VEGFR2 signaling enhances proliferation and some TCR responses in the absence of CD47. Thus, CD47 signaling modulates the ability of VEGF to regulate proliferation and TCR signaling, and autocrine production of VEGF by T cells contributes to this regulation. This provides a mechanism to understand the context-dependent effects of TSP1 and VEGF on T cell activation, and reveals an important role for CD47 signaling in regulating T cell production of the major angiogenic factor VEGF.

Published

2014

6. Telomerase variant A279T induces telomere dysfunction and inhibits non-canonical telomerase activity in esophageal carcinomas.

Author

Zhang Y, Calado R, Rao M, Hong JA, Meeker AK, Dumitriu B, Atay S, McCormick PJ, Garfield SH, Wangsa D, Padilla-Nash HM, Burkett S, Zhang M, Kunst TF, Peterson NR, Xi S, Inchauste S, Altorki NK, Casson AG, Beer DG, Harris CC, Ried T, Young NS, and Schrump DS

Subjects

Amino Acid Substitution, Animals, Cell Line, Tumor, Esophageal Neoplasms genetics, Esophageal Neoplasms pathology, Female, Humans, Male, Mice, Mice, Nude, Neoplasm Proteins genetics, RNA biosynthesis, RNA genetics, RNA, Neoplasm biosynthesis, RNA, Neoplasm genetics, Telomerase genetics, Telomere enzymology, Telomere genetics, Esophageal Neoplasms enzymology, Gene Expression Regulation, Enzymologic, Gene Expression Regulation, Neoplastic, Mutation, Missense, Neoplasm Proteins biosynthesis, Telomerase biosynthesis, Telomere Homeostasis

Abstract

Background: Although implicated in the pathogenesis of several chronic inflammatory disorders and hematologic malignancies, telomerase mutations have not been thoroughly characterized in human cancers. The present study was performed to examine the frequency and potential clinical relevance of telomerase mutations in esophageal carcinomas., Methods: Sequencing techniques were used to evaluate mutational status of telomerase reverse transcriptase (TERT) and telomerase RNA component (TERC) in neoplastic and adjacent normal mucosa from 143 esophageal cancer (EsC) patients. MTS, flow cytometry, time lapse microscopy, and murine xenograft techniques were used to assess proliferation, apoptosis, chemotaxis, and tumorigenicity of EsC cells expressing either wtTERT or TERT variants. Immunoprecipitation, immunoblot, immunofluorescence, promoter-reporter and qRT-PCR techniques were used to evaluate interactions of TERT and several TERT variants with BRG-1 and β-catenin, and to assess expression of cytoskeletal proteins, and cell signaling. Fluorescence in-situ hybridization and spectral karyotyping techniques were used to examine telomere length and chromosomal stability., Results: Sequencing analysis revealed one deletion involving TERC (TERC del 341-360), and two non-synonymous TERT variants [A279T (2 homozygous, 9 heterozygous); A1062T (4 heterozygous)]. The minor allele frequency of the A279T variant was five-fold higher in EsC patients compared to healthy blood donors (p<0.01). Relative to wtTERT, A279T decreased telomere length, destabilized TERT-BRG-1-β-catenin complex, markedly depleted β-catenin, and down-regulated canonical Wnt signaling in cancer cells; these phenomena coincided with decreased proliferation, depletion of additional cytoskeletal proteins, impaired chemotaxis, increased chemosensitivity, and significantly decreased tumorigenicity of EsC cells. A279T expression significantly increased chromosomal aberrations in mouse embryonic fibroblasts (MEFs) following Zeocin™ exposure, as well as Li Fraumeni fibroblasts in the absence of pharmacologically-induced DNA damage., Conclusions: A279T induces telomere dysfunction and inhibits non-canonical telomerase activity in esophageal cancer cells. These findings warrant further analysis of A279T expression in esophageal cancers and premalignant esophageal lesions.

Published

2014

7. Wnt and the cancer niche: paracrine interactions with gastrointestinal cancer cells undergoing asymmetric cell division.

Author

Xin HW, Ambe CM, Ray S, Kim BK, Koizumi T, Wiegand GW, Hari D, Mullinax JE, Jaiswal KR, Garfield SH, Stojadinovic A, Rudloff U, Thorgeirsson SS, and Avital I

Abstract

Objective: Stem-like cancer cells contribute to cancer initiation and maintenance. Stem cells can self-renew by asymmetric cell division (ACD). ACD with non-random chromosomal cosegregation (ACD-NRCC) is one possible self-renewal mechanism. There is a paucity of evidence supporting ACD-NRCC in human cancer. Our aim was to investigate ACD-NRCC and its potential interactions with the cancer niche (microenvironment) in gastrointestinal cancers., Design: We used DNA double and single labeling approaches with FACS to isolate live cells undergoing ACD-NRCC., Results: Gastrointestinal cancers contain rare subpopulations of cells capable of ACD-NRCC. ACD-NRCC was detected preferentially in subpopulations of cells previously suggested to be stem-like/tumor-initiating cancer cells. ACD-NRCC was independent of cell-to-cell contact, and was regulated by the cancer niche in a heat-sensitive paracrine fashion. Wnt pathway genes and proteins are differentially expressed in cells undergoing ACD-NRCC vs. symmetric cell division. Blocking the Wnt pathway with IWP2 (WNT antagonist) or siRNA-TCF4 resulted in suppression of ACD-NRCC. However, using a Wnt-agonist did not increase the relative proportion of cells undergoing ACD-NRCC., Conclusion: Gastrointestinal cancers contain subpopulations of cells capable of ACD-NRCC. Here we show for the first time that ACD-NRCC can be regulated by the Wnt pathway, and by the cancer niche in a paracrine fashion. However, whether ACD-NRCC is exclusively associated with stem-like cancer cells remains to be determined. Further study of these findings might generate novel insights into stem cell and cancer biology. Targeting the mechanism of ACD-NRCC might engender novel approaches for cancer therapy.

Published

2013

8. Biological profile of the less lipophilic and synthetically more accessible bryostatin 7 closely resembles that of bryostatin 1.

Author

Kedei N, Lewin NE, Géczy T, Selezneva J, Braun DC, Chen J, Herrmann MA, Heldman MR, Lim L, Mannan P, Garfield SH, Poudel YB, Cummins TJ, Rudra A, Blumberg PM, and Keck GE

Subjects

Bryostatins chemical synthesis, Bryostatins chemistry, Cell Line, Tumor, Down-Regulation, Humans, Isoenzymes metabolism, Male, Membrane Potential, Mitochondrial drug effects, Protein Kinase C metabolism, Real-Time Polymerase Chain Reaction, Subcellular Fractions enzymology, U937 Cells, Bryostatins pharmacology, Lipids chemistry

Abstract

The bryostatins are a group of 20 macrolides isolated by Pettit and co-workers from the marine organism Bugula neritina. Bryostatin 1, the flagship member of the family, has been the subject of intense chemical and biological investigations due to its remarkably diverse biological activities, including promising indications as therapy for cancer, Alzheimer's disease, and HIV. Other bryostatins, however, have attracted far less attention, most probably due to their relatively low natural abundance and associated scarcity of supply. Among all macrolides in this family, bryostatin 7 is biologically the most potent protein kinase C (PKC) ligand (in terms of binding affinity) and also the first bryostatin to be synthesized in the laboratory. Nonetheless, almost no biological studies have been carried out on this agent. We describe herein the total synthesis of bryostatin 7 based on our pyran annulation technology, which allows for the first detailed biological characterizations of bryostatin 7 with side-by-side comparisons to bryostatin 1. The results suggest that the more easily synthesized and less lipophilic bryostatin 7 may be an effective surrogate for bryostatin 1.

Published

2013

9. Molecular basis for failure of "atypical" C1 domain of Vav1 to bind diacylglycerol/phorbol ester.

Author

Geczy T, Peach ML, El Kazzouli S, Sigano DM, Kang JH, Valle CJ, Selezneva J, Woo W, Kedei N, Lewin NE, Garfield SH, Lim L, Mannan P, Marquez VE, and Blumberg PM

Subjects

Amino Acid Sequence, Cell Line, Tumor, Humans, Lactones metabolism, Ligands, Male, Molecular Sequence Data, Mutagenesis, Site-Directed, Phospholipids metabolism, Prostatic Neoplasms, Protein Binding physiology, Protein Kinase C-delta metabolism, Protein Structure, Tertiary, Proto-Oncogene Proteins c-vav genetics, Signal Transduction physiology, Diglycerides metabolism, Phorbol Esters metabolism, Proto-Oncogene Proteins c-vav chemistry, Proto-Oncogene Proteins c-vav metabolism

Abstract

C1 domains, the recognition motif of the second messenger diacylglycerol and of the phorbol esters, are classified as typical (ligand-responsive) or atypical (not ligand-responsive). The C1 domain of Vav1, a guanine nucleotide exchange factor, plays a critical role in regulation of Vav activity through stabilization of the Dbl homology domain, which is responsible for exchange activity of Vav. Although the C1 domain of Vav1 is classified as atypical, it retains a binding pocket geometry homologous to that of the typical C1 domains of PKCs. This study clarifies the basis for its failure to bind ligands. Substituting Vav1-specific residues into the C1b domain of PKCδ, we identified five crucial residues (Glu(9), Glu(10), Thr(11), Thr(24), and Tyr(26)) along the rim of the binding cleft that weaken binding potency in a cumulative fashion. Reciprocally, replacing these incompatible residues in the Vav1 C1 domain with the corresponding residues from PKCδ C1b (δC1b) conferred high potency for phorbol ester binding. Computer modeling predicts that these unique residues in Vav1 increase the hydrophilicity of the rim of the binding pocket, impairing membrane association and thereby preventing formation of the ternary C1-ligand-membrane binding complex. The initial design of diacylglycerol-lactones to exploit these Vav1 unique residues showed enhanced selectivity for C1 domains incorporating these residues, suggesting a strategy for the development of ligands targeting Vav1.

Published

2012

10. Tumor-initiating label-retaining cancer cells in human gastrointestinal cancers undergo asymmetric cell division.

Author

Xin HW, Hari DM, Mullinax JE, Ambe CM, Koizumi T, Ray S, Anderson AJ, Wiegand GW, Garfield SH, Thorgeirsson SS, and Avital I

Subjects

Animals, Cell Line, Tumor, Cell Survival, Gastrointestinal Neoplasms genetics, Gene Expression Profiling, Gene Expression Regulation, Neoplastic, Humans, Mice, Models, Biological, Pluripotent Stem Cells metabolism, Asymmetric Cell Division, Gastrointestinal Neoplasms metabolism, Gastrointestinal Neoplasms pathology, Neoplastic Stem Cells metabolism, Neoplastic Stem Cells pathology, Staining and Labeling

Abstract

Label-retaining cells (LRCs) have been proposed to represent adult tissue stem cells. LRCs are hypothesized to result from either slow cycling or asymmetric cell division (ACD). However, the stem cell nature and whether LRC undergo ACD remain controversial. Here, we demonstrate label-retaining cancer cells (LRCCs) in several gastrointestinal (GI) cancers including fresh surgical specimens. Using a novel method for isolation of live LRCC, we demonstrate that a subpopulation of LRCC is actively dividing and exhibits stem cells and pluripotency gene expression profiles. Using real-time confocal microscopic cinematography, we show live LRCC undergoing asymmetric nonrandom chromosomal cosegregation LRC division. Importantly, LRCCs have greater tumor-initiating capacity than non-LRCCs. Based on our data and that cancers develop in tissues that harbor normal-LRC, we propose that LRCC might represent a novel population of GI stem-like cancer cells. LRCC may provide novel mechanistic insights into the biology of cancer and regenerative medicine and present novel targets for cancer treatment., (Copyright © 2012 AlphaMed Press.)

Published

2012

11. Exosomes released by K562 chronic myeloid leukemia cells promote angiogenesis in a Src-dependent fashion.

Author

Mineo M, Garfield SH, Taverna S, Flugy A, De Leo G, Alessandro R, and Kohn EC

Subjects

Animals, Benzamides, Cell Communication drug effects, Cell Differentiation drug effects, Collagen drug effects, Culture Media, Conditioned pharmacology, Dasatinib, Drug Combinations, Endocytosis drug effects, Exosomes drug effects, Exosomes ultrastructure, Human Umbilical Vein Endothelial Cells cytology, Human Umbilical Vein Endothelial Cells drug effects, Human Umbilical Vein Endothelial Cells enzymology, Humans, Imatinib Mesylate, K562 Cells, Laminin drug effects, Leukemia, Myelogenous, Chronic, BCR-ABL Positive drug therapy, Mice, Mice, Nude, Nanotubes, Piperazines pharmacology, Piperazines therapeutic use, Proteoglycans drug effects, Pyrimidines pharmacology, Pyrimidines therapeutic use, Reproducibility of Results, Signal Transduction drug effects, Thiazoles pharmacology, Thiazoles therapeutic use, Time Factors, Exosomes metabolism, Leukemia, Myelogenous, Chronic, BCR-ABL Positive metabolism, Neovascularization, Physiologic drug effects, src-Family Kinases metabolism

Abstract

Exosomes, microvesicles of endocytic origin released by normal and tumor cells, play an important role in cell-to-cell communication. Angiogenesis has been shown to regulate progression of chronic myeloid leukemia (CML). The mechanism through which this happens has not been elucidated. We isolated and characterized exosomes from K562 CML cells and evaluated their effects on human umbilical endothelial cells (HUVECs). Fluorescent-labeled exosomes were internalized by HUVECs during tubular differentiation on Matrigel. Exosome localization was perinuclear early in differentiation, moving peripherally in cells undergoing elongation and connection. Exosomes move within and between nanotubular structures connecting the remodeling endothelial cells. They stimulated angiotube formation over a serum/growth factor-limited medium control, doubling total cumulative tube length (P = 0.003). Treatment of K562 cells with two clinically active tyrosine kinase inhibitors, imatinib and dasatinib, reduced their total exosome release (P < 0.009); equivalent concentrations of drug-treated exosomes induced a similar extent of tubular differentiation. However, dasatinib treatment of HUVECs markedly inhibited HUVEC response to drug control CML exosomes (P < 0.002). In an in vivo mouse Matrigel plug model angiogenesis was induced by K562 exosomes and abrogated by oral dasatinib treatment (P < 0.01). K562 exosomes induced dasatinib-sensitive Src phosphorylation and activation of downstream Src pathway proteins in HUVECs. Imatinib was minimally active against exosome stimulation of HUVEC cell differentiation and signaling. Thus, CML cell-derived exosomes induce angiogenic activity in HUVEC cells. The inhibitory effect of dasatinib on exosome production and vascular differentiation and signaling reveals a key role for Src in both the leukemia and its microenvironment.

Published

2012

12. N-methyl-substituted fluorescent DAG-indololactone isomers exhibit dramatic differences in membrane interactions and biological activity.

Author

Gal N, Kolusheva S, Kedei N, Telek A, Naeem TA, Lewin NE, Lim L, Mannan P, Garfield SH, El Kazzouli S, Sigano DM, Marquez VE, Blumberg PM, and Jelinek R

Subjects

Animals, CHO Cells, Cell Membrane drug effects, Cell Membrane metabolism, Cricetinae, Diglycerides chemistry, Diglycerides pharmacology, Guanine Nucleotide Exchange Factors metabolism, Humans, Indoles chemistry, Indoles pharmacokinetics, Indoles pharmacology, Isomerism, Lactones pharmacokinetics, Protein Isoforms antagonists & inhibitors, Protein Isoforms metabolism, Protein Kinase C-alpha antagonists & inhibitors, Protein Kinase C-alpha metabolism, Protein Kinase Inhibitors pharmacokinetics, Protein Transport drug effects, Lactones chemistry, Lactones pharmacology, Protein Kinase C antagonists & inhibitors, Protein Kinase C metabolism, Protein Kinase Inhibitors chemistry, Protein Kinase Inhibitors pharmacology

Abstract

N-methyl-substituted diacylglycerol-indololactones (DAG-indololactones) are newly synthesized effectors of protein kinase C (PKC) isoforms and exhibit substantial selectivity between RasGRP3 and PKCα. We present a comprehensive analysis of membrane interactions and biological activities of several DAG-indololactones. Translocation and binding activity assays underline significant variations between the PKC translocation characteristics affected by the ligands as compared to their binding activities. In parallel, the fluorescent properties of the ligands were employed for analysis of their membrane association profiles. Specifically, we found that a slight change in the linkage to the indole ring resulted in significant differences in membrane binding and association of the DAG-indololactones with lipid bilayers. Our analysis shows that seemingly small structural modifications of the hydrophobic regions of these biomimetic PKC effectors contribute to pronounced modulation of membrane interactions of the ligands.

Published

2011

13. The synthetic bryostatin analog Merle 23 dissects distinct mechanisms of bryostatin activity in the LNCaP human prostate cancer cell line.

Author

Kedei N, Telek A, Czap A, Lubart ES, Czifra G, Yang D, Chen J, Morrison T, Goldsmith PK, Lim L, Mannan P, Garfield SH, Kraft MB, Li W, Keck GE, and Blumberg PM

Subjects

Apoptosis drug effects, Bryostatins chemistry, Cell Division drug effects, Cell Line, Tumor, Down-Regulation, Humans, Male, Phosphorylation, Prostatic Neoplasms metabolism, Prostatic Neoplasms pathology, Protein Kinase C metabolism, Subcellular Fractions drug effects, Subcellular Fractions enzymology, Subcellular Fractions metabolism, Tetradecanoylphorbol Acetate pharmacology, Tumor Necrosis Factor-alpha metabolism, U937 Cells, Bryostatins pharmacology

Abstract

Bryostatin 1 has attracted considerable attention both as a cancer chemotherapeutic agent and for its unique activity. Although it functions, like phorbol esters, as a potent protein kinase C (PKC) activator, it paradoxically antagonizes many phorbol ester responses in cells. Because of its complex structure, little is known of its structure-function relations. Merle 23 is a synthetic derivative, differing from bryostatin 1 at only four positions. However, in U-937 human leukemia cells, Merle 23 behaves like a phorbol ester and not like bryostatin 1. Here, we characterize the behavior of Merle 23 in the human prostate cancer cell line LNCaP. In this system, bryostatin 1 and phorbol ester have contrasting activities, with the phorbol ester but not bryostatin 1 blocking cell proliferation or tumor necrosis factor alpha secretion, among other responses. We show that Merle 23 displays a highly complex pattern of activity in this system. Depending on the specific biological response or mechanistic change, it was bryostatin-like, phorbol ester-like, intermediate in its behavior, or more effective than either. The pattern of response, moreover, varied depending on the conditions. We conclude that the newly emerging bryostatin derivatives such as Merle 23 provide powerful tools to dissect subsets of bryostatin mechanism and response., (Published by Elsevier Inc.)

Published

2011

14. Some phorbol esters might partially resemble bryostatin 1 in their actions on LNCaP prostate cancer cells and U937 leukemia cells.

Author

Kedei N, Lubart E, Lewin NE, Telek A, Lim L, Mannan P, Garfield SH, Kraft MB, Keck GE, Kolusheva S, Jelinek R, and Blumberg PM

Subjects

Cell Line, Tumor, Cell Proliferation drug effects, Dose-Response Relationship, Drug, Humans, Inhibitory Concentration 50, Leukemia pathology, Male, Molecular Structure, Prostatic Neoplasms pathology, Antineoplastic Agents pharmacology, Bryostatins pharmacology, Phorbol Esters pharmacology

Abstract

Phorbol 12-myristate 13-acetate (PMA) and bryostatin 1 are both potent protein kinase C (PKC) activators. In LNCaP human prostate cancer cells, PMA induces tumor necrosis factor alpha (TNFα) secretion and inhibits proliferation; bryostatin 1 does not, and indeed blocks the response to PMA. This difference has been attributed to bryostatin 1 not localizing PKCδ to the plasma membrane. Since phorbol ester lipophilicity influences PKCδ localization, we have examined in LNCaP cells a series of phorbol esters and related derivatives spanning some eight logs in lipophilicity (logP) to see if any behave like bryostatin 1. The compounds showed marked differences in their effects on proliferation and TNFα secretion. For example, maximal responses for TNFα secretion relative to PMA ranged from 97 % for octyl-indolactam V to 24 % for phorbol 12,13-dibenzoate. Dose-response curves ranged from monophasic for indolactam V to markedly biphasic for sapintoxin D. The divergent patterns of response, however, correlated neither to lipophilicity, to plasma membrane translocation of PKCδ, nor to the ability to interact with model membranes. In U937 human leukemia cells, a second system in which PMA and bryostatin 1 have divergent effects, viz. PMA but not bryostatin 1 inhibits proliferation and induces attachment, all the compounds acted like PMA for proliferation, but several induced a reduced level or a biphasic dose-response curve for attachment. We conclude that active phorbol esters are not all equivalent. Depending on the system, some might partially resemble bryostatin 1 in their behavior; this encourages the concept that bryostatin-like behavior may be obtained from other structural templates., (Copyright © 2011 WILEY-VCH Verlag GmbH & Co. KGaA, Weinheim.)

Published

2011

15. Thrombospondin-1 inhibits VEGF receptor-2 signaling by disrupting its association with CD47.

Author

Kaur S, Martin-Manso G, Pendrak ML, Garfield SH, Isenberg JS, and Roberts DD

Subjects

Animals, Cattle, Cell Membrane metabolism, Endothelial Cells cytology, Humans, Mice, Microscopy, Confocal methods, Neovascularization, Pathologic, Nitric Oxide Synthase Type III metabolism, Phosphorylation, Signal Transduction, Thrombospondins metabolism, CD47 Antigen metabolism, Thrombospondin 1 metabolism, Vascular Endothelial Growth Factor Receptor-2 metabolism

Abstract

Thrombospondin-1 (TSP1) can inhibit angiogenic responses directly by interacting with VEGF and indirectly by engaging several endothelial cell TSP1 receptors. We now describe a more potent mechanism by which TSP1 inhibits VEGF receptor-2 (VEGFR2) activation through engaging its receptor CD47. CD47 ligation is known to inhibit downstream signaling targets of VEGFR2, including endothelial nitric-oxide synthase and soluble guanylate cyclase, but direct effects on VEGFR2 have not been examined. Based on FRET and co-immunoprecipitation, CD47 constitutively associated with VEGFR2. Ligation of CD47 by TSP1 abolished resonance energy transfer with VEGFR2 and inhibited phosphorylation of VEGFR2 and its downstream target Akt without inhibiting VEGF binding to VEGFR2. The inhibitory activity of TSP1 in large vessel and microvascular endothelial cells was replicated by a recombinant domain of the protein containing its CD47-binding site and by a CD47-binding peptide derived from this domain but not by the CD36-binding domain of TSP1. Inhibition of VEGFR2 phosphorylation was lost when CD47 expression was suppressed in human endothelial cells and in murine CD47-null cells. These results reveal that anti-angiogenic signaling through CD47 is highly redundant and extends beyond inhibition of nitric oxide signaling to global inhibition of VEGFR2 signaling.

Published

2010

16. The skin cancer chemotherapeutic agent ingenol-3-angelate (PEP005) is a substrate for the epidermal multidrug transporter (ABCB1) and targets tumor vasculature.

Author

Li L, Shukla S, Lee A, Garfield SH, Maloney DJ, Ambudkar SV, and Yuspa SH

Subjects

ATP Binding Cassette Transporter, Subfamily B, ATP Binding Cassette Transporter, Subfamily B, Member 1 antagonists & inhibitors, Administration, Topical, Animals, Antineoplastic Agents pharmacokinetics, Antineoplastic Agents pharmacology, Carcinoma, Squamous Cell blood supply, Carcinoma, Squamous Cell drug therapy, Carcinoma, Squamous Cell metabolism, Cell Line, Tumor, Diterpenes pharmacokinetics, Diterpenes pharmacology, Drug Eruptions enzymology, Drug Eruptions etiology, Enzyme Activation drug effects, Humans, Keratinocytes drug effects, Keratinocytes enzymology, Melanoma, Experimental blood supply, Melanoma, Experimental drug therapy, Melanoma, Experimental metabolism, Mice, Mice, Inbred BALB C, Mice, Nude, Neovascularization, Pathologic drug therapy, Neovascularization, Pathologic metabolism, Protein Binding, Protein Kinase C metabolism, Skin drug effects, Skin enzymology, Skin Neoplasms blood supply, Tetradecanoylphorbol Acetate pharmacology, ATP Binding Cassette Transporter, Subfamily B, Member 1 metabolism, Antineoplastic Agents metabolism, Diterpenes metabolism, Skin Neoplasms drug therapy, Skin Neoplasms metabolism

Abstract

Ingenol-3-angelate (Ing3A), extracted from Euphorbia peplus, is currently in clinical trials for eradicating basal cell carcinoma, actinic keratosis, and squamous cell carcinoma (SCC) in situ by topical application. Although structurally related to phorbol esters and a protein kinase C activator, topical Ing3A, but not phorbol 12-myristate 13-acetate (PMA), inhibited the growth of subcutaneous tumors derived from PAM212 (mouse SCC) and B16 (mouse melanoma). Ing3A and PMA both induced acute neutrophilic inflammation on mouse skin, but only Ing3A caused subcutaneous hemorrhage and vascular damage. Both Ing3A and PMA activated extracellular signal-regulated kinase 1/2 (ERK1/2) in epidermis, but Ing3A also activated ERK1/2 in skin dermal fibroblasts and endothelial cells. Pretreatment with topical cyclosporin A (CsA), verapamil, or XR9576, modulators of P-glycoprotein (P-gp), prevented Ing3A-induced hemorrhage but not neutrophil infiltration. CsA also impaired the anticancer activity of Ing3A, whereas the anti-inflammatory dexamethasone did not. Ing3A, but not PMA, blocked photoaffinity labeling of human P-gp with [(125)I]iodoaryazidoprazosin and inhibited P-gp-mediated drug resistance to HCT-15 cells. The intracellular levels of Ing3A were significantly lower in P-gp-expressing cells, and treatment with XR9576 increased the levels to those of cells that do not express P-gp, showing that Ing3A binds to and is transported by P-gp. Taken together, our results suggest that P-gp-mediated absorptive transport, dermal penetration, and vascular damage contribute to the anticancer activity of Ing3A in vivo., (Copyright 2010 AACR.)

Published

2010

17. Characterization of the differential roles of the twin C1a and C1b domains of protein kinase C-delta.

Author

Pu Y, Garfield SH, Kedei N, and Blumberg PM

Subjects

Amino Acid Sequence, Animals, Cell Line, Cricetinae, Down-Regulation, Humans, Ligands, Mice, Molecular Sequence Data, Mutation genetics, Phorbol Esters metabolism, Protein Binding, Protein Kinase C-delta genetics, Protein Structure, Tertiary, Protein Transport, Substrate Specificity, Zinc Fingers, Protein Kinase C-delta chemistry, Protein Kinase C-delta metabolism

Abstract

Classic and novel protein kinase C (PKC) isozymes contain two zinc finger motifs, designated "C1a" and "C1b" domains, which constitute the recognition modules for the second messenger diacylglycerol (DAG) or the phorbol esters. However, the individual contributions of these tandem C1 domains to PKC function and, reciprocally, the influence of protein context on their function remain uncertain. In the present study, we prepared PKCdelta constructs in which the individual C1a and C1b domains were deleted, swapped, or substituted for one another to explore these issues. As isolated fragments, both the deltaC1a and deltaC1b domains potently bound phorbol esters, but the binding of [(3)H]phorbol 12,13-dibutyrate ([(3)H]PDBu) by the deltaC1a domain depended much more on the presence of phosphatidylserine than did that of the deltaC1b domain. In intact PKCdelta, the deltaC1b domain played the dominant role in [(3)H]PDBu binding, membrane translocation, and down-regulation. A contribution from the deltaC1a domain was nonetheless evident, as shown by retention of [(3)H]PDBu binding at reduced affinity, by increased [(3)H]PDBu affinity upon expression of a second deltaC1a domain substituting for the deltaC1b domain, and by loss of persistent plasma membrane translocation for PKCdelta expressing only the deltaC1b domain, but its contribution was less than predicted from the activity of the isolated domain. Switching the position of the deltaC1b domain to the normal position of the deltaC1a domain (or vice versa) had no apparent effect on the response to phorbol esters, suggesting that the specific position of the C1 domain within PKCdelta was not the primary determinant of its activity.

Published

2009

18. Disruption of microfilaments by cytochalasin B decreases accumulation of cisplatin in human epidermal carcinoma and liver carcinoma cell lines.

Author

Liang XJ, Yin JJ, Taylor B, Winkovitch SM, Garfield SH, Shen DW, Gottesman MM, and Aszalos A

Subjects

Actin Cytoskeleton drug effects, Biological Transport drug effects, Carcinoma metabolism, Carcinoma, Hepatocellular metabolism, Cell Division drug effects, Cell Line, Tumor drug effects, Cell Line, Tumor metabolism, Cell Membrane Permeability drug effects, Cisplatin pharmacology, Humans, KB Cells drug effects, KB Cells metabolism, Liver Neoplasms metabolism, Membrane Fluidity drug effects, Membrane Potentials drug effects, Skin Neoplasms metabolism, Actin Cytoskeleton physiology, Carcinoma pathology, Carcinoma, Hepatocellular pathology, Cisplatin metabolism, Cytochalasin B pharmacology, Drug Resistance, Neoplasm drug effects, Liver Neoplasms pathology, Skin Neoplasms pathology

Abstract

Background: Although cisplatin is a frequently used cancer chemotherapeutic drug, its effectiveness is hindered by the development of resistance in cancer cells. In order to understand the reason(s) for this resistance, the mechanism of uptake of cisplatin into cells must be characterized. While several previous studies showed structural differences between cisplatin-sensitive and resistant cells, the influence of microfilaments, known to affect transport of molecules into cells, and the influence of certain biophysical characteristics of the plasma membrane needed clarification., Results: We show that resistant human epidermal carcinoma (KB-CP20) and liver carcinoma (BEL-7404-CP20) cells become relatively more resistant if their already weak microfilaments are degraded by cytochalasin B treatment (.5-2 microM). The sensitive counterparts of these cells with intact microfilaments are not significantly affected by this treatment. We also show that the "fluidity" of the plasma membrane and the membrane potential of the sensitive and resistant cells studied do not appear to influence the uptake of cisplatin into the cells., Conclusion: Our results suggest that the status of the microfilament system influences the mechanism of uptake of cisplatin into cells.

Published

2008

19. Conformationally constrained analogues of diacylglycerol (DAG). 28. DAG-dioxolanones reveal a new additional interaction site in the C1b domain of PKC delta.

Author

Choi Y, Pu Y, Peach ML, Kang JH, Lewin NE, Sigano DM, Garfield SH, Blumberg PM, and Marquez VE

Subjects

Amino Acid Sequence, Animals, Binding Sites, CHO Cells, Cell Membrane metabolism, Cricetinae, Cricetulus, Diglycerides pharmacology, Dioxolanes pharmacology, Glutamine chemistry, Green Fluorescent Proteins genetics, Molecular Conformation, Molecular Sequence Data, Mutation, Protein Binding, Protein Kinase C-delta genetics, Protein Kinase C-delta metabolism, Protein Structure, Tertiary, Protein Transport, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Stereoisomerism, Diglycerides chemistry, Dioxolanes chemistry, Lactones chemistry, Models, Molecular, Protein Kinase C-delta chemistry

Abstract

Diacylglycerol (DAG) lactones have provided a powerful platform for structural exploration of the interactions between ligands and the C1 domains of protein kinase C (PKC). In this study, we report that DAG-dioxolanones, novel derivatives of DAG-lactones, exploit an additional point of contact (glutamine 27) in their binding with the C1b domain of PKC delta. Mutation of this point of contact to glutamate selectively impairs binding of the DAG-dioxolanones compared to that of the corresponding DAG-lactones (1200- to 3000-fold versus 35- to 55-fold, respectively). The differential response of this mutated C1b domain to the DAG-dioxolanones relative to the DAG-lactones provides a unique tool to probe the role of the C1b domain in PKC delta function, where the response to the DAG-lactones affords a positive control for retained function. Using this approach, we show that the C1b domain of PKC delta plays the predominant role in the translocation of PKC delta to the membrane in the presence of DAG.

Published

2007

20. Conformationally constrained analogues of diacylglycerol (DAG). 27. Modulation of membrane translocation of protein kinase C (PKC) isozymes alpha and delta by diacylglycerol lactones (DAG-lactones) containing rigid-rod acyl groups.

Author

Malolanarasimhan K, Kedei N, Sigano DM, Kelley JA, Lai CC, Lewin NE, Surawski RJ, Pavlyukovets VA, Garfield SH, Wincovitch S, Blumberg PM, and Marquez VE

Subjects

Animals, Binding Sites, Cell Adhesion, Cell Line, Cell Proliferation drug effects, Cricetinae, Cricetulus, Diglycerides chemistry, Diglycerides pharmacology, Extracellular Signal-Regulated MAP Kinases metabolism, Interleukin-6 metabolism, Isoenzymes metabolism, Kinetics, Lactones chemistry, Lactones pharmacology, Ligands, Molecular Conformation, Phosphorylation, Protein Binding, Protein Kinase C beta, Protein Transport, Structure-Activity Relationship, Cell Membrane metabolism, Diglycerides chemical synthesis, Lactones chemical synthesis, Protein Kinase C metabolism, Protein Kinase C-alpha metabolism

Abstract

Highly rigid and geometrically well-defined rods composed of ethynylene-substituted aromatic spacers [oligo(p-phenyleneethynylene), OPE] were incorporated as acyl moieties on diacylglycerol lactones (DAG-lactones) and investigated for their ability to bind to protein kinase C (PKC) and translocate PKC alpha and delta isoforms to plasma and internal membranes. The kinetics of PKC translocation were correlated with biological responses, viz. ERK phosphorylation, induction of IL-6 secretion, inhibition of cell proliferation, and induction of cellular attachment, that display very different time courses. Because OPE rods assemble through noncovalent forces and form stable films, they may influence the microdomain environment around the DAG-lactone membrane-binding site. A comparison of two DAG-lactones (1 and 10), one with two PE units (1) and the other with an equivalent flexible acyl chain (10) of matching lipophilicity, clearly demonstrated the effect of the rigid OPE chain in substantially prolonging the translocated state of both PKC alpha and delta.

Published

2007

21. Artificially introduced aneuploid chromosomes assume a conserved position in colon cancer cells.

Author

Sengupta K, Upender MB, Barenboim-Stapleton L, Nguyen QT, Wincovitch SM Sr, Garfield SH, Difilippantonio MJ, and Ried T

Subjects

Adenocarcinoma genetics, Animals, Chromosomes, Human, Pair 18, Chromosomes, Human, Pair 19, Chromosomes, Human, Pair 7, Colonic Neoplasms genetics, Gene Dosage, Gene Expression Regulation, Neoplastic, Humans, In Situ Hybridization, Fluorescence, Interphase, Mice, Microscopy, Confocal, Transcription, Genetic, Trisomy, Tumor Cells, Cultured ultrastructure, Adenocarcinoma pathology, Aneuploidy, Colonic Neoplasms pathology, Intranuclear Space ultrastructure

Abstract

Background: Chromosomal aneuploidy is a defining feature of carcinomas. For instance, in colon cancer, an additional copy of Chromosome 7 is not only observed in early pre-malignant polyps, but is faithfully maintained throughout progression to metastasis. These copy number changes show a positive correlation with average transcript levels of resident genes. An independent line of research has also established that specific chromosomes occupy a well conserved 3D position within the interphase nucleus., Methodology/principal Findings: We investigated whether cancer-specific aneuploid chromosomes assume a 3D-position similar to that of its endogenous homologues, which would suggest a possible correlation with transcriptional activity. Using 3D-FISH and confocal laser scanning microscopy, we show that Chromosomes 7, 18, or 19 introduced via microcell-mediated chromosome transfer into the parental diploid colon cancer cell line DLD-1 maintain their conserved position in the interphase nucleus., Conclusions: Our data is therefore consistent with the model that each chromosome has an associated zip code (possibly gene density) that determines its nuclear localization. Whether the nuclear localization determines or is determined by the transcriptional activity of resident genes has yet to be ascertained.

Published

2007

22. Effects on ligand interaction and membrane translocation of the positively charged arginine residues situated along the C1 domain binding cleft in the atypical protein kinase C isoforms.

Author

Pu Y, Peach ML, Garfield SH, Wincovitch S, Marquez VE, and Blumberg PM

Subjects

Amino Acid Sequence, Animals, Arginine genetics, Cell Line, Tumor, Computational Biology, Cricetinae, Humans, Ions chemistry, Isoenzymes chemistry, Isoenzymes genetics, Isoenzymes metabolism, Ligands, Models, Molecular, Molecular Sequence Data, Mutagenesis, Site-Directed, Protein Binding, Protein Kinase C genetics, Protein Structure, Tertiary, Protein Transport, Sequence Alignment, Static Electricity, Arginine chemistry, Arginine metabolism, Cell Membrane enzymology, Protein Kinase C chemistry, Protein Kinase C metabolism

Abstract

The C1 domain zinc finger structure is highly conserved among the protein kinase C (PKC) superfamily members. As the interaction site for the second messenger sn-1,2-diacylglycerol (DAG) and for the phorbol esters, the C1 domain has been an important target for developing selective ligands for different PKC isoforms. However, the C1 domains of the atypical PKC members are DAG/phorbol ester-insensitive. Compared with the DAG/phorbol ester-sensitive C1 domains, the rim of the binding cleft of the atypical PKC C1 domains possesses four additional positively charged arginine residues (at positions 7, 10, 11, and 20). In this study, we showed that mutation to arginines of the four corresponding sites in the C1b domain of PKCdelta abolished its high potency for phorbol 12,13-dibutyrate in vitro, with only marginal remaining activity for phorbol 12-myristate 13-acetate in vivo. We also demonstrated both in vitro and in vivo that the loss of potency to ligands was cumulative with the introduction of the arginine residues along the rim of the binding cavity rather than the consequence of loss of a single, specific residue. Computer modeling reveals that these arginine residues reduce access of ligands to the binding cleft and change the electrostatic profile of the C1 domain surface, whereas the basic structure of the binding cleft is still maintained. Finally, mutation of the four arginine residues of the atypical PKC C1 domains to the corresponding residues in the deltaC1b domain conferred response to phorbol ester. We speculate that the arginine residues of the C1 domain of atypical PKCs may provide an opportunity for the design of ligands selective for the atypical PKCs.

Published

2006

23. Multispectral imaging of clinically relevant cellular targets in tonsil and lymphoid tissue using semiconductor quantum dots.

Author

Fountaine TJ, Wincovitch SM, Geho DH, Garfield SH, and Pittaluga S

Subjects

Antigens analysis, B-Lymphocytes chemistry, B-Lymphocytes pathology, Biomarkers analysis, Chromogenic Compounds, Dendritic Cells, Follicular chemistry, Dendritic Cells, Follicular pathology, Diagnostic Imaging, Fluorescent Antibody Technique, Fluorescent Dyes, Humans, Lasers, Lymphoid Tissue pathology, Microchemistry instrumentation, Microscopy, Confocal, Nanotechnology instrumentation, Semiconductors, Spectrometry, Fluorescence instrumentation, Streptavidin chemistry, T-Lymphocytes chemistry, T-Lymphocytes pathology, Lymphoid Tissue chemistry, Microchemistry methods, Nanotechnology methods, Quantum Dots, Spectrometry, Fluorescence methods

Abstract

Determination of the expression and spatial distribution of molecular epitopes, or antigens, in patient tissue specimens has substantially improved the pathologist's ability to classify disease processes. Certain disease pathophysiologies are marked by characteristic increased or decreased expression of developmentally controlled antigens, defined as Cluster of Differentiation markers, that currently form the foundation for understanding lymphoid malignancies. While chromogens and organic fluorophores have been utilitized for some time in immunohistochemical analyses, developments in synthetic, inorganic fluorophore semiconductors, namely quantum dots, offer a versatile alternative reporter system. Quantum dots are stable fluorophores, are resistant to photobleaching, and are attributed with wide excitation ranges and narrow emission spectra. To date, routinely processed, formalin-fixed tissues have only been probed with two quantum dot reporters simultaneously. In the present study, streptavidin-conjugated quantum dots with distinct emission spectra were tested for their utility in identifying a variety of differentially expressed antigens (surface, cytoplasmic, and nuclear). Slides were analyzed using confocal laser scanning microscopy, which enabled with a single excitation wavelength (488 nm argon laser) the detection of up to seven signals (streptavidin-conjugated quantum dots 525, 565, 585, 605, 655, 705 and 805 nm) plus the detection of 4'6-DiAmidino-2-PhenylIndole with an infra-red laser tuned to 760 nm for two photon excitation. Each of these signals was specific for the intended morphologic immunohistochemical target. In addition, five of the seven streptavidin-conjugated quantum dots tested (not streptavidin-conjugated quantum dots 585 or 805 nm) were used on the same tissue section and could be analyzed simultaneously on routinely processed formalin-fixed, paraffin-embedded sections. Application of this multiplexing method will enable investigators to explore the clinically relevant multidimensional cellular interactions that underlie diseases, simultaneously., (Published online 16 June 2006.)

Published

2006

24. Melanosomal sequestration of cytotoxic drugs contributes to the intractability of malignant melanomas.

Author

Chen KG, Valencia JC, Lai B, Zhang G, Paterson JK, Rouzaud F, Berens W, Wincovitch SM, Garfield SH, Leapman RD, Hearing VJ, and Gottesman MM

Subjects

Antineoplastic Agents analysis, Biological Transport, Cell Line, Tumor, Cisplatin analysis, Cytoplasm chemistry, Cytoplasm metabolism, Humans, Indoles metabolism, Melanoma ultrastructure, Melanosomes chemistry, Skin Neoplasms ultrastructure, Antineoplastic Agents metabolism, Cisplatin metabolism, Drug Resistance, Multiple, Drug Resistance, Neoplasm, Melanoma metabolism, Melanosomes enzymology, Skin Neoplasms metabolism

Abstract

Multidrug resistance mechanisms underlying the intractability of malignant melanomas remain largely unknown. In this study, we demonstrate that the development of multidrug resistance in melanomas involves subcellular sequestration of intracellular cytotoxic drugs such as cis-diaminedichloroplatinum II (cisplatin; CDDP). CDDP is initially sequestered in subcellular organelles such as melanosomes, which significantly reduces its nuclear localization when compared with nonmelanoma/KB-3-1 epidermoid carcinoma cells. The melanosomal accumulation of CDDP remarkably modulates melanogenesis through a pronounced increase in tyrosinase activity. The altered melanogenesis manifested an approximately 8-fold increase in both intracellular pigmentation and extracellular transport of melanosomes containing CDDP. Thus, our experiments provide evidence that melanosomes contribute to the refractory properties of melanoma cells by sequestering cytotoxic drugs and increasing melanosome-mediated drug export. Preventing melanosomal sequestration of cytotoxic drugs by inhibiting the functions of melanosomes may have great potential as an approach to improving the chemosensitivity of melanoma cells.

Published

2006

25. Kinetics of penetration influence the apparent potency of vanilloids on TRPV1.

Author

Lazar J, Braun DC, Tóth A, Wang Y, Pearce LV, Pavlyukovets VA, Blumberg PM, Garfield SH, Wincovitch S, Choi HK, and Lee J

Subjects

Animals, Benzaldehydes chemistry, CHO Cells, Cricetinae, Microscopy, Confocal, Molecular Structure, Benzaldehydes pharmacokinetics, TRPV Cation Channels drug effects

Abstract

Evidence that the ligand binding site of TRPV1 lies on the inner face of the plasma membrane and that much of the TRPV1 itself is localized to internal membranes suggests that the rate of ligand entry into the cell may be an important determinant of the kinetics of ligand action. In this study, we synthesized a BODIPY TR-labeled fluorescent capsaicin analog (CHK-884) so that we could directly measure ligand entry. We report that CHK-884 penetrated only slowly into Chinese hamster ovary (CHO) cells expressing rat TRPV1, with a t1/2 of 30 +/- 4 min, and localized in the endoplasmic reticulum and Golgi. Although CHK-884 was only weakly potent for TRPV1 binding (Ki = 6400 +/- 230 nM), it was appreciably more potent when assayed by intracellular calcium imaging and was 3.2-fold more potent with a 1-h incubation time (37 nM) than with a 5-min incubation time. Olvanil, a highly lipophilic vanilloid, yielded an EC50 of 4.3 nM upon intracellular calcium imaging with an incubation time of 1 h, compared with an EC50 value of 29.5 nM for calcium imaging assayed at 5 min. Likewise, the antagonist 5-iodo-resiniferatoxin (5-iodo-RTX) displayed a Ki of 4.2 pM if incubated with CHO-TRPV1 cells for 2 h before addition of capsaicin compared with 1.5 nM if added simultaneously. We conclude that some vanilloids may have slow kinetics of uptake; this slow uptake may affect assessment of structure activity relations and may represent a significant factor for vanilloid drug design.

Published

2006

26. ING2 regulates the onset of replicative senescence by induction of p300-dependent p53 acetylation.

Author

Pedeux R, Sengupta S, Shen JC, Demidov ON, Saito S, Onogi H, Kumamoto K, Wincovitch S, Garfield SH, McMenamin M, Nagashima M, Grossman SR, Appella E, and Harris CC

Subjects

Acetylation, Cell Division physiology, Cell Line, Cell Proliferation, Homeodomain Proteins biosynthesis, Humans, Nuclear Proteins metabolism, Phosphorylation, Protein Processing, Post-Translational, Receptors, Cytoplasmic and Nuclear biosynthesis, Serine metabolism, Trans-Activators metabolism, Tumor Suppressor Proteins biosynthesis, Cellular Senescence physiology, Homeodomain Proteins physiology, Nuclear Proteins physiology, Receptors, Cytoplasmic and Nuclear physiology, Trans-Activators physiology, Tumor Suppressor Protein p53 metabolism, Tumor Suppressor Proteins physiology

Abstract

ING2 is a candidate tumor suppressor gene that can activate p53 by enhancing its acetylation. Here, we demonstrate that ING2 is also involved in p53-mediated replicative senescence. ING2 protein expression increased in late-passage human primary cells, and it colocalizes with serine 15-phosphorylated p53. ING2 and p53 also complexed with the histone acetyltransferase p300. ING2 enhanced the interaction between p53 and p300 and acted as a cofactor for p300-mediated p53 acetylation. The level of ING2 expression directly modulated the onset of replicative senescence. While overexpression of ING2 induced senescence in young fibroblasts in a p53-dependent manner, expression of ING2 small interfering RNA delayed the onset of senescence. Hence, ING2 can act as a cofactor of p300 for p53 acetylation and thereby plays a positive regulatory role during p53-mediated replicative senescence.

Published

2005

27. A quantitative determination of multi-protein interactions by the analysis of confocal images using a pixel-by-pixel assessment algorithm.

Author

Goucher DR, Wincovitch SM, Garfield SH, Carbone KM, and Malik TH

Subjects

Animals, Hippocampus metabolism, Hippocampus pathology, Measles pathology, Mice, Neurons pathology, Algorithms, Chemokine CCL5 metabolism, Image Interpretation, Computer-Assisted methods, Measles metabolism, Microscopy, Confocal methods, Neurons metabolism, Protein Interaction Mapping methods, Software

Abstract

Motivation: Recent advances in confocal microscopy have allowed scientists to assess the expression, and to some extent, the interaction/colocalization of multiple molecules within cells and tissues. In some instances, accurately quantifying the colocalization of two or more proteins may be critical. This can require the acquisition of multiple Z plane images (Z stacks) throughout a specimen and, as such, we report here the successful development of a freeware, open-source image analysis tool, IMAJIN&#95;COLOC, developed in PERL (v. 5.8, build 806), using the PERLMagick libraries (ImageMagick). Using a pixel-by-pixel analysis algorithm, IMAJIN&#95;COLOC can analyze images for antigen expression (any number of colors) and can measure all possible combinations of colocalization for up to three colors by analyzing a Z stack gallery acquired for each sample. The simultaneous (i.e. in a single pass) analysis of three-color colocalization, and batch analysis capabilities are distinctive features of this program., Results: A control image, containing known individual and colocalized pixel counts, was used to validate the accuracy of IMAJIN&#95;COLOC. As further validation, pixel counts and colocalization values from the control image were compared to those obtained with the software packaged with the Zeiss laser-scanning microscope (LSM AIM, version 3.2). The values from both programs were found to be identical. To demonstrate the applicability of this program in addressing novel biological questions, we examined the role of neurons in eliciting an immune reaction in response to viral infection. Specifically, we successfully examined expression of the chemokine RANTES in measles virus (MV) infected hippocampal neurons and quantified changes in RANTES production throughout the disease period. The resultant quantitative data were also evaluated visually, using a gif image created during the analysis., Availability: PERL (ActivePerl, version 5.8) is available at activestate.com; the PERLMagick libraries are available at imagemagick.org, and IMAJIN&#95;COLOC, the source code and user documentation can be downloaded from http://www.fda.gov/cber/research/imaging/imageanalysis.htm.

Published

2005

28. A novel diacylglycerol-lactone shows marked selectivity in vitro among C1 domains of protein kinase C (PKC) isoforms alpha and delta as well as selectivity for RasGRP compared with PKCalpha.

Author

Pu Y, Perry NA, Yang D, Lewin NE, Kedei N, Braun DC, Choi SH, Blumberg PM, Garfield SH, Stone JC, Duan D, and Marquez VE

Subjects

Animals, Binding Sites, Cell Line, Cell Membrane metabolism, DNA-Binding Proteins metabolism, Guanine Nucleotide Exchange Factors metabolism, Humans, Isoenzymes, Phorbol 12,13-Dibutyrate pharmacology, Phosphorylation drug effects, Protein Binding, Protein Kinase C chemistry, Protein Kinase C-alpha, Protein Kinase C-delta, Protein Transport, ras Guanine Nucleotide Exchange Factors, Diglycerides pharmacology, Lactones pharmacology, Protein Kinase C metabolism

Abstract

Although multiple natural products are potent ligands for the diacylglycerol binding C1 domain of protein kinase C (PKC), RasGRP, and related targets, the high conservation of C1 domains has impeded the development of selective ligands. We characterized here a diacylglycerol-lactone, 130C037, emerging from a combinatorial chemical synthetic strategy, which showed substantial selectivity. 130C037 gave shallow binding curves for PKC isoforms alpha, beta, gamma, delta, and epsilon, with apparent Ki values ranging from 340 nm for PKCalpha to 29 nm for PKCepsilon. When binding to isolated C1 domains of PKCalpha and -delta, 130C037 showed good affinity (Ki= 1.78 nm) only for deltaC1b, whereas phorbol 12,13-dibutyrate showed affinities within 10-fold for all. In LNCaP cells, 130C037 likewise selectively induced membrane translocation of deltaC1b. 130C037 bound intact RasGRP1 and RasGRP3 with Ki values of 3.5 and 3.8 nm, respectively, reflecting 8- and 90-fold selectivity relative to PKCepsilon and PKCalpha. By Western blot of Chinese hamster ovary cells, 130C037 selectively induced loss from the cytosol of RasGRP3 (ED50 = 286 nm), partial reduction of PKCepsilon (ED50 > 10 microm), and no effect on PKCalpha. As determined by confocal microscopy in LNCaP cells, 130C037 caused rapid translocation of RasGRP3, limited slow translocation of PKCepsilon, and no translocation of PKCalpha. Finally, 130C037 induced Erk phosphorylation in HEK-293 cells ectopically expressing RasGRP3 but not in control cells, whereas phorbol ester induced phosphorylation in both. The properties of 130C037 provide strong proof of principle for the feasibility of developing ligands with selectivity among C1 domain-containing therapeutic targets.

Published

2005

29. Analysis by fluorescence resonance energy transfer of the interaction between ligands and protein kinase Cdelta in the intact cell.

Author

Braun DC, Garfield SH, and Blumberg PM

Subjects

Animals, Apoptosis, Bacterial Proteins metabolism, Biological Transport, Blotting, Western, CHO Cells, Cell Line, Cell Membrane metabolism, Cricetinae, Cytosol metabolism, Dose-Response Relationship, Drug, Green Fluorescent Proteins metabolism, Humans, Kinetics, Ligands, Luminescent Proteins metabolism, Mice, Microscopy, Confocal, Models, Biological, Phorbol 12,13-Dibutyrate chemistry, Plasmids metabolism, Protein Binding, Protein Kinase C-delta, Protein Transport, Recombinant Proteins chemistry, Time Factors, Transfection, Fluorescence Resonance Energy Transfer methods, Protein Kinase C metabolism, Protein Kinase C physiology

Abstract

The role of the protein kinase C (PKC) family of serine/threonine kinases in cellular differentiation, proliferation, apoptosis, and other responses makes them attractive therapeutic targets. The activation of PKCs by ligands in vivo varies depending upon cell type; therefore, methods are needed to screen the potency of PKCs in this context. Here we describe a genetically encoded chimera of native PKCdelta fused to yellow- and cyan-shifted green fluorescent protein, which can be expressed in mammalian cells. This chimeric protein kinase, CY-PKCdelta, retains native or near-native activity in the several biological and biochemical parameters that we tested. Binding assays showed that CY-PKCdelta and native human PKCdelta have similar binding affinity for phorbol 12,13-dibutyrate. Analysis of translocation by Western blotting and confocal microscopy showed that CY-PKCdelta translocates from the cytosol to the membrane upon treatment with ligand, that the translocation has similar dose dependence as that of endogenous PKCdelta, and that the pattern of translocation is indistinguishable from that of the green fluorescent protein-PKCdelta fusion well characterized from earlier studies. Treatment with phorbol ester of cells expressing CY-PKCdelta resulted in a dose-dependent increase in FRET that could be visualized in situ by confocal microscopy or measured fluorometrically. By using this construct, we were able to measure the kinetics and potencies of 12 known PKC ligands, with respect to CY-PKCdelta, in the intact cell. The CY-PKCdelta chimera and the in vivo assays described here therefore show potential for high throughput screening of prospective PKCdelta ligands within the context of cell type.

Published

2005

30. Trafficking and localization of platinum complexes in cisplatin-resistant cell lines monitored by fluorescence-labeled platinum.

Author

Liang XJ, Shen DW, Chen KG, Wincovitch SM, Garfield SH, and Gottesman MM

Subjects

Antineoplastic Agents chemistry, Antineoplastic Agents pharmacology, Cell Fractionation, Cisplatin chemistry, Cisplatin pharmacology, Contrast Media metabolism, Golgi Apparatus metabolism, Humans, KB Cells drug effects, Microscopy, Fluorescence methods, Platinum chemistry, Triiodobenzoic Acids metabolism, Antineoplastic Agents metabolism, Cisplatin metabolism, Drug Resistance, Neoplasm, Fluorescent Dyes metabolism, Platinum metabolism

Abstract

Cisplatin is a chemotherapeutic agent commonly used in the treatment of a wide variety of malignant tumors. Resistance to cisplatin represents a major obstacle to effective cancer therapy because clinically significant levels of resistance quickly emerge after treatment. Based on previous studies indicating abnormal plasma membrane protein trafficking in cisplatin-resistant (CP-r) cells, Fluorescence (Alexa Fluor)-labeled cisplatin was used to determine whether this defect altered the trafficking and localization of cisplatin by comparing drug sensitive KB-3-1 and KB-CP-r cells. Alexa Fluor-cisplatin was readily internalized and localized throughout the KB-3-1 cells, but overall fluorescence decreased in KB-CP-r cells, as detected by flow cytometry (FACS) and confocal microscopy. Only punctate cytoplasmic staining was observed in KB-CP-r cells with less fluorescence observed in the nucleus. Colocalization experiments with a Golgi-selective stain indicate the involvement of Golgi-like vesicles in initial intracellular processing of Alexa Fluor conjugated cisplatin complexes. As detected using an antibody to Alexa Fluor-cisplatin, cisplatin complex-binding proteins (CCBPs) were reduced in membrane fractions of single-step cisplatin-resistant KB-CP.5 cells, and increased in the cytoplasm of KB-CP.5 cells compared to KB-3-1 cells. CCBPs localized to lower density fractions in KB-CP.5 cells than in KB-3-1 cells as determined by iodixanol gradient centrifugation. In summary, inappropriate trafficking of CCBPs might explain resistance to cisplatin in cultured cancer cells, presumably because membrane binding proteins for cisplatin are not properly located on the cell surface in these cells, but are instead trapped in low density vesicles within the cytoplasm., (2004 Wiley-Liss, Inc.)

Published

2005

31. Role of phorbol ester localization in determining protein kinase C or RasGRP3 translocation: real-time analysis using fluorescent ligands and proteins.

Author

Braun DC, Cao Y, Wang S, Garfield SH, Hur GM, and Blumberg PM

Subjects

Animals, Biological Transport, CHO Cells, Cricetinae, Fluorescent Dyes, Humans, Kinetics, Ligands, Microscopy, Confocal, Phorbol 12,13-Dibutyrate pharmacokinetics, Protein Transport, Recombinant Fusion Proteins metabolism, ras Guanine Nucleotide Exchange Factors, Guanine Nucleotide Exchange Factors metabolism, Phorbol 12,13-Dibutyrate pharmacology, Protein Kinase C metabolism, Tetradecanoylphorbol Acetate pharmacology

Abstract

The diacylglycerol signaling pathway, involving protein kinase C (PKC) and RasGRP, is a promising therapeutic target for both cancer and other indications. The phorbol esters, ultrapotent diacylglycerol analogues, bind to and activate PKC and RasGRP. Here, using fluorescent phorbol esters and complementary fluorescent PKC and RasGRP constructs, we determined the localization of the phorbol ester as a function of time after addition and how the resultant PKC or RasGRP3 translocation related to ligand localization. For these studies, we prepared fluorescently labeled phorbol esters of varying lipophilicities based on the BODIPY FL (green) or BODIPY 581/591 (red) fluorophores, and by using fusion constructs of green fluorescent protein or DsRed with PKC isoforms or RasGRP3 expressed in Chinese hamster ovary cells, we simultaneously compared the kinetics and pattern of localization of PKC or RasGRP3 with that of the fluorescent red or green phorbol esters. Binding assays showed that the fluorescent derivatives were potent ligands. Uptake followed a one-compartment pharmacokinetic model with a half-time of minutes to hours, depending on the ligand, and all of the fluorescent phorbol esters localized primarily to intracellular membranes, with little plasma membrane localization. The fluorescent phorbol esters induced translocation of and generally colocalized with PKCdelta or RasGRP3. However, PKCalpha and, initially, PKCdelta, translocated to the plasma membrane, in which little phorbol ester accumulated. The findings argue that the rate of uptake of phorbol esters influences the subsequent pattern of PKCdelta translocation, and that the specificity for PKCalpha translocation is dominated by factors other than the localization of the ligand.

Published

2005

32. PKCdelta associates with and is involved in the phosphorylation of RasGRP3 in response to phorbol esters.

Author

Brodie C, Steinhart R, Kazimirsky G, Rubinfeld H, Hyman T, Ayres JN, Hur GM, Toth A, Yang D, Garfield SH, Stone JC, and Blumberg PM

Subjects

Animals, Biological Transport, CHO Cells, Cricetinae, Electrophoresis, Female, Guanine Nucleotide Exchange Factors drug effects, Humans, Mitogen-Activated Protein Kinases metabolism, Phosphorylation drug effects, Protein Kinase C-delta, Serine metabolism, Transfection, ras Guanine Nucleotide Exchange Factors, Guanine Nucleotide Exchange Factors metabolism, Protein Kinase C metabolism, Tetradecanoylphorbol Acetate pharmacology

Abstract

RasGRP is a family of guanine nucleotide exchange factors that activate small GTPases and contain a C1 domain similar to the one present in protein kinase C (PKC). In this study, we examined the interaction of RasGRP3 and PKC in response to the phorbol ester PMA. In Chinese hamster ovary or LN-229 cells heterologously expressing RasGRP3, phorbol 12-myristate 13-acetate (PMA) induced translocation of RasGRP3 to the perinuclear region and a decrease in the electrophoretic mobility of RasGRP3. The mobility shift was associated with phosphorylation of RasGRP3 on serine residues and seemed to be PKCdelta-dependent because it was blocked by the PKCdelta inhibitor rottlerin as well as by a PKCdelta kinase-dead mutant. Using coimmunoprecipitation, we found that PMA induced the physical association of RasGRP3 with PKCdelta and, using in situ methods, we showed colocalization of PKCdelta and RasGRP3 in the perinuclear region. PKCdelta phosphorylated RasGRP3 in vitro. Previous studies suggest that ectopic expression of RasGRP3 increases activation of Erk1/2. We found that overexpression of either PKCdelta or RasGRP3 increased the activation of Erk1/2 by PMA. In contrast, coexpression of PKCdelta and RasGRP3 yielded a level of phosphorylation of Erk1/2 similar to that of control vector cells. Our results suggest that PKCdelta may act as an upstream kinase associating with and phosphorylating RasGRP3 in response to PMA. The interaction between RasGRP3 and PKCdelta points to the existence of complex cross-talk between various members of the phorbol ester receptors which can have important impact on major signal transduction pathways and cellular processes induced by phorbol esters or DAG

Published

2004

33. Characterization of the interaction of ingenol 3-angelate with protein kinase C.

Author

Kedei N, Lundberg DJ, Toth A, Welburn P, Garfield SH, and Blumberg PM

Subjects

Animals, CHO Cells, Cricetinae, Diterpenes chemistry, Diterpenes metabolism, Down-Regulation, Euphorbia chemistry, Humans, Interleukin-6 biosynthesis, Isoenzymes metabolism, Ligands, Liposomes chemistry, Tetradecanoylphorbol Acetate pharmacology, Diterpenes pharmacology, Protein Kinase C metabolism

Abstract

Ingenol 3-angelate (I3A) is one of the active ingredients in Euphorbia peplus, which has been used in traditional medicine. Here, we report the initial characterization of I3A as a protein kinase C (PKC) ligand. I3A bound to PKC-alpha in the presence of phosphatidylserine with high affinity; however, under these assay conditions, little PKC isoform selectivity was observed. PKC isoforms did show different sensitivity and selectivity for down-regulation by I3A and phorbol 12-myristate 13-acetate (PMA) in WEHI-231, HOP-92, and Colo-205 cells. In all of the three cell types, I3A inhibited cell proliferation with somewhat lower potency than did PMA. In intact CHO-K1 cells, I3A was able to translocate different green fluorescent protein-tagged PKC isoforms, visualized by confocal microscopy, with equal or higher potency than PMA. PKC-delta in particular showed a different pattern of translocation in response to I3A and PMA. I3A induced a higher level of secretion of the inflammatory cytokine interleukin 6 compared with PMA in the WEHI-231 cells and displayed a marked biphasic dose-response curve for the induction. I3A was unable to cause the same extent of association of the C1b domain of PKC-delta with lipids, compared with PMA or the physiological regulator diacylglycerol, and was able to partially block the association induced by these agents, measured by surface plasmon resonance. The in vitro kinase activity of PKC-alpha induced by I3A was lower than that induced by PMA. The novel pattern of behavior of I3A makes it of great interest for further evaluation.

Published

2004

34. Altered localization of retinoid X receptor alpha coincides with loss of retinoid responsiveness in human breast cancer MDA-MB-231 cells.

Author

Tanaka T, Dancheck BL, Trifiletti LC, Birnkrant RE, Taylor BJ, Garfield SH, Thorgeirsson U, and De Luca LM

Subjects

Adenoviridae genetics, Adenoviridae metabolism, Apoptosis, Breast Neoplasms pathology, Cell Line, Tumor, Epithelial Cells cytology, Epithelial Cells metabolism, Female, Gene Expression Regulation, Humans, Ligands, Mammary Glands, Human cytology, Mammary Glands, Human pathology, Receptors, Retinoic Acid genetics, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Retinoid X Receptors, Subcellular Fractions metabolism, Transcription Factors genetics, Transcription, Genetic, Antineoplastic Agents metabolism, Breast Neoplasms metabolism, Drug Resistance, Neoplasm, Receptors, Retinoic Acid metabolism, Retinoids metabolism, Transcription Factors metabolism

Abstract

To understand the mechanism of retinoid resistance, we studied the subcellular localization and function of retinoid receptors in human breast cancer cell lines. Retinoid X receptor alpha (RXR alpha) localized throughout the nucleoplasm in retinoid-sensitive normal human mammary epithelial cells and in retinoid-responsive breast cancer cell line (MCF-7), whereas it was found in the splicing factor compartment (SFC) of the retinoid-resistant MDA-MB-231 breast cancer cell line and in human breast carcinoma tissue. In MDA-MB-231 cells, RXR alpha was not associated with active transcription site in the presence of ligand. Similarly, ligand-dependent RXR homo- or heterodimer-mediated transactivation on RXR response element or RARE showed minimal response to ligand in MDA-MB-231 cells. Infecting MDA-MB-231 cells with adenoviral RXR alpha induced nucleoplasmic overexpression of RXR alpha and resulted in apoptosis upon treatment with an RXR ligand. This suggests that nucleoplasmic RXR alpha restores retinoid sensitivity. Epitope-tagged RXR alpha and a C-terminus deletion mutant failed to localize to the SFC. Moreover, RXR alpha localization to the SFC was inhibited with RXR alpha C-terminus peptide. This peptide also induced ligand-dependent transactivation on RXRE. Therefore, the RXR alpha C terminus may play a role in the intranuclear localization of RXR alpha. Our results provide evidence that altered localization of RXR alpha to the SFC may be an important factor for the loss of retinoid responsiveness in MDA-MB-231 breast cancer cells.

Published

2004

35. p53 interacts with hRAD51 and hRAD54, and directly modulates homologous recombination.

Author

Linke SP, Sengupta S, Khabie N, Jeffries BA, Buchhop S, Miska S, Henning W, Pedeux R, Wang XW, Hofseth LJ, Yang Q, Garfield SH, Stürzbecher HW, and Harris CC

Subjects

Cell Line, Cell Nucleus metabolism, DNA Helicases, DNA-Binding Proteins antagonists & inhibitors, DNA-Binding Proteins metabolism, Fibroblasts, Humans, Nuclear Proteins metabolism, Protein Binding, Protein Structure, Tertiary, Rad51 Recombinase, Tumor Suppressor Protein p53 deficiency, Tumor Suppressor Protein p53 metabolism, DNA-Binding Proteins physiology, Nuclear Proteins physiology, Recombination, Genetic physiology, Tumor Suppressor Protein p53 physiology

Abstract

p53 inhibits tumorigenesis through a variety of functions, including mediation of cell cycle arrest, premature senescence, and apoptosis.p53 also can associate with several DNA helicases and proteins involved in homologous recombination. In this study, we show that p53, hRAD51, and hRAD54 coimmunoprecipitated and colocalized with each other at endogenous levels in normal cells. Colocalization was observed with the phosphoserine-15 form of p53 at presumed DNA processing sites after the induction of DNA breaks. hRAD54 bound directly to the p53 COOH terminus in vitro without a nucleic acid intermediate. We then investigated the functional consequences of these protein interactions. A host cell reactivation assay revealed that the elevation in recombination observed after p53 inactivation is dependent on the hRAD51 pathway and that p53-dependent antirecombinogenic activity can be attributed to p53 binding to hRAD51 directly. These data support the hypothesis that p53 helps maintain genetic stability through transcription-independent modulation of homologous recombination factors.

Published

2003

36. BLM helicase-dependent transport of p53 to sites of stalled DNA replication forks modulates homologous recombination.

Author

Sengupta S, Linke SP, Pedeux R, Yang Q, Farnsworth J, Garfield SH, Valerie K, Shay JW, Ellis NA, Wasylyk B, and Harris CC

Subjects

Adenosine Triphosphatases genetics, Bloom Syndrome, Bromodeoxyuridine metabolism, Cell Cycle physiology, Cell Line, DNA Helicases genetics, DNA-Binding Proteins metabolism, Fibroblasts cytology, Fibroblasts metabolism, Humans, Hydroxyurea metabolism, Models, Genetic, Nuclear Proteins genetics, Nuclear Proteins metabolism, Phosphorylation, Protein Binding, Rad51 Recombinase, RecQ Helicases, Serine metabolism, Tumor Suppressor Protein p53 genetics, Active Transport, Cell Nucleus physiology, Adenosine Triphosphatases metabolism, DNA Helicases metabolism, DNA Replication, Recombination, Genetic, Tumor Suppressor Protein p53 metabolism

Abstract

Diverse functions, including DNA replication, recombination and repair, occur during S phase of the eukaryotic cell cycle. It has been proposed that p53 and BLM help regulate these functions. We show that p53 and BLM accumulated after hydroxyurea (HU) treatment, and physically associated and co-localized with each other and with RAD51 at sites of stalled DNA replication forks. HU-induced relocalization of BLM to RAD51 foci was p53 independent. However, BLM was required for efficient localization of either wild-type or mutated (Ser15Ala) p53 to these foci and for physical association of p53 with RAD51. Loss of BLM and p53 function synergistically enhanced homologous recombination frequency, indicating that they mediated the process by complementary pathways. Loss of p53 further enhanced the rate of spontaneous sister chromatid exchange (SCE) in Bloom syndrome (BS) cells, but not in their BLM-corrected counterpart, indicating that involvement of p53 in regulating spontaneous SCE is BLM dependent. These results indicate that p53 and BLM functionally interact during resolution of stalled DNA replication forks and provide insight into the mechanism of genomic fidelity maintenance by these nuclear proteins.

Published

2003

37. Iridals are a novel class of ligands for phorbol ester receptors with modest selectivity for the RasGRP receptor subfamily.

Author

Shao L, Lewin NE, Lorenzo PS, Hu Z, Enyedy IJ, Garfield SH, Stone JC, Marner FJ, Blumberg PM, and Wang S

Subjects

Acrolein analogs & derivatives, Acrolein metabolism, Acrolein pharmacology, Antineoplastic Agents, Phytogenic metabolism, Antineoplastic Agents, Phytogenic pharmacology, Binding, Competitive, Carrier Proteins, Cell Line, Crystallography, X-Ray, Cyclohexanols metabolism, Cyclohexanols pharmacology, Databases, Factual, Drug Screening Assays, Antitumor, Green Fluorescent Proteins, Guanine Nucleotide Exchange Factors genetics, Humans, Isoenzymes chemistry, Isoenzymes metabolism, Ligands, Luminescent Proteins genetics, Mitogen-Activated Protein Kinase 1 metabolism, Mitogen-Activated Protein Kinase 3, Mitogen-Activated Protein Kinases metabolism, Models, Molecular, Phosphorylation, Protein Kinase C chemistry, Protein Kinase C-alpha, Protein Kinase C-delta, Radioligand Assay, Recombinant Fusion Proteins metabolism, Spiro Compounds metabolism, Spiro Compounds pharmacology, Stereoisomerism, Terpenes pharmacology, Tumor Cells, Cultured, ras Guanine Nucleotide Exchange Factors, Acrolein chemistry, Antineoplastic Agents, Phytogenic chemistry, Caenorhabditis elegans Proteins, Cyclohexanols chemistry, Diterpenes, Guanine Nucleotide Exchange Factors metabolism, Iridaceae chemistry, Phorbols metabolism, Protein Kinase C metabolism, Receptors, Drug metabolism, Spiro Compounds chemistry

Abstract

Since 1990, the National Cancer Institute has performed extensive in vitro screening of compounds for anticancer activity. To date, more than 70 000 compounds have been screened for their antiproliferation activities against a panel of 60 human cancer cell lines. We probed this database to identify novel structural classes with a pattern of biological activity on these cell lines similar to that of the phorbol esters. The iridals form such a structural class. Using the program Autodock, we show that the iridals dock to the same position on the C1b domain of protein kinase C delta as do the phorbol esters, with the primary hydroxyl group of the iridal at the C3 position forming two hydrogen bonds with the amide group of Thr12 and with the carbonyl group of Leu 21 and the aldehyde oxygen of the iridal forming a hydrogen bond with the amide group of Gly23. Biological analysis of two iridals, NSC 631939 and NSC 631941, revealed that they bound to protein kinase C alpha with K(i) values of 75.6 +/- 1.3 and 83.6 +/- 1.5 nM, respectively. Protein kinase C is now recognized to represent only one of five families of proteins with C1 domains capable of high-affinity binding of diacylglycerol and the phorbol esters. NSC 631939 and NSC 631941 bound to RasGRP3, a phorbol ester receptor that directly links diacylglycerol/phorbol ester signaling with Ras activation, with K(i) values of 15.5 +/- 2.3 and 41.7 +/- 6.5 nM, respectively. Relative to phorbol 12,13-dibutyrate, they showed 15- and 6-fold selectivity for RasGRP3. Both compounds caused translocation of green fluorescent protein tagged RasGRP3 expressed in HEK293 cells, and both compounds induced phosphorylation of ERK1/2, a downstream indicator of Ras activation, in a RasGRP3-dependent fashion. We conclude that the iridals represent a promising structural motif for design of ligands for phorbol ester receptor family members.

Published

2001

38. An optimized protein kinase C activating diacylglycerol combining high binding affinity (Ki) with reduced lipophilicity (log P).

Author

Nacro K, Sigano DM, Yan S, Nicklaus MC, Pearce LL, Lewin NE, Garfield SH, Blumberg PM, and Marquez VE

Subjects

Animals, Binding Sites, Binding, Competitive, CHO Cells, Cricetinae, Databases as Topic, Diglycerides chemical synthesis, Enzyme Activation, Hydrogen Bonding, Kinetics, Models, Molecular, Molecular Conformation, Phorbol 12,13-Dibutyrate pharmacokinetics, Protein Conformation, Protein Structure, Secondary, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins metabolism, Structure-Activity Relationship, Transfection, Tryptophan, Tyrosine, Zinc Fingers, Diglycerides chemistry, Diglycerides pharmacology, Protein Kinase C chemistry, Protein Kinase C metabolism

Abstract

A small, focused combinatorial library encompassing all possible permutations of acyl branched alkyl chains-small and large, saturated and unsaturated-was generated from the active diacylglycerol enantiomer (S-DAG) to help identify the analogue with the highest binding affinity (lowest Ki) for protein kinase C (PK-C) combined with the minimum lipophilicity (log P). The selected ligand (3B) activated PK-C more effectively than sn-1,2-dioctanoylglycerol (diC8) despite being 1.4 log units more hydrophilic. Compound 3B indeed represents the most potent, hydrophilic DAG ligand to date. With the help of a green fluorescent protein (GFP)-tagged PK-Calpha, 3B was able to translocate the full length protein to the membrane with an optimal dose of 100 microM in CHO-K1 cells, while diC8 failed to achieve translocation even at doses 3-fold higher. Molecular modeling of 3B into an empty C1b domain of PK-Cdelta clearly showed the existence of a preferred binding orientation. In addition, molecular dynamic simulations suggest that binding discrimination could result from a favorable van der Waals (VDW) interaction between the large, branched sn-1 acyl group of 3B and the aromatic rings of Trp252 (PK-Cdelta) or Tyr252 (PK-Calpha). The DAG analogue of 3B in which the acyl groups are reversed (2C) showed a decrease in binding affinity reflecting the capacity of PK-C to effectively discriminate between alternative orientations of the acyl chains.

Published

2001

39. Phorbol esters modulate the Ras exchange factor RasGRP3.

Author

Lorenzo PS, Kung JW, Bottorff DA, Garfield SH, Stone JC, and Blumberg PM

Subjects

Amino Acid Sequence, Animals, Carcinogens metabolism, Carrier Proteins, Cell Line, Cell Membrane metabolism, Chromosome Mapping, Enzyme Activation, Humans, Kinetics, Mitogen-Activated Protein Kinase 1 metabolism, Mitogen-Activated Protein Kinase 3, Mitogen-Activated Protein Kinases metabolism, Molecular Sequence Data, Monomeric GTP-Binding Proteins metabolism, Phorbol Esters metabolism, Protein Kinase C metabolism, Protein Structure, Tertiary, Rats, Receptors, Drug metabolism, Sequence Homology, Amino Acid, Subcellular Fractions metabolism, Tetradecanoylphorbol Acetate metabolism, Tetradecanoylphorbol Acetate pharmacology, ras Guanine Nucleotide Exchange Factors, Caenorhabditis elegans Proteins, Carcinogens pharmacology, Guanine Nucleotide Exchange Factors metabolism, Phorbol Esters pharmacology

Abstract

RasGRP represents the prototype of a new class of guanine nucleotide exchange factors that activate small GTPases. The guanyl nucleotide-releasing protein (GRP) family members contain catalytic domains related to CDC25, the Ras exchange factor of Saccharomyces cerevisiae. They also contain a motif resembling a pair of calcium-binding EF-hands and a C1 domain similar to the diacylglycerol interaction domain of protein kinase C. The sequence of KIAA0846, identified in a human brain cDNA library, encodes a member of the GRP family that we refer to as RasGRP3. We show here that RasGRP3 bound phorbol esters with high affinity. This binding depended on anionic phospholipids, which is characteristic of phorbol ester binding to C1 domain proteins. In addition, phorbol esters also caused activation of the RasGRP3 exchange activity in intact cells, as determined by an increase in RasGTP and phosphorylation of the extracellular-regulated kinases. Finally, both phorbol 12-myristate 13-acetate and the diacylglycerol analogue 1,2-dioctanoyl-sn-glycerol induced redistribution of RasGRP3 to the plasma membrane and/or perinuclear area in HEK-293 cells, as demonstrated using a green fluorescent fusion protein. We conclude that RasGRP3 serves as a PKC-independent pathway to link the tumor-promoting phorbol esters with activation of Ras GTPases.

Published

2001

40. Phosphorylation of protein kinase Cdelta on distinct tyrosine residues regulates specific cellular functions.

Author

Kronfeld I, Kazimirsky G, Lorenzo PS, Garfield SH, Blumberg PM, and Brodie C

Subjects

Animals, Cell Division, Cloning, Molecular, Enzyme Inhibitors pharmacology, Genes, Dominant, Glutamate-Ammonia Ligase metabolism, Green Fluorescent Proteins, Immunoblotting, Luminescent Proteins metabolism, Mice, Microscopy, Confocal, Mutagenesis, Site-Directed, Phenylalanine chemistry, Phosphorylation, Platelet-Derived Growth Factor metabolism, Precipitin Tests, Protein Kinase C-delta, Protein Kinases metabolism, Protein Structure, Tertiary, Proto-Oncogene Proteins genetics, Proto-Oncogene Proteins metabolism, Proto-Oncogene Proteins c-fyn, Pyrazoles pharmacology, Pyrimidines pharmacology, Recombinant Fusion Proteins metabolism, Tetradecanoylphorbol Acetate pharmacology, Transfection, Tumor Cells, Cultured, Tyrosine chemistry, src-Family Kinases antagonists & inhibitors, Isoenzymes metabolism, Protein Kinase C metabolism, Tyrosine metabolism

Abstract

Protein kinase Cdelta (PKCdelta) inhibits proliferation and decreases expression of the differentiation marker glutamine synthetase (GS) in C6 glioma cells. Here, we report that distinct, specific tyrosine residues on PKCdelta are involved in these two responses. Transfection of cells with PKCdelta mutated at tyrosine 155 to phenylalanine caused enhanced proliferation in response to 12-phorbol 12-myristate 13-acetate, whereas GS expression resembled that for the PKCdelta wild-type transfectant. Conversely, transfection with PKCdelta mutated at tyrosine 187 to phenylalanine resulted in increased expression of GS, whereas the rate of proliferation resembled that of the PKCdelta wild-type transfectant. The tyrosine phosphorylation of PKCdelta and the decrease in GS expression induced by platelet-derived growth factor (PDGF) were abolished by the Src kinase inhibitors PP1 and PP2. In response to PDGF, Fyn associated with PKCdelta via tyrosine 187. Finally, overexpression of dominant negative Fyn abrogated the decrease in GS expression and reduced the tyrosine phosphorylation of PKCdelta induced by PDGF. We conclude that the tyrosine phosphorylation of PKCdelta and its association with tyrosine kinases may be an important point of divergence in PKC signaling.

Published

2000

41. Differential roles of the tandem C1 domains of protein kinase C delta in the biphasic down-regulation induced by bryostatin 1.

Author

Lorenzo PS, Bögi K, Hughes KM, Beheshti M, Bhattacharyya D, Garfield SH, Pettit GR, and Blumberg PM

Subjects

3T3 Cells, Animals, Binding Sites, Bryostatins, Down-Regulation, Isoenzymes biosynthesis, Isoenzymes chemistry, Isoenzymes genetics, Ligands, Macrolides, Mice, Mutagenesis, Site-Directed, Phorbol 12,13-Dibutyrate metabolism, Protein Conformation, Protein Kinase C biosynthesis, Protein Kinase C chemistry, Protein Kinase C genetics, Protein Kinase C-delta, Tritium, Antineoplastic Agents metabolism, Isoenzymes metabolism, Lactones metabolism, Protein Kinase C metabolism

Abstract

Bryostatin 1 (Bryo), currently in clinical trials, has been shown to induce a biphasic concentration-response curve for down-regulating protein kinase C (PKC) delta, with protection of the enzyme from down-regulation at high Bryo doses. In our ongoing studies to identify the basis for this unique behavior of PKCdelta, we examined the participation of the two ligand binding sites (C1a and C1b) in the regulatory domain of the enzyme. Three mutants of PKCdelta prepared by introducing a point mutation in either C1a or Clb or both C1a and Clb were overexpressed in NIH 3T3 cells. All of the constructs retained a biphasic response to down-regulation assessed after 24-h treatment with Bryo. However, the roles of the individual C1 domains were different for the two phases of the response. For down-regulation, both the C1a and the C1b mutants displayed equivalent 3-4-fold reductions in their affinities for the ligand. For protection from down-regulation, a reduced protection was observed for the C1a mutant, which showed a broader biphasic curve compared with those for wild-type PKCdelta and the Clb mutant. Like wild-type PKCdelta, all of the mutants showed the same subcellular partitioning of the protected enzyme to the particulate fraction of the cells, arguing against changes in sensitivity to Bryo due to differences in localization. Likewise, relatively similar patterns of localization were observed using green fluorescent protein-PKCdelta constructs. We conclude that the C1 domains of PKCdelta do not have equivalent roles in inducing protection against Bryo-induced down-regulation. The C1a domain plays a critical role in conferring the degree of protection at high concentrations of Bryo. Elucidation of the differential effect of Bryo on PKCdelta may suggest strategies for the design of novel ligands with Bryo-like activities.

Published

1999

42. Tissue inhibitor of metalloproteinases-1 (TIMP-1) binds to the cell surface and translocates to the nucleus of human MCF-7 breast carcinoma cells.

Author

Ritter LM, Garfield SH, and Thorgeirsson UP

Subjects

Amino Acid Sequence, Animals, Breast cytology, Breast Neoplasms pathology, CHO Cells, Coculture Techniques, Cricetinae, Endoplasmic Reticulum metabolism, Epithelial Cells, Golgi Apparatus metabolism, Green Fluorescent Proteins, Humans, Luminescent Proteins chemistry, Luminescent Proteins genetics, Luminescent Proteins metabolism, Microscopy, Confocal, Molecular Sequence Data, Molecular Weight, Protein Sorting Signals genetics, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Temperature, Tissue Inhibitor of Metalloproteinase-1 chemistry, Tissue Inhibitor of Metalloproteinase-1 genetics, Transfection, Tumor Cells, Cultured, Breast Neoplasms metabolism, Cell Membrane metabolism, Cell Nucleus metabolism, Tissue Inhibitor of Metalloproteinase-1 metabolism

Abstract

To study cellular and subcellular localization of TIMP-1, we constructed a cDNA which would express a chimeric protein, TIMP-1-EGFP, having the enhanced green fluorescent protein of the jelly fish Aequorea victoria fused to the carboxyl-terminus of TIMP-1. Chinese Hamster Ovary (CHO) cells were stably transfected with the TIMP-1-EGFP expressing plasmid. The secreted chimera was processed through the endoplasmic reticulum and Golgi, as was shown by fluorescent confocal microscopy after incubations at temperatures which block processing at the intermediate compartment and the trans-Golgi network. In a co-culture system, secreted TIMP-1-EGFP could be visualized binding to the surface of MCF-7 breast carcinoma cells but not non-neoplastic HBL-100 breast epithelial cells. TIMP-1-EGFP localized to the nucleus of MCF-7 cells after 72 hrs in co-culture. These findings suggest that TIMP-1 may preferentially bind to and be taken up by malignant breast epithelial cells and that TIMP-1 may play a yet unidentified role in nuclear functions., (Copyright 1999 Academic Press.)

Published

1999

43. Expression of epidermal growth factor receptor proto-oncogene mRNA in regenerating rat liver.

Author

Johnson AC, Garfield SH, Merlino GT, and Pastan I

Subjects

Actins genetics, Animals, DNA genetics, Hepatectomy, Kinetics, Male, Nucleic Acid Hybridization, Proto-Oncogene Mas, Rats, ErbB Receptors genetics, Liver Regeneration, Proto-Oncogenes, RNA, Messenger biosynthesis

Abstract

The expression of EGF receptor mRNAs in regenerating rat liver was measured using two nonoverlapping cDNA probes for the human gene from a highly conserved region. These probes (pE7 and pE62) both hybridized to RNA species of 10 and 6 kb. The 10 and 6 kb RNA species were shown to decrease in the first 12 hours after partial hepatectomy. However, significant increases above control levels were noted at 24h and 72h. The level of alpha-actin mRNA increased as has been previously reported. These results suggest that a transcriptional and/or a posttranscriptional regulatory mechanism exists in regenerating rat liver with respect to EGF receptor gene expression.

Published

1988