Your search keyword '"Cell Line, Transformed chemistry"' showing total 58 results

1. Polymorphisms in promoter sequences of the p15 ( INK4B ) and PTEN genes of normal Japanese individuals.

Author

Ohsaka Y, Yogosawa S, Nakanishi R, Sakai T, and Nishino H

Subjects

Base Sequence genetics, Cell Line, Transformed chemistry, Cyclin-Dependent Kinase Inhibitor p15 blood, Cyclin-Dependent Kinase Inhibitor p15 chemistry, DNA blood, DNA genetics, Genes, Reporter, Humans, Japan, Luciferases analysis, Molecular Sequence Data, Mutation genetics, PTEN Phosphohydrolase blood, PTEN Phosphohydrolase chemistry, Transcription Factors metabolism, Cyclin-Dependent Kinase Inhibitor p15 genetics, Cyclin-Dependent Kinase Inhibitor p15 metabolism, Gene Expression Regulation, PTEN Phosphohydrolase genetics, PTEN Phosphohydrolase metabolism, Polymorphism, Genetic, Promoter Regions, Genetic

Abstract

Gene promoter regions of p15(INK4B), a cyclin-dependent kinase inhibitor, and phosphatase and tensin homolog (PTEN), a dual-function protein and lipid phosphatase, interact with regulatory factors for gene transcription and methylation. Normal individuals exhibit sequence polymorphisms in these regulatory genes. We isolated genomic DNA from whole blood of healthy Japanese individuals and sequenced promoter regions of the p15 ( INK4B ) and PTEN genes. We also examined the influence of polymorphisms on promoter activity in several cell lines. We identified polymorphisms at positions -699, -394, and -242 and an insertion at position -320 in the p15 ( INK4B ) gene and a polymorphism at position -1142 in the PTEN gene. Reporter gene analysis revealed that these polymorphisms influenced transcriptional regulation in their cell lines. Our results indicate for the first time that promoter sequences of the p15 ( INK4B ) and PTEN genes differ among normal Japanese individuals and that promoter polymorphisms can influence gene transcription.

Published

2010

2. Survival of liver failure pigs by transplantation of reversibly immortalized human hepatocytes with Tamoxifen-mediated self-recombination.

Author

Totsugawa T, Yong C, Rivas-Carrillo JD, Soto-Gutierrez A, Navarro-Alvarez N, Noguchi H, Okitsu T, Westerman KA, Kohara M, Reth M, Tanaka N, Leboulch P, and Kobayashi N

Subjects

Animals, Biomarkers analysis, Cell Line, Transformed chemistry, Cell Line, Transformed cytology, Hepatocytes chemistry, Hepatocytes drug effects, Humans, Integrases genetics, Liver Failure pathology, Recombination, Genetic, Retroviridae genetics, Sus scrofa, Tamoxifen pharmacology, Treatment Outcome, Cell Line, Transformed transplantation, Hepatocytes transplantation, Liver Failure surgery

Abstract

Background/aims: Hepatocyte transplantation and bioartificial liver treatment are attractive alternatives to liver transplantation. The availability of well-characterized human hepatocyte lines facilitates such cell therapies., Methods: Human hepatocytes were immortalized with a retroviral vector SSR#197 expressing catalytic subunit of human telomerase reverse transcriptase (hTERT) and enhanced green fluorescent protein (EGFP) cDNAs flanked by a pair of loxP recombination targets. Then, Tamoxifen-dependent Cre recombinase was expressed in SSR#197-immortalized hepatocytes. Cre/LoxP recombination was performed in the established cells by simple exposure to 500 nM Tamoxifen for a week. Then, the reverted population of the cells was recovered by EGFP-negative cell sorting and characterized in vitro and in vivo using a pig model of acute liver failure (ALF) induced by d-galactosamine (0.5 g/kg) injection., Results: A human hepatocyte cell line 16T-3 was established. Reverted 16-T3 cells showed the increased expression of hepatic markers in association with enhanced levels of transcriptional factors. Compared to normal human hepatocytes, albumin production and lidocaine-metabolizing activities of reverted 16-T3 cells were 0.32 and 0.50-fold, respectively. Transplantation of reverted 16T-3 cells significantly prolonged the survival of ALF pigs., Conclusions: Here we demonstrate the usefulness of Cre/LoxP -mediated reversible immortalization of human hepatocytes with Tamoxifen-mediated self-recombination.

Published

2007

3. Nuclear-mitochondrial genomic profiling reveals a pattern of evolution in epithelial ovarian tumor stem cells.

Author

Wani AA, Sharma N, Shouche YS, and Bapat SA

Subjects

Adenocarcinoma, Papillary genetics, Adenocarcinoma, Papillary pathology, Amino Acid Substitution, Ascites genetics, Ascites pathology, CREB-Binding Protein genetics, Cell Line, Transformed chemistry, Cell Line, Transformed pathology, Cell Lineage, Cell Nucleus chemistry, Clone Cells chemistry, Clone Cells ultrastructure, Cystadenocarcinoma, Serous genetics, Cystadenocarcinoma, Serous pathology, Cystadenocarcinoma, Serous secondary, Cystadenoma genetics, Cystadenoma pathology, DNA Repair, Embryonal Carcinoma Stem Cells, Evolution, Molecular, Female, Genes, Tumor Suppressor, Germ-Line Mutation, Humans, Mutagenesis, Mutation, Missense, Neoplasm Proteins genetics, Neoplastic Stem Cells pathology, Point Mutation, DNA Mutational Analysis, DNA, Mitochondrial genetics, DNA, Neoplasm genetics, Gene Expression Profiling, Neoplastic Stem Cells metabolism, Ovarian Neoplasms pathology

Abstract

Analyses of genome orthologs in cancer on the background of tumor heterogeneity, coupled with the recent identification that the tumor propagating capacity resides within a very small fraction of cells (the tumor stem cells-TSCs), has not been achieved. Here, we describe a strategy to explore genetic drift in the mitochondrial genome accompanying varying stem cell dynamics in epithelial ovarian cancer. A major and novel outcome is the identification of a specific mutant mitochondrial DNA profile associated with the TSC lineage that is drastically different from the germ line profile. This profile, however, is often camouflaged in the primary tumor, and sometimes may not be detected even after metastases, questioning the validity of whole tumor profiling towards determining individual prognosis. Continuing mutagenesis in subsets with a mutant mitochondrial genome could result in transformation through a cooperative effect with nuclear genes - a representative example in our study is a tumor suppressor gene viz. cAMP responsive element binding binding protein. This specific profile could be a critical predisposing step undertaken by a normal stem cell to overcome a tightly regulated mutation rate and DNA repair in its evolution towards tumorigenesis. Our findings suggest that varying stem cell dynamics and mutagenesis define TSC progression that may clinically translate into increasing tumor aggression with serious implications for prognosis.

Published

2006

4. Simultaneous localization of MLL, AF4 and ENL genes in interphase nuclei by 3D-FISH: MLL translocation revisited.

Author

Gué M, Sun JS, and Boudier T

Subjects

Adolescent, Adult, Cell Line, Transformed chemistry, Cell Line, Transformed ultrastructure, Cell Line, Tumor chemistry, Cell Line, Tumor ultrastructure, Cell Nucleus ultrastructure, Chromosomes, Human, Pair 11 genetics, Chromosomes, Human, Pair 11 ultrastructure, Chromosomes, Human, Pair 19 genetics, Chromosomes, Human, Pair 19 ultrastructure, Chromosomes, Human, Pair 4 genetics, Chromosomes, Human, Pair 4 ultrastructure, HL-60 Cells chemistry, HL-60 Cells ultrastructure, Herpesvirus 4, Human, Histone-Lysine N-Methyltransferase, Humans, Interphase, Leukemia, Monocytic, Acute genetics, Leukemia, Monocytic, Acute pathology, Male, Models, Genetic, Multiple Myeloma pathology, Precursor B-Cell Lymphoblastic Leukemia-Lymphoma genetics, Precursor B-Cell Lymphoblastic Leukemia-Lymphoma pathology, Transcriptional Elongation Factors, Translocation, Genetic, Cell Nucleus chemistry, DNA-Binding Proteins genetics, Genes, Imaging, Three-Dimensional, In Situ Hybridization, Fluorescence methods, Myeloid-Lymphoid Leukemia Protein genetics, Neoplasm Proteins genetics, Nuclear Proteins genetics, Transcription Factors genetics

Abstract

Background: Haematological cancer is characterised by chromosomal translocation (e.g. MLL translocation in acute leukaemia) and two models have been proposed to explain the origins of recurrent reciprocal translocation. The first, established from pairs of translocated genes (such as BCR and ABL), considers the spatial proximity of loci in interphase nuclei (static "contact first" model). The second model is based on the dynamics of double strand break ends during repair processes (dynamic "breakage first" model). Since the MLL gene involved in 11q23 translocation has more than 40 partners, the study of the relative positions of the MLL gene with both the most frequent partner gene (AF4) and a less frequent partner gene (ENL), should elucidate the MLL translocation mechanism., Methods: Using triple labeling 3D FISH experiments, we have determined the relative positions of MLL, AF4 and ENL genes, in two lymphoblastic and two myeloid human cell lines., Results: In all cell lines, the ENL gene is significantly closer to the MLL gene than the AF4 gene (with P value < 0.0001). According to the static "contact first" model of the translocation mechanism, a minimal distance between loci would indicate a greater probability of the occurrence of t(11;19)(q23;p13.3) compared to t(4;11)(q21;q23). However this is in contradiction to the epidemiology of 11q23 translocation., Conclusion: The simultaneous multi-probe hybridization in 3D-FISH is a new approach in addressing the correlation between spatial proximity and occurrence of translocation. Our observations are not consistent with the static "contact first" model of translocation. The recently proposed dynamic "breakage first" model offers an attractive alternative explanation.

Published

2006

5. Genomic characterization of KIR2DL4 in families and unrelated individuals reveals extensive diversity in exon and intron sequences including a common frameshift variation occurring in several alleles.

Author

Gedil MA, Steiner NK, and Hurley CK

Subjects

Alleles, Amino Acid Motifs, Amino Acid Substitution, Cell Line, Transformed chemistry, Consanguinity, DNA Mutational Analysis, Exons genetics, Frameshift Mutation, Genotype, Humans, Introns genetics, Mutation, Missense, Phylogeny, Point Mutation, Polymerase Chain Reaction, Protein Structure, Tertiary, Receptors, KIR, Receptors, KIR2DL4, Repetitive Sequences, Nucleic Acid, Sequence Alignment, Sequence Analysis, DNA, Sequence Homology, Nucleic Acid, Receptors, Immunologic genetics

Abstract

The KIR2DL4 gene including a portion of exon 1 through exon 9 was sequenced from two families and eight cell lines from the International Histocompatibility Workshop (IHWS). Two known alleles and eight variants were detected. Overall, there were five synonymous and three non-synonymous changes when the variants were compared to the coding sequences of the most closely related known alleles plus a common frameshift change in five of the variant alleles. Alignment of the new variants with all known alleles showed that the regions encoding the extracellular region and the cytoplasmic tail were the most polymorphic. Two non-synonymous changes, P146H and L161V, occurred in an extracellular immunoglobulin-like domain. Five of the eight variants had a single adenine deletion in the exon encoding the transmembrane region, potentially resulting in a truncated protein lacking the cytoplasmic tail. The distribution of the deletion variant among many KIR2DL4 alleles may explain the high frequency of this variation in the population. Four of the eight consanguineous IHWS cell lines were found to be heterozygous for KIR2DL4 carrying two alleles that differed from one another by a few nucleotide substitutions. Analysis of intron sequences in the families revealed the nature and distribution of interspersed repeat elements which comprise 46% of the KIR2DL4 nucleotide sequence and consist of 12 elements including six SINEs (13.73% of the total length), one LINE (12.41%), and five LTR elements (19.51%). The results revealed the presence of extensive diversity in the KIR2DL4 gene. This is the first extensive report providing both exon and intron data in related individuals.

Published

2005

6. Heterologous expression in Tritrichomonas foetus of functional Trichomonas vaginalis AP65 adhesin.

Author

Kucknoor AS, Mundodi V, and Alderete JF

Subjects

Animals, Antibodies, Monoclonal, Cell Adhesion genetics, Cell Adhesion Molecules physiology, Cell Fractionation methods, Cell Line, Transformed chemistry, Cell Membrane chemistry, DNA, Recombinant, Female, Humans, Immunoblotting, Microscopy, Fluorescence methods, Plasmids genetics, Protein Transport, Protozoan Proteins physiology, Transfection, Trichomonas vaginalis physiology, Tritrichomonas foetus genetics, Vagina cytology, Cell Adhesion Molecules genetics, Epithelial Cells parasitology, Gene Expression, Protozoan Proteins genetics, Trichomonas vaginalis genetics, Vagina parasitology

Abstract

Background: Trichomonosis, caused by Trichomonas vaginalis, is the number one, nonviral sexually transmitted infection that has adverse consequences for the health of women and children. The interaction of T. vaginalis with vaginal epithelial cells (VECs), a step preparatory to infection, is mediated in part by the prominent surface protein AP65. The bovine trichomonad, Tritrichomonas foetus, adheres poorly to human VECs. Thus, we established a transfection system for heterologous expression of the T. vaginalis AP65 in T. foetus, as an alternative approach to confirm adhesin function for this virulence factor., Results: In this study, we show stable transfection and expression of the T. vaginalis ap65 gene in T. foetus from an episomal pBS-ap65-neo plasmid. Expression of the gene and protein was confirmed by RT-PCR and immunoblots, respectively. AP65 in transformed T. foetus bound to host cells. Specific mAbs revealed episomally-expressed AP65 targeted to the parasite surface and hydrogenosome organelles. Importantly, surface-expression of AP65 in T. foetus paralleled increased levels of adherence of transfected bovine trichomonads to human VECs., Conclusion: The T. vaginalis AP65 adhesin was stably expressed in T. foetus, and the data obtained using this heterologous system strongly supports the role of AP65 as a prominent adhesin for T. vaginalis. In addition, the heterologous expression in T. foetus of a T. vaginalis gene offers an important, new approach for confirming and characterizing virulence factors.

Published

2005

7. Proteomic analysis of androgen-regulated protein expression in a mouse fetal vas deferens cell line.

Author

Umar A, Luider TM, Berrevoets CA, Grootegoed JA, and Brinkmann AO

Subjects

Animals, Cell Line, Transformed chemistry, Cell Line, Transformed physiology, Cell Lineage physiology, DNA-Binding Proteins analysis, DNA-Binding Proteins genetics, Female, Gene Expression Regulation, Developmental drug effects, LIM Domain Proteins, Male, Mice, Mice, Inbred CBA, Mice, Transgenic, Pregnancy, Receptors, Androgen genetics, Repressor Proteins analysis, Repressor Proteins genetics, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Stromal Cells cytology, Transcription Factors analysis, Transcription Factors genetics, Vas Deferens cytology, Androgens pharmacology, Heterogeneous-Nuclear Ribonucleoprotein Group A-B, Proteomics, Receptors, Androgen analysis, Vas Deferens embryology, Vas Deferens physiology

Abstract

During sex differentiation, androgens are essential for development of the male genital tract. The Wolffian duct is an androgen-sensitive target tissue that develops into the epididymis, vas deferens, and seminal vesicle. The present study aimed to identify androgen-regulated proteins that are involved in development of Wolffian duct-derived structures. We have used male mouse embryos transgenic for temperature-sensitive simian virus 40 large tumor antigen at 18 d of gestation, to generate immortalized mouse fetal vas deferens (MFVD) parental and clonal cell lines. The MFVD parental and clonal cell lines express androgen receptor protein and show features of Wolffian duct mesenchymal cells. Clonal cell line MFVD A6 was selected for proteomic analysis and cultured in the absence or presence of androgens. Subsequently, two-dimensional gel electrophoresis was performed on total cell lysates. Differentially expressed proteins were analyzed by matrix-assisted laser desorption/ionization time-of-flight mass spectrometry and two androgen-regulated proteins were identified as mElfin and CArG-binding factor-A (CBF-A). CBF-A and mElfin are known to bind to cytoskeletal F-actin. Both proteins appeared to be regulated by androgens at the posttranslational level, possibly involving phosphorylation. Posttranslational modification of mElfin and CBF-A by androgens may be associated with a cytoskeletal change that is involved in androgen-regulated gene expression.

Published

2003

8. Hyposialated 185 kDa CD45RA+ molecules attain a high concentration in B lymphoma cells and in activated human B cells.

Author

Yu Y, Rabinowitz R, Polliack A, Ben-Bassat H, and Schlesinger M

Subjects

Antigens, Neoplasm analysis, B-Lymphocytes immunology, Cell Line, Transformed chemistry, Cell Transformation, Viral, Glycoside Hydrolases pharmacology, Glycosylation drug effects, Herpesvirus 4, Human, Humans, Leukemia, Lymphocytic, Chronic, B-Cell metabolism, Leukemia, T-Cell metabolism, Leukocyte Common Antigens analysis, Molecular Weight, Neuraminidase pharmacology, Plasmacytoma chemistry, Protein Processing, Post-Translational drug effects, T-Lymphocytes chemistry, Trypsin pharmacology, Tumor Cells, Cultured chemistry, Tunicamycin pharmacology, Antigens, Neoplasm chemistry, B-Lymphocytes chemistry, Leukocyte Common Antigens chemistry, Lymphocyte Activation, Lymphoma, B-Cell chemistry, N-Acetylneuraminic Acid analysis

Abstract

Alternate splicing of exons of the CD45 molecule generates multiple isoforms differing in their molecular weights (MWs). In B-lymphocytes the CD45RA isoform was previously shown to be expressed on glycoproteins with MWs of 220 and 205 kDa, while the CD45RO isoform was expressed on glycoproteins with MW of 180 kDa. The present study demonstrated that B cell lymphomas and activated B-cells contain CD45 molecules with a MW of 185 kDa that express the CD45RA and CD45RC specificities but neither the CD45RB nor the CD45RO specificities. 185 kDa CD45RA+ molecules were detected in B cell lymphoma B lines, in Epstein-Barr virus (EBV)-transformed lymphoblastoid cell lines, and in tonsillar B cells, but not in normal, unstimulated peripheral blood B cells. These molecules were not detected in neoplastic and normal T cells. CD45RA+ 185 kDa molecules were present in B cells from three non-Hodgkin's patients in leukemic phase were not detected in B lymphocytes of seven of nine CLL patients tested. Trypsin treatment eliminated only 220 kDa CD45RA+ molecules but not 185 kDa CD45RA+ molecules, indicating that the 185 kDa CD45RA+ molecules are not expressed on the cell surface. Pulse-chase experiments, and studies on the effects of tunicamycin, neuraminidase and O-glycosidase, indicated that the 185 kDa molecules are partially glycosylated CD45RABC molecules that constitute precursors of the 220 kDa molecules. The high concentration of 185 kDa CD45RA+ molecules in B lymphoma cells and in activated B cells seems to reflect a high turnover of CD45RA+ molecules characteristic for these cells.

Published

2002

9. Characterization of a transformed rat retinal ganglion cell line.

Author

Krishnamoorthy RR, Agarwal P, Prasanna G, Vopat K, Lambert W, Sheedlo HJ, Pang IH, Shade D, Wordinger RJ, Yorio T, Clark AF, and Agarwal N

Subjects

Animals, Animals, Newborn, Antibodies, Monoclonal, Antigens, Surface analysis, Antigens, Surface immunology, Apoptosis drug effects, Apoptosis physiology, Biomarkers, Brain-Derived Neurotrophic Factor genetics, Brain-Derived Neurotrophic Factor pharmacology, Cell Culture Techniques methods, Cell Differentiation drug effects, Cell Differentiation physiology, Cell Line, Transformed chemistry, Culture Media, Serum-Free pharmacology, DNA-Binding Proteins analysis, DNA-Binding Proteins immunology, GPI-Linked Proteins, Glaucoma pathology, Glial Fibrillary Acidic Protein analysis, Glial Fibrillary Acidic Protein genetics, Glial Fibrillary Acidic Protein immunology, Glutamic Acid toxicity, In Situ Nick-End Labeling, Nerve Growth Factors genetics, Nerve Growth Factors pharmacology, Nerve Tissue Proteins analysis, Nerve Tissue Proteins immunology, Neuropeptides genetics, Neuroprotective Agents metabolism, Neuroprotective Agents pharmacology, Rats, Receptors, GABA-B genetics, Retinal Ganglion Cells chemistry, Synaptophysin genetics, Syntaxin 1, Thy-1 Antigens analysis, Thy-1 Antigens genetics, Thy-1 Antigens immunology, Transcription Factor Brn-3, Transcription Factor Brn-3C, Transcription Factors analysis, Transcription Factors immunology, Cell Line, Transformed cytology, Retinal Ganglion Cells cytology

Abstract

The purpose of the present study was to establish a rat retinal ganglion cell line by transformation of rat retinal cells. For this investigation, retinal cells were isolated from postnatal day 1 (PN1) rats and transformed with the psi2 E1A virus. In order to isolate retinal ganglion cells (RGC), single cell clones were chosen at random from the transformed cells. Expression of Thy-1 (a marker for RGC), glial fibrillary acidic protein (GFAP, a positive marker for Muller cells), HPC-1/syntaxin (a marker for amacrine cells), 8A1 (a marker for horizontal and ganglion cells) and neurotrophins was studied using reverse transcriptase-polymerase chain reaction (RT-PCR), immunoblotting and immunocytochemistry. One of the retinal cell clones, designated RGC-5, was positive for Thy-1, Brn-3C, Neuritin, NMDA receptor, GABA-B receptor, and synaptophysin expression and negative for GFAP, HPC-1, and 8A1, suggesting that it represented a putative RGC clone. The results of RT-PCR analysis were confirmed by immunocytochemistry for Thy-1 and GFAP. Upon further characterization by immunoblotting, the RGC-5 clone was positive for Thy-1, negative for GFAP, 8A1 and syntaxin. RGC 5 cells were also positive for the expression of neurotrophins and their cognate receptors. To establish the physiological relevance of RGC-5, the effects of serum/trophic factor deprivation and glutamate toxicity were analyzed to determine if these cells would undergo apoptosis. The protective effects of neurotrophins on RGC-5 after serum deprivation was also investigated. Apoptosis was studied by terminal deoxynucleotidyl transferase-mediated fluoresceinated dUTP nick end labeling (TUNEL). Serum deprivation resulted in apoptosis and supplementation with both BDNF and NT-4 in the growth media, protected the RGC-5 cells from undergoing apoptosis. On differentiation with succinyl concanavalin A (sConA), RGC-5 cells became sensitive to glutamate toxicity, which could be reversed by inclusion of ciplizone (MK801). In conclusion, a transformed rat retinal cell line, RGC-5, has certain characteristics of retinal ganglion cells based on Thy-1 and Brn-3C expression and its sensitivity to glutamate excitotoxicity and neurotrophin withdrawal. These cells may be valuable in understanding of retinal ganglion cell biology and physiology including in vitro manipulations in experimental models of glaucoma.

Published

2001

10. BAP37 and Prohibitin are specifically recognized by an SV40 T antigen antibody.

Author

Darmon AJ and Jat PS

Subjects

3T3 Cells, Animals, Antigen-Antibody Complex chemistry, Antigens, Polyomavirus Transforming immunology, Blotting, Western, Cell Line, Transformed chemistry, Epitopes immunology, Mice, Precipitin Tests, Prohibitins, Sequence Analysis, Protein, Antibodies, Monoclonal metabolism, Antibody Specificity, Antigens, Viral, Tumor immunology, Proteins immunology, Repressor Proteins

Abstract

We have identified two cellular proteins that are specifically immunoprecipitated by an anti-SV40 T antigen monoclonal antibody. This antibody, PAb419, recognizes an epitope contained within a region of T antigen which we have recently demonstrated is required for the initiation of immortalization by SV40 T antigen, but is not essential for maintenance of the immortal state. The two proteins were identified as BAP37 and Prohibitin. Recent results suggest Prohibitin may enhance the transcriptional inactivation of E2F by the retinoblastoma family of pocket proteins (pRb, p107, p130). BAP37 and Prohibitin are specifically recognized by PAb419 and PAb210, another anti-SV40 T antigen monoclonal antibody, which has an overlapping epitope, but not by other anti-SV40 T antigen monoclonal antibodies, demonstrating the specificity of the interaction., (Copyright 2001 Academic Press.)

Published

2000

11. Receptor-mediated endocytosis of transthyretin by ependymoma cells.

Author

Kuchler-Bopp S, Dietrich JB, Zaepfel M, and Delaunoy JP

Subjects

Animals, Biological Transport physiology, Blotting, Northern, Cell Line, Transformed chemistry, Cell Line, Transformed metabolism, Cell Line, Transformed ultrastructure, Ependyma cytology, Gene Expression Regulation, Neoplastic, Humans, Iodine Radioisotopes, Mice, Mice, Transgenic, Microscopy, Electron, Prealbumin genetics, RNA, Messenger analysis, Rats, Receptors, Albumin analysis, Receptors, Albumin metabolism, Brain Neoplasms, Endocytosis physiology, Ependymoma, Prealbumin pharmacokinetics

Abstract

Transthyretin (TTR) is involved in the transport of thyroxine (T4) and retinol-binding protein (RBP) in cerebrospinal fluid (CSF) and serum. TTR is secreted in the CSF by the epithelial cells of choroid plexus. The binding of [(125)I]TTR to cultured ependymoma cells which form the brain cerebrospinal barrier, was studied to determine whether these cells carry receptor(s) for TTR. TTR was bound by ependymoma cells in a time-dependent manner reaching equilibrium within 2 h. Scatchard analysis was consistent with a single class of high-affinity binding sites with a K(d) of approximately 18 nM. Saturable high-affinity binding of human TTR has previously been described in rat primary hepatocytes and human renal adenocarcinoma, neuroblastoma, hepatoma and astrocytoma cells, and also transformed lung cells. Endocytosis of fluorescent or biotinylated TTR was observed in ependymoma cells in cytoplasmic vesicles but TTR did not colocalize with clathrin in endocytic coated vesicles. Endocytosis of TTR was inhibited by high sucrose concentration (0.45 M). Finally, ligand blotting and chemical-linking experiments revealed the presence of a approximately 100 kDa putative TTR receptor on the ependymoma cell membrane. Receptor binding of TTR provides a potential mechanism for the delivery of T4 within the central nervous system.

Published

2000

12. Immortalisation of human bone marrow endothelial cells: characterisation of new cell lines.

Author

Rood PM, Calafat J, von dem Borne AE, Gerritsen WR, and van der Schoot CE

Subjects

Antigens, CD34 analysis, Bone Marrow Cells chemistry, Bone Marrow Cells metabolism, Cell Line, Transformed chemistry, Cell Line, Transformed metabolism, Cell Line, Transformed ultrastructure, DNA analysis, E-Selectin metabolism, Endothelium, Vascular chemistry, Endothelium, Vascular metabolism, Flow Cytometry, Hematopoietic Stem Cells chemistry, Hematopoietic Stem Cells metabolism, Hematopoietic Stem Cells ultrastructure, Humans, Immunophenotyping, Intercellular Adhesion Molecule-1 metabolism, Microscopy, Electron, Umbilical Veins cytology, Vascular Cell Adhesion Molecule-1 metabolism, Bone Marrow Cells ultrastructure, Cell Culture Techniques methods, Endothelium, Vascular ultrastructure

Abstract

Background: Adhesion of haematopoietic progenitor cells (HPC) to human bone marrow endothelial cells (HBMEC) plays a key role in homing of HPC to bone marrow. Here we describe four new HBMEC cell lines that can be used to study the (specific) adhesion of HPC to HBMEC., Design: HBMEC were immortalised with a retroviral construct containing the human papilloma virus 16 E6/E7 genes. Four cell lines were characterised., Results: The cell lines showed their endothelial nature by the expression of von Willebrand Factor and VE-cadherin (CD144). Electron microscopic analysis revealed normal endothelial-cell characteristics, including the presence of Weibel-Palade bodies and intercellular junction structures. An extensive phenotypic analysis of the cell-lines was performed, they were found to resemble primary HBMEC. The only difference found was the absence of expression of E-selectin (CD62e) and VCAM-1 (CD106) on resting HBMEC cell lines. Upon stimulation with IL-1beta the expression of E-selectin, VCAM-1 and ICAM-1 (CD54) was upregulated. All resting cell lines bound CD34+ HPC. Adhesion was increased by addition of the phorbol ester PMA. Two cell lines showed increased binding upon IL-1beta prestimulation. Highest adhesion was observed after the combination of IL-1beta prestimulation of the endothelial cells and addition of PMA. Binding of CD34+ HPC to HBMEC was compared with the binding to human umbilical vein endothelial cell lines and to a human dermal microvascular endothelial cell line (HMEC-1). So far, we have only found relatively less binding of HPC to IL-1beta prestimulated HMEC-1 cells, which could be explained by a reduced induction of E-selectin and VCAM-1 upon IL-1beta stimulation of these cells., Conclusion: The immortalised HBMEC cell lines have maintained their normal phenotype for the majority of characteristics examined. The expression of E-selectin and VCAM-1, which are not constitutively expressed on the cell lines, can be induced by stimulation of the endothelial cells with IL-1beta. The cell lines have furthermore maintained their capability to bind HPC. They will therefore be useful to investigate the interactions between HPC and HBMEC involved in homing of HPC.

Published

2000

13. Enzymatic amplification staining for flow cytometric analysis of cell surface molecules.

Author

Kaplan D and Smith D

Subjects

Annexin A5 analysis, Annexin A5 immunology, Antibodies, Monoclonal, Antigens, CD analysis, Antigens, CD immunology, Antigens, CD34 analysis, Antigens, CD34 immunology, Antigens, CD7 analysis, Antigens, CD7 immunology, Antigens, Differentiation, T-Lymphocyte analysis, Antigens, Differentiation, T-Lymphocyte immunology, Apoptosis, CD3 Complex analysis, CD3 Complex immunology, CD4 Antigens analysis, CD4 Antigens immunology, CD5 Antigens analysis, CD5 Antigens immunology, Cell Line, Transformed chemistry, Cell Line, Transformed cytology, Fas Ligand Protein, Histocompatibility Antigens Class I analysis, Histocompatibility Antigens Class I immunology, Histocompatibility Antigens Class II analysis, Histocompatibility Antigens Class II immunology, Humans, Jurkat Cells, Leukocyte Common Antigens analysis, Leukocyte Common Antigens immunology, Leukocytes, Mononuclear chemistry, Membrane Glycoproteins analysis, Membrane Glycoproteins immunology, Phosphatidylserines analysis, Phosphatidylserines immunology, Sensitivity and Specificity, Antigens, Surface analysis, Clinical Enzyme Tests methods, Flow Cytometry methods

Abstract

Background: Flow cytometric analysis is a powerful technique for the single cell assessment of cell surface expression of selected molecules. The major deficiency of flow cytometry has been its relative insensitivity. Only molecules expressed in abundance have been readily observed., Methods: We have developed an enzymatic amplification procedure for the analysis of cell surface molecules by flow cytometry. Transformed and nontransformed cells expressing MHC class I, CD5, CD3, CD4, CD6, CD7, CD34, CD45, MHC class II, Fas ligand, and phosphatidylserine were assessed., Results: Our enzymatic amplification technology increased the fluorescence signal between 10 and 100-fold for all surface molecules tested., Conclusions: Enzymatic amplification staining produces a significant enhancement in the resolving power of flow cytometric analysis of cell surface molecules. Using this technique, we have been able to detect the presence of molecules that could not be observed by the standard procedure., (Copyright 2000 Wiley-Liss, Inc.)

Published

2000

14. Modulation of G-protein linked cAMP accumulation in immortalized murine cortical astrocytes by retroviral infection.

Author

Raofi S, Wong PK, and Wilcox RE

Subjects

Adenylyl Cyclases metabolism, Adrenergic beta-Agonists pharmacology, Adrenergic beta-Antagonists pharmacology, Animals, Astrocytes cytology, Astrocytes metabolism, Biological Transport drug effects, Biological Transport physiology, Cell Line, Transformed chemistry, Cell Line, Transformed enzymology, Cell Line, Transformed virology, Colforsin pharmacology, Isoproterenol pharmacology, Mice, Neocortex cytology, Propranolol pharmacology, Receptors, Adrenergic, beta metabolism, Astrocytes virology, Cyclic AMP metabolism, GTP-Binding Proteins metabolism, Leukemia, Experimental metabolism, Moloney murine leukemia virus, Retroviridae Infections metabolism, Tumor Virus Infections metabolism

Abstract

The present study characterized beta-adrenergic receptors (beta-AR) in a clonal cell line (C1) immortalized from cerebral cortical astroglial cells of FVB/N mice. We also determined whether the wild type Moloney murine leukemia virus (wt-MoMuLV) and one of its neuropathogenic mutants, ts1-MoMuLV, modulated the beta-AR system in these cells. We observed that C1 cells possess a functional beta-AR system coupled to cAMP accumulation and capable of normal agonist-induced regulation (desensitization). Significant increases were observed in forskolin stimulated cAMP accumulation in C1 cells infected by wt MoMuLV and by ts1-MoMuLV. In contrast, the cAMP response to beta-AR stimulated by isoproterenol was relatively spared after viral exposure.

Published

2000

15. A subset of cells expressing SV40 large T antigen contain elevated p53 levels and have an altered cell cycle phenotype.

Author

Sladek TL, Laffin J, Lehman JM, and Jacobberger JW

Subjects

3T3 Cells, Animals, Antigens, Polyomavirus Transforming genetics, Cell Line, Transformed chemistry, Cell Line, Transformed cytology, Cell Line, Transformed virology, DNA analysis, Flow Cytometry, Fluorescent Antibody Technique, Gene Expression Regulation, Viral, Immunoblotting, Immunophenotyping, Mice, Tumor Suppressor Protein p53 genetics, Antigens, Polyomavirus Transforming analysis, Cell Cycle physiology, Tumor Suppressor Protein p53 analysis

Abstract

Cells transformed by the simian virus 40 (SV40) large T antigen (Tag) contain elevated levels of cellular p53 protein. To quantify this relationship, levels of p53 were measured in NIH 3T3 cells that expressed different concentrations of Tag. Using immunoblotting, average p53 levels were shown to increase linearly with Tag concentrations in these cell lines. Single-cell measurements were also performed using flow cytometry to measure p53 immunofluorescence. Surprisingly, the flow cytometry experiments showed that two distinct cell populations, based on p53 content, were present in cells expressing high levels of Tag. One cell population contained elevated p53 levels. A second population did not contain elevated p53, even though high concentrations of Tag were present in the cells. This latter cell population did not appear to arise because of mutations in either Tag or p53. The two cell populations also had phenotypic differences. In exponentially growing cells, Tag alters the cell cycle distribution (decreases the percentage of G1 phase cells and increases the percentages of S and G2 + M phase cells). This phenotype was maximum in the cell population containing elevated p53. A lesser phenotype was found in the cell population that did not contain elevated p53. These data show, firstly, that cells can express significant levels of Tag and not contain elevated levels of p53 and, secondly, that elevated p53 correlates with the altered cell cycle distribution produced by Tag in growing cells.

Published

2000

16. Characterization of immortalized human umbilical and iliac vein endothelial cell lines after transfection with SV40 large T-antigen.

Author

van Leeuwen EB, Veenstra R, van Wijk R, Molema G, Hoekstra A, Ruiters MH, and van der Meer J

Subjects

Biomarkers, Cell Culture Techniques, Cell Line, Transformed chemistry, Cloning, Organism, Endothelium, Vascular chemistry, Enzyme-Linked Immunosorbent Assay, Flow Cytometry, Humans, Iliac Vein chemistry, Immunohistochemistry, Plasminogen Activator Inhibitor 1 analysis, Platelet Endothelial Cell Adhesion Molecule-1 analysis, Reverse Transcriptase Polymerase Chain Reaction, Thromboplastin analysis, Tissue Plasminogen Activator analysis, Transfection, Umbilical Veins chemistry, von Willebrand Factor analysis, Antigens, Polyomavirus Transforming pharmacology, Endothelium, Vascular cytology, Iliac Vein cytology, Umbilical Veins cytology

Abstract

Most in vitro studies of human endothelial cells have relied on cells derived from human umbilical veins (HUVEC); however, heterogeneity of primary cultured endothelial cells can make critical interpretation of results difficult. Several endothelial cell lines have been produced to serve as a more constant source of endothelial cells. In this study, we characterized the endothelial cell lines EVLB3 and EVLC2 derived from HUVEC, and EVLK1 and EVLK2 derived from human iliac vein endothelial cells (HIVEC). These cell lines maintained the typical endothelial cell cobblestone morphology and appeared to be growth factor independent. They lost PECAM-1 and von Willebrand factor, GP96 was reduced to the level of vascular smooth muscle cells (SMC), but aSMC-actin was far less than in vascular SMC. Antigen levels of tissue-type plasminogen activator (tPA) and plasminogen activator inhibitor (PAI-1) were comparable with young endothelial cells, and mRNA was present for tPA, PAI-1, tissue factor (TF), tissue factor pathway inhibitor and thrombomodulin. This study revealed that mRNA and protein expression of coagulation and fibrinolytic factors was influenced by the stage of cell confluence. No differences could be detected between the endothelial cell lines derived from HUVEC and HIVEC. These cell lines may be a useful tool for studies on cellular interactions of fibrinolytic components or exploring the regulation of TF expression.

Published

2000

17. Forced MyHCIIB expression following targeted genetic manipulation of conditionally immortalized muscle precursor cells.

Author

Harris JM, Morgan JE, Rosenblatt JD, Peckham M, Edwards YH, Partridge TA, and Porter AC

Subjects

Animals, Cell Differentiation genetics, Cell Line, Transformed chemistry, Cell Line, Transformed cytology, Cloning, Molecular methods, Gene Expression physiology, Gene Transfer Techniques, Mice, Muscle Fibers, Fast-Twitch chemistry, Muscle Fibers, Slow-Twitch chemistry, Muscle, Skeletal cytology, Mutagenesis, Insertional physiology, Plasmids, Promoter Regions, Genetic physiology, Stem Cells chemistry, Transfection, Muscle Fibers, Fast-Twitch cytology, Muscle Fibers, Slow-Twitch cytology, Myosin Heavy Chains genetics, Stem Cells cytology

Abstract

The ability to carry out gene targeting in somatic stem cells while maintaining their stem cell characteristics would have important implications for gene therapy and for the analysis of gene function. Using mouse myoblasts, we have explored this possibility by attempting to alter the promoter of a myosin heavy chain gene (MyHCIIB) characteristic of physiologically "fast" muscle so as to force its unscheduled expression in physiologically "slow" muscle fibers. Conditionally immortalized muscle precursor cells were transfected with a gene targeting construct designed to replace the MyHCIIB promoter with that for the carbonic anhydrase III gene (CAIII), which is highly expressed in slow muscle. A potentially targeted clone was isolated and differentiated in culture to form myotubes which expressed MyHCIIB. Cells from the same clone were injected into both slow and fast muscle of host mice, where they contributed to fiber formation. In slow muscle, the fibers derived from this clone did not express MyHCIIB; this may reflect an instability of the targeted MyHCIIB locus and/or a failure of the hybrid promoter to function in slow fibers in vivo. Nonetheless, we have demonstrated that a "promoter knock-in" gene targeting procedure can be used to generate unique MyHCIIB-expressing myotubes in culture and that conditionally immortalized myoblasts can be subjected to extensive passaging and genetic manipulation without losing their ability to form fibers in culture and in vivo.

Published

1999

18. Expression of neurofilament L-promoter green-fluorescent protein constructs in immortalized Schwann cell-neuron coculture.

Author

Haynes LW, Schmitz S, Clegg JC, and Fooks AR

Subjects

Animals, Cell Communication physiology, Cell Culture Techniques methods, Cell Line, Transformed chemistry, Cell Line, Transformed physiology, Gene Expression physiology, Genes, Reporter, Green Fluorescent Proteins, Humans, Indicators and Reagents, Myelin Sheath physiology, Neurons chemistry, Neurons cytology, Rats, Schwann Cells chemistry, Schwann Cells cytology, Luminescent Proteins genetics, Neurofilament Proteins genetics, Neurons physiology, Promoter Regions, Genetic, Schwann Cells physiology

Abstract

The neurofilament L/68 protein (NF-L/68) gene is expressed in the immature Schwann cell phenotype but suppressed after myelin-formation. We have investigated conditions which regulate the activity of the NF-L/68 promoter in green fluorescent protein reporter constructs expressed in the immortal rat Schwann cell strain SCL4.1/F7 in coculture with neurons. Constructs expressed in a plasmid vector containing both the full-length promoter and the 3' proximal 107 bp sequence which includes the cyclic AMP response element (CRE), were active in SCL4.1/F7 cells, but were suppressed as the cells underwent spontaneous growth-arrest. Interaction of SCL4.1/F7 with axons accelerated downregulation of expression from both constructs, however expression of the full-length promoter continued in some cells until the onset of myelin-formation. Expression of the NFL/68 construct recommenced when demyelination was induced in culture by exposure to human sera from patients with paraproteinemic gammopathy. We have demonstrated a method to study the regulation of gene expression patterns in single Schwann cells interacting with neurons and shown that different promoter regions may be controlled by axon-related and -unrelated factors.

Published

1999

19. Characterization of cell surface lectin-binding patterns of human airway epithelium.

Author

Dorscheid DR, Conforti AE, Hamann KJ, Rabe KF, and White SR

Subjects

Cell Line, Transformed chemistry, Cell Line, Transformed ultrastructure, Flow Cytometry, Glycoconjugates biosynthesis, Histocytochemistry, Humans, Lung metabolism, Epithelial Cells metabolism, Epithelial Cells ultrastructure, Lectins metabolism, Lung cytology, Membrane Glycoproteins biosynthesis, Membrane Glycoproteins metabolism

Abstract

Glycosylated structures on the cell surface have a role in cell adhesion, migration, and proliferation. Repair of the airway epithelium after injury requires each of these processes, but the normal cell surface glycosylation of non-mucin producing airway epithelial cells is unknown. We examined cell surface glycosylation in human airway epithelial cells in tissue sections and in human airway epithelial cell lines in culture. Thirty-eight lectin probes were used to determine specific carbohydrate residues by lectin-histochemistry. Galactose or galactosamine-specific lectins labeled basal epithelial cells, lectins specific for several different carbohydrate structures bound columnar epithelial cells, and fucose-specific lectins labeled all airway epithelial cells. The epithelial cell lines 1HAEo- and 16HBE14o- bound lectins that were specific to basal epithelial cells. Flow cytometry of these cell lines with selected lectins demonstrated that lectin binding was to cell surface carbohydrates, and revealed possible hidden tissue antigens on dispersed cultured cells. We demonstrate specific lectin-binding patterns on the surface of normal human airway epithelial cells. The expression of specific carbohydrate residues may be useful to type epithelial cells and as a tool to examine cell events involved in epithelial repair.

Published

1999

20. Novel dipeptidyl proteasome inhibitors overcome Bcl-2 protective function and selectively accumulate the cyclin-dependent kinase inhibitor p27 and induce apoptosis in transformed, but not normal, human fibroblasts.

Author

An B, Goldfarb RH, Siman R, and Dou QP

Subjects

Amino Acid Chloromethyl Ketones pharmacology, Apoptosis drug effects, Caspase Inhibitors, Caspases metabolism, Cell Line, Transformed chemistry, Cell Line, Transformed cytology, Cell Line, Transformed enzymology, Chymotrypsin metabolism, Cyclin-Dependent Kinase Inhibitor p21, Cyclin-Dependent Kinase Inhibitor p27, Cyclins antagonists & inhibitors, Cyclins metabolism, Cysteine Proteinase Inhibitors pharmacology, Dimethyl Sulfoxide pharmacology, Dipeptides metabolism, Etoposide pharmacology, Fibroblasts chemistry, Fibroblasts cytology, Fibroblasts enzymology, Gene Expression Regulation, Viral, HL-60 Cells chemistry, HL-60 Cells cytology, HL-60 Cells enzymology, Humans, Jurkat Cells chemistry, Jurkat Cells cytology, Jurkat Cells enzymology, Microtubule-Associated Proteins antagonists & inhibitors, Nucleic Acid Synthesis Inhibitors pharmacology, Poly Adenosine Diphosphate Ribose metabolism, Poly(ADP-ribose) Polymerase Inhibitors, Poly(ADP-ribose) Polymerases metabolism, Proteasome Endopeptidase Complex, Simian virus 40 genetics, Solvents pharmacology, Apoptosis physiology, Cell Cycle Proteins, Cysteine Endopeptidases metabolism, Dipeptides pharmacology, Microtubule-Associated Proteins metabolism, Multienzyme Complexes metabolism, Phthalimides pharmacology, Proto-Oncogene Proteins c-bcl-2 antagonists & inhibitors, Proto-Oncogene Proteins c-bcl-2 metabolism, Tumor Suppressor Proteins

Abstract

It has been suggested that overexpression of the Bcl-2 oncoprotein in human cancer cells contributes to their resistance to apoptosis induced by chemotherapy. We report here that a novel dipeptidyl proteasome inhibitor, CEP1612, at low concentrations rapidly induces apoptosis in human Jurkat T cells overexpressing Bcl-2 and also in all human prostate, breast, tongue and brain tumor cell lines we have tested to date, without exception. In contrast, etoposide, a standard anticancer drug, fails to kill these cells when employed under the same conditions. The apoptosis-inducing abilities of CEP1612 and its analogous compounds match precisely their order for inhibition of the proteasome chymotrypsin-like activity. CEP1612-induced apoptosis is p53-independent, inhibitable by a tetrapeptide caspase inhibitor, and associated with accumulation of the cyclin-dependent kinase inhibitors p21 and p27. Furthermore, CEP1612 selectively accumulates p27 and induces apoptosis in simian virus 40-transformed, but not the parental normal, human fibroblasts. Proteasome inhibitors such as those investigated herein might therefore have potential use as novel anticancer drugs.

Published

1998

21. Aryl-hydrocarbon receptor is an inhibitory regulator of lipid synthesis and of commitment to adipogenesis.

Author

Alexander DL, Ganem LG, Fernandez-Salguero P, Gonzalez F, and Jefcoate CR

Subjects

3T3 Cells chemistry, 3T3 Cells cytology, Animals, Basic Helix-Loop-Helix Transcription Factors, Cell Differentiation physiology, Cell Division physiology, Cell Line, Transformed chemistry, Cell Line, Transformed cytology, Cellular Senescence physiology, Cytochrome P-450 CYP1B1, Cytochrome P-450 Enzyme System genetics, Cytochrome P-450 Enzyme System metabolism, Gene Expression physiology, Mice, Receptors, Cytoplasmic and Nuclear genetics, Receptors, Cytoplasmic and Nuclear metabolism, Transcription Factors genetics, Transcription Factors metabolism, Transfection, Adipose Tissue chemistry, Adipose Tissue metabolism, Aryl Hydrocarbon Hydroxylases, Receptors, Aryl Hydrocarbon genetics, Receptors, Aryl Hydrocarbon metabolism, Triglycerides biosynthesis

Abstract

The aryl-hydrocarbon receptor (AhR) is a ligand-dependent transcription factor that mediates the biological effects of 2,3,7, 8-tetrachlorodibenzo-p-dioxin (TCDD). In mouse embryo fibroblasts, TCDD activates expression of multiple genes, including CYP1B1, the predominant cytochrome P450 expressed in these cells. Here, we analyze constitutive functions of the AhR in primary mouse embryo fibroblasts (MEFs) and spontaneously immortalized MEF cell lines derived from wild-type (WT) C57BL/6 mice and also from congenic mice with a targeted disruption of the AhR gene (AhR-/-). After multiple passages, primary MEFs exhibit spontaneous differentiation, growth cessation and senescence. Eventually, colonies of immortalized MEFs arise to provide clonal lines. The senescent phase occurs much earlier for AhR-/- MEFs, while immortalization is substantially delayed. Comparison of AhR-/- and WT MEFs also indicates that constitutive AhR activity is required for basal expression of CYP1B1 and suppresses lipogenesis in subconfluent cultures. Primary WT and AhR-/- MEFs and the corresponding lines undergo adipogenesis when treated at confluence with the appropriate hormonal inducers. Addition of TCDD before or concurrent with hormonal induction suppressed PPAR gamma mRNA and adipogenesis, as measured by lipid accumulation, glycerol phosphate dehydrogenase activity and stearoyl CoA desaturase type 1 mRNA expression. This effect of TCDD treatment was absent in AhR-/- MEFs, establishing the role of AhR in hormone-induced adipogenesis. Such hormonal activation of confluent MEFs and preadipocytes results in a limited proliferative expansion followed by irreversible growth arrest. TCDD-treated MEFs undergo the mitotic expansion but fail to exit the cell cycle. In AhR-/- MEFs, there is no such effect of TCDD. These findings implicate the AhR as a constitutive inhibitor of triglyceride synthesis, and as an early regulator of adipocyte differentiation. AhR interference with cell-cycle arrest in differentiation may be linked to the increased rate of senescence.

Published

1998

22. Insulin-like growth factor-I-mediated survival from anoikis: role of cell aggregation and focal adhesion kinase.

Author

Valentinis B, Reiss K, and Baserga R

Subjects

3T3 Cells chemistry, 3T3 Cells cytology, 3T3 Cells enzymology, Animals, Apoptosis physiology, Cell Aggregation physiology, Cell Line, Transformed chemistry, Cell Line, Transformed cytology, Cell Line, Transformed physiology, Cell Survival physiology, DNA biosynthesis, Dose-Response Relationship, Drug, Flow Cytometry, Focal Adhesion Kinase 1, Focal Adhesion Protein-Tyrosine Kinases, Genes, src physiology, Mice, Phosphorylation, Polyhydroxyethyl Methacrylate, Cell Adhesion Molecules metabolism, Insulin-Like Growth Factor I metabolism, Insulin-Like Growth Factor I pharmacology, Protein-Tyrosine Kinases metabolism

Abstract

Anoikis is a form of cell death that occurs when cells are denied attachment to the extra-cellular matrix. Using p6 cells, that are 3T3 cells overexpressing the type 1 insulin-like growth factor receptor (IGF-IR), we show that these cells undergo apoptosis when seeded on polyHEMA plates in serum-free medium (SFM). IGF-I protects p6 cells from anoikis, without inducing mitogenesis or DNA synthesis. In the surviving p6 cells in suspension cultures, the focal adhesion kinase (FAK) is tyrosyl phosphorylated by IGF-I, although this phosphorylation occurs only after several hours. The importance of FAK in protection from anoikis is confirmed by v-src-transformed R-cells, in which FAK is constitutively phosphorylated, that survive even in SFM. Surviving cells, whether p6 or v-src transformed, tend to form large cell aggregates, whose appearance precedes the phosphorylation of FAK. These and other findings suggest that FAK phosphorylation in the case of IGF-I is a mediated effect rather than a direct one. When p6 cells are plated on polyHEMA dishes, IGF-I induces cell aggregation and this aggregation correlates with survival and the eventual phosphorylation of FAK.

Published

1998

23. Heregulin-dependent autocrine loop regulates growth of K-ras but not erbB-2 transformed rat thyroid epithelial cells.

Author

Mincione G, Piccirelli A, Lazzereschi D, Salomon DS, and Colletta G

Subjects

Amphiregulin, Animals, Antibodies pharmacology, Antineoplastic Agents metabolism, Betacellulin, Binding, Competitive immunology, Breast Neoplasms, Carrier Proteins immunology, Cell Line, Transformed chemistry, Cell Line, Transformed physiology, Colonic Neoplasms, EGF Family of Proteins, Epithelial Cells chemistry, Epithelial Cells physiology, ErbB Receptors genetics, GPI-Linked Proteins, Gene Expression physiology, Glycoproteins immunology, Growth Substances genetics, Humans, Neoplasm Proteins genetics, Neutralization Tests, Proto-Oncogene Proteins genetics, RNA, Messenger analysis, Rats, Receptor, ErbB-3, Receptor, ErbB-4, Tumor Cells, Cultured, Autocrine Communication physiology, Carrier Proteins genetics, Epidermal Growth Factor, Glycoproteins genetics, Intercellular Signaling Peptides and Proteins, Membrane Glycoproteins, Neuregulin-1, Receptor, ErbB-2 genetics, Thyroid Gland cytology, ras Proteins genetics

Abstract

The EGF-like family of proteins, such as epidermal growth factor (EGF), transforming growth factor alpha (TGFalpha), amphiregulin (AR), betacellulin (BTC), cripto-1 (CR-1), and heregulin (HRG), plays an important role in the pathogenesis of several human carcinomas as autocrine growth factors. Differentiation and proliferation of rat thyroid cells in culture (FRTL-5 cells) are regulated by thyrotropin (TSH); withdrawal of TSH from culture medium produces growth arrest, whereas its addition to quiescent cells stimulates cell entry into S phase. Instead, transformed thyroid cell lines as FRTL-5H2 cell line, overexpressing erbB-2, Kimol cells, transformed by the wild-type K-ras and A6 clone, transformed by a temperature sensitive K-ras mutant, can grow without addition of TSH to the culture medium. In order to identify whether EGF-like growth factors and corresponding receptors (erbB-2, erbB-3, and erbB-4) could be involved in the autonomous growth of these transformed rat thyroid epithelial cells, Northern blot for mRNA analysis and Western blot for protein expression were performed. In contrast to normal control FRTL-5 cells, both K-ras and erbB-2-transformed cells expressed elevated levels of erbB-2 receptor. Moreover, both K-ras transformed cells, Kimol and A6 cells, but no FRTL-5H2 cells, were found able to express also high levels of erbB-4 receptor and HRG/NDF ligand. Treatment of K-ras transformed thyroid cells with neutralizing antibody against HRG/NDF reduced by 50% cell proliferation. These data indicate that unlike the erbB-2 overexpressing FRTL-5 cells, in K-ras rat thyroid epithelial cells, the growth factor heregulin signals through the heterodimer erbB-2/erbB-4 receptors in an autocrine fashion.

Published

1998

24. Mrp1 multidrug resistance-associated protein and P-glycoprotein expression in rat brain microvessel endothelial cells.

Author

Regina A, Koman A, Piciotti M, El Hafny B, Center MS, Bergmann R, Couraud PO, and Roux F

Subjects

ATP Binding Cassette Transporter, Subfamily B, Member 1 analysis, ATP Binding Cassette Transporter, Subfamily B, Member 1 antagonists & inhibitors, Animals, Antineoplastic Agents, Phytogenic pharmacokinetics, Astrocytes cytology, Astrocytes physiology, Benzbromarone pharmacology, Capillaries chemistry, Capillaries physiology, Carcinogens pharmacology, Cell Line, Transformed chemistry, Cell Line, Transformed physiology, Colchicine pharmacokinetics, Cyclosporine pharmacology, DNA-Binding Proteins analysis, DNA-Binding Proteins antagonists & inhibitors, Endothelium, Vascular cytology, Endothelium, Vascular drug effects, Enzyme Inhibitors pharmacology, Gene Expression Regulation, Neoplastic, Genistein pharmacology, Gout Suppressants pharmacokinetics, Immunoblotting, MutS Homolog 3 Protein, Polymerase Chain Reaction, Probenecid pharmacology, RNA, Messenger metabolism, Rats, Rats, Sprague-Dawley, Sulfinpyrazone pharmacology, Uricosuric Agents pharmacology, Vinblastine pharmacokinetics, Vincristine pharmacokinetics, ATP Binding Cassette Transporter, Subfamily B, Member 1 genetics, Brain blood supply, DNA-Binding Proteins genetics, Endothelium, Vascular chemistry, Multidrug Resistance-Associated Proteins

Abstract

Two membrane glycoproteins acting as energy-dependent efflux pumps, mdr-encoded P-glycoprotein (P-gp) and the more recently described multidrug resistance-associated protein (MRP), are known to confer cellular resistance to many cytotoxic hydrophobic drugs. In the brain, P-gp has been shown to be expressed specifically in the capillary endothelial cells forming the blood-brain barrier, but localization of MRP has not been well characterized yet. Using RT-PCR and immunoblot analysis, we have compared the expression of P-gp and Mrp1 in homogenates, isolated capillaries, primary cultured endothelial cells, and RBE4 immortalized endothelial cells from rat brain. Whereas the mdr1a P-gp-encoding mRNA was specifically detected in brain microvessels and mdr1b mRNA in brain parenchyma, mrp1 mRNA was present both in microvessels and in parenchyma. However, Mrp1 was weakly expressed in microvessels. Mrp1 expression was higher in brain parenchyma, as well as in primary cultured brain endothelial cells and in immortalized RBE4 cells. This Mrp1 overexpression in cultured brain endothelial cells was less pronounced when the cells were cocultured with astrocytes. A low Mrp activity could be demonstrated in the endothelial cell primary monocultures, because the intracellular [3H]vincristine accumulation was increased by several MRP modulators. No Mrp activity was found in the cocultures or in the RBE4 cells. We suggest that in rat brain, Mrp1, unlike P-gp, is not predominantly expressed in the blood-brain barrier endothelial cells and that Mrp1 and the mdr1b P-gp isoform may be present in other cerebral cells.

Published

1998

25. Virally activated Ras cooperates with integrin to induce tubulogenesis in sinusoidal endothelial cell lines.

Author

Maru Y, Yamaguchi S, Takahashi T, Ueno H, and Shibuya M

Subjects

ADP Ribose Transferases pharmacology, Animals, Cadherins analysis, Calcium-Calmodulin-Dependent Protein Kinases analysis, Cell Adhesion Molecules analysis, Cell Line, Transformed chemistry, Cell Line, Transformed drug effects, Cell Line, Transformed physiology, Collagen pharmacology, Cytoskeletal Proteins analysis, Desmoplakins, Drug Combinations, Endothelium chemistry, Endothelium cytology, Endothelium enzymology, Enzyme Inhibitors pharmacology, Extracellular Matrix chemistry, Extracellular Matrix enzymology, Flavonoids pharmacology, Humans, Laminin pharmacology, Liver blood supply, Liver physiology, Neovascularization, Physiologic physiology, Proteins physiology, Proteoglycans pharmacology, Rats, Receptor Protein-Tyrosine Kinases genetics, Receptors, Growth Factor genetics, Receptors, Mitogen genetics, Receptors, Vascular Endothelial Growth Factor, Retroviridae genetics, Shc Signaling Adaptor Proteins, Signal Transduction drug effects, Signal Transduction physiology, Src Homology 2 Domain-Containing, Transforming Protein 1, Umbilical Veins cytology, alpha Catenin, beta Catenin, src Homology Domains physiology, Adaptor Proteins, Signal Transducing, Adaptor Proteins, Vesicular Transport, Botulinum Toxins, Gene Expression Regulation, Viral, Integrins physiology, Liver cytology, Trans-Activators, ras Proteins genetics

Abstract

Four cell lines, named nonparenchymal 11 (NP11), NP26, NP31, and NP32, were established from sinusoidal endothelial cells (SECs) of rat liver. They still retained expression of receptors for vascular endothelial growth factor (VEGF), Fit-1, and kinase domain-containing receptor (KDR). NP31 and NP32 turned out to be incapable of tubulogenesis in basement membrane matrix (Matrigel), which belongs to endothelial properties, as shown by SECs in primary culture. Expression of temperature-sensitive, virally activated Ras (ts-v-Ras) restored tubulogenic behaviors back to NP31 only at permissive temperature. Matrigel induced long-lasting tyrosine phosphorylation of Shc, with recruitment of Grb-2 and microtubule-associated protein kinase (MAPK) activation in both parental NP31 and NP31 transformed by ts-v-Ras, which was blocked by anti-beta1 integrin antibody. Tubulogenesis was inhibited by adenovirus-mediated expression of dominant-negative Ras in human umbilical vein endothelial cells (HUVECs). PD 098059, a selective inhibitor of MAPK kinase (MEK), nearly perfectly blocked tubulogenesis by ts-v-Ras-expressing NP31 cells at permissive temperature. Furthermore, the botulinum C3 toxin, an inhibitor for Rho, caused fragmentation of branching cords in networks formed by NP31 that expressed ts-v-Ras at permissive temperature. These data suggest that the integrin-mediated Ras signals may be necessary but are not sufficient for tubulogenesis and that an artificial expression of v-Ras might substitute for the second signal required in this system.

Published

1998

26. Enzymatic and molecular biological analysis of palmitoyl protein thioesterase deficiency in infantile neuronal ceroid lipofuscinosis.

Author

Cho S and Dawson G

Subjects

B-Lymphocytes cytology, Blotting, Northern, Carbon Radioisotopes, Carcinoma, Hepatocellular, Cell Line, Transformed chemistry, Cell Line, Transformed enzymology, Gene Expression Regulation, Enzymologic, Genetic Carrier Screening, Humans, Kidney cytology, Kinetics, Lysosomes enzymology, Neuroblastoma, Oligodendroglioma, Palmitoyl-CoA Hydrolase genetics, Peptides metabolism, RNA, Messenger analysis, Substrate Specificity, Brain enzymology, Neuronal Ceroid-Lipofuscinoses diagnosis, Neuronal Ceroid-Lipofuscinoses metabolism, Palmitoyl-CoA Hydrolase deficiency

Abstract

Infantile neuronal ceroid lipofuscinosis (INCL) is a neurodegenerative lysosomal storage disease that results from a deficiency of palmitoyl protein thioesterase (PPT), a deacylating enzyme that removes cysteine-bound palmitate from proteins. We developed an in vitro PPT enzyme assay that can be readily used for the clinical diagnosis of both INCL patients and carriers. The substrate is a palmitoylated peptide (IRY[14C]palmitoyl-CWLRR) synthesized by reacting [14C] palmitoyl-CoA with a synthetic octapeptide from the PNS P0 glycoprotein. The PPT assay performed in immortalized lymphoblastoid B-cells or the postmortem brain homogenate showed the optimal enzyme activity at pH 5.0, consistent with the findings that PPT is a lysosomal enzyme. PPT activity in lymphoblasts from INCL patients was <4% of that of control lymphoblasts. In addition, obligatory carriers showed 74% of the control activity. Other pathological controls, including the juvenile form of NCL, showed PPT activities that were not different from normal. Furthermore, one brain sample from an INCL patient contained only 7% PPT activity when compared with an unaffected brain. Thus, the enzyme activity assay gives a confident diagnosis of INCL. In contrast, when the total RNA extract from lymphoblasts was probed with 32P-labeled PPT by northern blot analysis, the level of transcript varied among independent INCL families and was not related to PPT activity. In conclusion, whereas variant genetic modifications result in PPT deficiency, all giving similar INCL phenotype, both affected patients and heterozygote carriers can now be screened with a reliable in vitro PPT assay.

Published

1998

27. Regulated expression of neurogenic basic helix-loop-helix transcription factors during differentiation of the immortalized neuronal progenitor cell line HC2S2 into neurons.

Author

Ohtsuka T, Asahi M, Matsuura N, Kikuchi H, Hojo M, Kageyama R, Ohkubo H, and Hoshimaru M

Subjects

Animals, Basic Helix-Loop-Helix Transcription Factors, Blotting, Northern, Cell Differentiation genetics, Cell Line, Transformed chemistry, Cell Line, Transformed cytology, Cell Line, Transformed physiology, DNA-Binding Proteins analysis, DNA-Binding Proteins genetics, Fluorescent Antibody Technique, GAP-43 Protein analysis, GAP-43 Protein genetics, Hippocampus cytology, Homeodomain Proteins analysis, Homeodomain Proteins genetics, Nerve Tissue Proteins analysis, Nerve Tissue Proteins genetics, Neurons chemistry, Neurons physiology, Neuropeptides analysis, Neuropeptides genetics, RNA, Messenger analysis, Rats, Repressor Proteins analysis, Repressor Proteins genetics, Stem Cells chemistry, Stem Cells physiology, Transcription Factor HES-1, Transcription Factors analysis, Gene Expression Regulation, Developmental, Helix-Loop-Helix Motifs genetics, Neurons cytology, Stem Cells cytology, Transcription Factors genetics, Xenopus Proteins

Abstract

Expression of nine neurogenic basic helix-loop-helix (bHLH) transcription factors was examined in an immortalized neuronal progenitor cell line HC2S2, which differentiates into neurons after suppression of the v-myc expression with tetracycline. Expression of MASH-1, NeuroD, NeuroD-related factor (NDRF) and HES-1 was demonstrated in HC2S2 cells by Northern blot analysis using total RNA. Expression of MASH-1 mRNA was downregulated upon differentiation of HC2S2 cells into mature neurons. In contrast, NeuroD and NDRF mRNA expression was maintained all through the differentiation. The expression of HES-1, a negative regulator of the neuronal differentiation, was upregulated temporarily in accordance with the suppression of the v-myc expression and was downregulated upon the differentiation of HC2S2 cells into neurons. The reduced expression of HES-1 mRNA in undifferentiated HC2S2 cells may be explained by the transcriptional suppression of HES-1 by the myc oncoprotein. The above data imply that both HES-1 and MASH-1 need to be downregulated at the time of accomplishment of the terminal differentiation into mature neurons and that NeuroD and NDRF participate in the regulatory process of the terminal differentiation in combination.

Published

1998

28. Herpesvirus saimiri transformation of HIV type 1 suppressive CD8+ lymphocytes from an HIV type 1-infected asymptomatic individual.

Author

Lacey SF, Weinhold KJ, Chen CH, McDanal C, Oei C, and Greenberg ML

Subjects

Cell Line, Transformed chemistry, Chemokine CCL3, Chemokine CCL4, Chemokine CCL5 analysis, Chemokine CCL5 chemistry, DNA, Viral analysis, HIV Seropositivity, Humans, Lymphocyte Activation, Macrophage Inflammatory Proteins analysis, Macrophage Inflammatory Proteins chemistry, Suppressor Factors, Immunologic isolation & purification, T-Lymphocytes, Cytotoxic immunology, CD8-Positive T-Lymphocytes virology, Cell Transformation, Viral physiology, HIV-1, Herpesvirus 2, Saimiriine physiology

Abstract

CD8+ T lymphocytes from HIV+ individuals can potently suppress HIV-1 replication in a noncytolytic manner. This suppression appears to be multifactorial and the molecules contributing have not been fully elucidated. As an approach to this question we used herpesvirus saimiri (HVS) to transform CD8+ T lymphocytes from an HIV+ asymptomatic donor to a continuously growing, activation-independent, IL-2-dependent phenotype. The transformed cell population, termed CD8(HVS), had an activated phenotype, contained HVS sequences, did not shed infectious HVS virus, and was polyclonal. The CD8(HVS) cells, despite the absence of detectable CTL activity, potently suppressed HIV-1 production by both autologous and heterologous CD4+ cells from infected donors. The CD8(HVS) cells in coculture also suppressed virus production from PBMCs acutely infected with syncytium-inducing (SI) strains or NSI primary isolates of HIV-1. The supernatants from the CD8(HVS) cells and their concentrates derived from these supernatants were suppressive to NSI primary isolates of HIV-1 but not to SI strains. Fractionation of these concentrates showed that the suppressive activity was associated with low molecular mass (6500- to 19,300-Da) protein species. Western blotting and ELISA indicated that the CC chemokines MIP-1alpha, MIP-1beta, and RANTES were present in these fractions. Antibody-blocking studies with antibodies to the CC chemokines indicated that a significant portion of the soluble HIV-suppressive activity was due to these molecules. However, these experiments also suggested the inhibitory activity of the CD8(HVS) cells in coculture is not due exclusively to the CC chemokines. The HVS-transformed cells provide a useful tool for the study of noncytolytic CD8+ T lymphocyte-mediated suppression of HIV-1.

Published

1998

29. Protein profiles and identification of high performance liquid chromatography isolated proteins of cancer cell lines using matrix-assisted laser desorption/ionization time-of-flight mass spectrometry.

Author

Chong BE, Lubman DM, Rosenspire A, and Miller F

Subjects

Cell Line, Transformed chemistry, Chromatography, High Pressure Liquid, Electrophoresis, Polyacrylamide Gel, Female, Fibroblast Growth Factor 3, Fibroblast Growth Factors chemistry, Fibroblast Growth Factors isolation & purification, Fibrocystic Breast Disease pathology, Humans, Molecular Weight, Neoplasm Proteins isolation & purification, Proto-Oncogene Proteins chemistry, Proto-Oncogene Proteins isolation & purification, Proto-Oncogene Proteins c-myc chemistry, Proto-Oncogene Proteins c-myc isolation & purification, Proto-Oncogene Proteins p21(ras) chemistry, Proto-Oncogene Proteins p21(ras) isolation & purification, Receptor, ErbB-2 chemistry, Receptor, ErbB-2 isolation & purification, Receptors, Thyroid Hormone chemistry, Receptors, Thyroid Hormone isolation & purification, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization instrumentation, Tumor Cells, Cultured chemistry, Tumor Suppressor Protein p53 chemistry, Tumor Suppressor Protein p53 isolation & purification, Neoplasm Proteins chemistry, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization methods

Abstract

Matrix-assisted laser desorption/ionization time-of-flight mass spectrometry (MALDI-TOFMS) has been used to rapidly profile the protein content of human cell lysates from MCF-10 cell and variant lines. The method was used to study the protein profiles of these cells as they progressed from normal breast epithelium to fully malignant cells. Distinct differences in the protein profiles were observed with progression, and specific proteins associated with carcinogenesis (p53, c-myc, and c-erbB-2) were heavily expressed in these cells as detected by MALDI-TOFMS. These proteins were also isolated using non-porous reversed-phase high performance liquid chromatography (NP-RP-HPLC) and mass analyzed by MALDI-TOFMS to provide molecular weight information without interference from other proteins in the whole cell lysates, and to avoid suppression effects in mixtures of proteins detected by MALDI-TOFMS. In order to confirm the identity of these oncoproteins, the cell lysates were subjected to one-dimensional (1-D) gel separation and subsequently electroblotted onto a poly(vinylidene difluoride) (PVDF) membrane for further analysis. Trypsin and cyanogen bromide digestions were performed on these proteins eluted from excised PVDF bands which were then analyzed by MALDI-TOFMS. The identity of these proteins was confirmed by database matching procedures.

Published

1998

30. Dendritic cells generated from blood precursors of chronic myelogenous leukemia patients carry the Philadelphia translocation and can induce a CML-specific primary cytotoxic T-cell response.

Author

Eibl B, Ebner S, Duba C, Böck G, Romani N, Erdel M, Gächter A, Niederwieser D, and Schuler G

Subjects

Cell Line, Transformed chemistry, Cells, Cultured, Clone Cells, Cytotoxicity Tests, Immunologic, Cytotoxicity, Immunologic, Dendritic Cells chemistry, Flow Cytometry, Humans, In Situ Hybridization, Fluorescence, Leukemia, Myelogenous, Chronic, BCR-ABL Positive genetics, Leukemia, Myelogenous, Chronic, BCR-ABL Positive pathology, Leukocytes, Mononuclear chemistry, Lymphocyte Activation genetics, T-Lymphocytes, Cytotoxic chemistry, T-Lymphocytes, Cytotoxic immunology, Dendritic Cells physiology, Leukemia, Myelogenous, Chronic, BCR-ABL Positive immunology, Philadelphia Chromosome, T-Lymphocytes, Cytotoxic physiology

Abstract

Dendritic cells (DC) are professional antigen-presenting cells specialized in the initiation of primary immune responses. We were interested to know whether mature DC can be grown in vitro from peripheral blood mononuclear cells (PBMC) of patients with chronic myelogenous leukemia (CML), and whether they carry the Philadelphia (Ph) translocation. Using a method recently described, DC were generated from PBMC precursors of 12 patients with CML using GM-CSF, IL-4, and monocyte-conditioned medium. DC exhibited the typical morphology with thin cytoplasmatic processes and expressed high levels of MHC class II, CD86, and CD83 typical for mature DC. After sorting with the monoclonal antibody CD83, a cell population of more than 95% CD83 positive cells was obtained. The presence of the Ph translocation was analyzed in these cells, in PBMC, lymphoblastoid cell lines (LCL), and in phytohemagglutinin (PHA)-induced T blasts from the same patients by fluorescence in situ hybridization (FISH). In contrast to all other cells analyzed, the vast majority of DC (95.9 +/- 0.7%) displayed the Ph translocation, irrespective of disease stage or therapy. PBMC were predominantly positive for the Ph chromosome (67.6 +/- 7.3%), whereas only 11.4 +/- 1% of the B cells and 4.4 +/- 1.1% of the PHA blasts carried the Ph translocation. Using such leukemic DC as antigen-presenting cells, a primary CML-directed cytotoxic immune response in vitro was obtained, as shown by the specific recognition of Ph chromosome positive cells. We conclude that DC can be generated from blood progenitors of CML patients in vitro and exhibit, to a large extent, the Ph translocation. Such DC, which in a preliminary experiment have been able to induce a primary CML-directed cytotoxic immune response in vitro, might be ideal candidates for adoptive immunotherapy either by direct transfer of DC for in vivo generation of a T-cell response or by in vitro generation of CML-specific cytotoxic autologous or HLA-matched normal T-cell clones for use in vivo.

Published

1997

31. AMF-R tubules concentrate in a pericentriolar microtubule domain after MSV transformation of epithelial MDCK cells.

Author

Nabi IR, Guay G, and Simard D

Subjects

Animals, Antigens analysis, Antigens, CD analysis, Calcium-Binding Proteins analysis, Calnexin, Cell Line, Transformed chemistry, Cell Nucleus ultrastructure, Centrioles ultrastructure, Coatomer Protein, Dogs, Epithelium chemistry, Epithelium ultrastructure, Fluorescent Antibody Technique, Indirect, Golgi Apparatus ultrastructure, Lysosomal Membrane Proteins, Membrane Glycoproteins analysis, Microscopy, Confocal, Microtubule-Associated Proteins analysis, Microtubules drug effects, Moloney murine sarcoma virus, Nocodazole pharmacology, Receptors, Autocrine Motility Factor, Ubiquitin-Protein Ligases, Microtubules metabolism, Receptors, Cytokine analysis, Tubulin analysis

Abstract

Autocrine motility factor receptor (AMF-R) is localized to an intracellular microtubule-associated membranous organelle, the AMF-R tubule. In well-spread untransformed MDCK epithelial cells, the microtubules originate from a broad perinuclear region and AMF-R tubules extend throughout the cytoplasm of the cells. In Moloney sarcoma virus (mos)-transformed MDCK (MSV-MDCK) cells, microtubules accumulate around the centrosome, forming a microtubule domain rich in stabilized detyrosinated microtubules. AMF-R tubules are quantitatively associated with this pericentriolar microtubule domain and the rough endoplasmic reticulum and lysosomes also co-distribute with the pericentriolar mass of microtubules. The Golgi apparatus is closely associated with the microtubule organizing center (MTOC) within the juxtanuclear mass of AMF-R tubules, and no co-localization of AMF-R tubules with the Golgi marker beta-COP could be detected by confocal microscopy. After nocodazole treatment and washout, microtubule nucleation occurs exclusively at the centrosome of MSV-MDCK cells, and only after microtubule extension to the cell periphery does the microtubule cytoskeleton reorganize to generate the pericentriolar microtubule domain after 30-60 min. AMF-R tubules dispersed by nocodazole treatment concentrate in the pericentriolar region in parallel with the reorganization of the microtubule cytoskeleton. MSV transformation of epithelial MDCK cells results in the stabilization of a pericentriolar microtubule domain responsible for the concentration and polarized distribution of AMF-R tubules.

Published

1997

32. Measuring S-adenosylmethionine in whole blood, red blood cells and cultured cells using a fast preparation method and high-performance liquid chromatography.

Author

Wise CK, Cooney CA, Ali SF, and Poirier LA

Subjects

Animals, B-Lymphocytes chemistry, Cell Line, Transformed chemistry, Chemical Precipitation, Drug Stability, Female, Humans, Male, Mice, Mice, Inbred C57BL, Mice, Inbred Strains, Rats, Rats, Inbred F344, S-Adenosylmethionine analysis, Temperature, Time Factors, Trichloroacetic Acid chemistry, Chromatography, High Pressure Liquid methods, Erythrocytes chemistry, S-Adenosylmethionine blood

Abstract

The physiological methyl donor S-adenosylmethionine (SAM) plays a key role in the maintenance of human health and in the prevention of disease. A convenient clinical test for blood SAM does not exist, even though blood SAM is increasingly seen as an important indicator of health. We have developed a simple procedure to extract SAM from small amounts of blood or cells. The extracted SAM is then measured by high-performance liquid chromatography (HPLC). This measurement is sensitive, precise and uses as little as 200 microliters of blood or 0.5-10(6) cultured cells per determination. SAM, as tested with this method, under acidic conditions, is stable for hours and can be frozen for later analysis. The method has been used to show that blood SAM varies with species, sex and treatment. We have also measured the SAM levels in cultured cells, and have been able to detect wide variations depending upon treatments administered during the growth of those cells. In conclusion, this is a very rapid and easy method to measure SAM in biological fluids and cell culture and which could be adapted to the clinical setting.

Published

1997

33. Possible role of cytochrome P450 in inactivation of testosterone in immortalized hippocampal neurons.

Author

Thuerl C, Otten U, Knoth R, Meyer RP, and Volk B

Subjects

Age Factors, Animals, Antibodies pharmacology, Aromatase analysis, Aromatase metabolism, Cell Differentiation drug effects, Cell Differentiation physiology, Cell Line, Transformed chemistry, Cell Line, Transformed drug effects, Cell Line, Transformed metabolism, Cytochrome P-450 Enzyme System analysis, Cytochrome P450 Family 2, Cytoskeleton chemistry, Cytoskeleton metabolism, Cytoskeleton ultrastructure, Fetus cytology, Hippocampus cytology, Hybrid Cells chemistry, Hybrid Cells drug effects, Hybrid Cells metabolism, Mice, Microscopy, Immunoelectron, Neuroblastoma, Neurons drug effects, Neurons enzymology, Testosterone immunology, Testosterone pharmacology, Tubulin analysis, Tubulin metabolism, Aryl Hydrocarbon Hydroxylases, Cytochrome P-450 Enzyme System physiology, Neurons cytology, Steroid Hydroxylases, Testosterone metabolism

Abstract

The hippocampus as part of the limbic system is sensitive to gonadal hormones. The time-dependent expression of steroid receptors and the testosterone converting enzyme aromatase (CYP19) is well studied. In contrast, little is known about other cytochrome P450 enzymes in hippocampus which inactivate the gonadal hormones. For investigation of the total cytochrome P450 content and the expression of testosterone degrading CYP2B10 we used embryonic (E18) in comparison to postnatal (P21) immortalized hippocampal neurons. These embryonic neurons were demonstrated to react to hormones according a 'critical period' of sexual differentiation: testosterone treatment (1 microM to 5 microM in the culture medium) resulted in a decrease of beta-tubulin, as showed by immunocytochemistry and Western blotting. Measurements with reduced CO-difference spectrum elucidated that the P450 concentration in the embryonic neurons (10.2 pmol/mg protein; S.D. +/- 1.9) was twice as high as in the postnatal ones (5.2 pmol/mg protein; S.D. +/- 1.0). Correspondingly, a high value of the mitochondrial subfraction of approx. 141 pmol P450/mg protein was found in the embryonic neurons relative to the mitochondrial value of 37.7 pmol P450/mg protein in the postnatal neurons. Our results suggest a differential expression of cytochrome P450 during development. CYP2B10 was proved by electron microscopy and hormone degrading activity.

Published

1997

34. Studies on rLMP7, a beta-subunit of the multicatalytic proteinase.

Author

Ren L and Clawson GA

Subjects

Amino Acid Sequence, Animals, Base Sequence, Cell Line, Transformed chemistry, Cell Line, Transformed metabolism, Cell Nucleus chemistry, Cysteine Endopeptidases metabolism, Cytosol chemistry, DNA, Complementary, Electrophoresis, Polyacrylamide Gel, Fluorescent Antibody Technique, Gene Expression Regulation, Enzymologic physiology, Green Fluorescent Proteins, Humans, Liver cytology, Luminescent Proteins genetics, Male, Mice, Molecular Sequence Data, Multienzyme Complexes metabolism, Polymerase Chain Reaction, Precipitin Tests, Protein Precursors analysis, RNA, Messenger metabolism, Rats, Rats, Sprague-Dawley, Recombinant Fusion Proteins genetics, Transfection, Cysteine Endopeptidases chemistry, Cysteine Endopeptidases genetics, Multienzyme Complexes chemistry, Multienzyme Complexes genetics

Abstract

Subunit rLMP7 of the multicatalytic proteinase (MCP), which has been associated with chymotrypsin-like proteinase activity, was examined in rat liver and hepatocyte-derived cell lines. rLMP7 was detected in both nucleus and cytosol in liver by immunohistochemistry and immunoblotting, using a peptide-specific anti-rLMP7 antibody. A M(r) 30,000 precursor protein was present only in cytosol, as was a minor component of M(r) 25,000. Mature rLMP7 (M(r) 23,000) was present in MCP in both nucleus and cytosol, although it was not detectable in the nuclear scaffold. Two rLMP7 cDNAs (designated rLMP7.1 and rLMP7.s) were identified by rapid amplification of 5' ends using RT/PCR, a result which was confirmed by Northern blot analysis and RNase protection assays. rLMP7.1 is 3-4x more abundant than rLMP7.s; it is 50 nt longer than the previously reported cDNA sequence and includes an upstream in-frame ATG within a consensus translation initiation sequence, which encodes the M(r) 30,000 rLMP7 precursor protein identified in vivo. rLMP7.s is 100 nt shorter than rLMP7.1 and does not contain the most 5' ATG. Transient transfection analyses with rLMP7.1 and rLMP7.s constructs coupled to green fluorescent protein showed that both transcripts were efficiently expressed in vivo. In vitro expression of these two rLMP7 cDNAs showed that rLMP7.1 produces the M(r) 30,000 precursor protein, whereas rLMP7.s produces two smaller peptides of M(r) 25,000 and 23,000. Purified 20S MCP preparations were able to proteolytically process the M(r) 30,000 precursor to the M(r) 25,000 product but not to the mature rLMP7 form. However, incorporation of this processed M(r) 25,000 product (or of either M(r) form produced from rLMP7.s) did not occur in vitro. In vitro processing and pulse-chase experiments suggested that the mature M(r) 23,000 subunit is derived, at least in part, from the M(r) 30,000 precursor. The M(r) 25,000 form may be a stable product produced directly from rLMP7.s.

Published

1997

35. Altered differentiation of CNS neural progenitor cells after transplantation into the injured adult rat spinal cord.

Author

Onifer SM, Cannon AB, and Whittemore SR

Subjects

Animals, Bromodeoxyuridine, Cell Differentiation physiology, Cell Line, Transformed chemistry, Cell Line, Transformed transplantation, Choline O-Acetyltransferase analysis, Choline O-Acetyltransferase genetics, Denervation, Excitatory Amino Acid Agonists, Female, Intermediate Filament Proteins analysis, Intermediate Filament Proteins genetics, Kainic Acid, Lac Operon, Male, Nerve Crush, Nestin, Neurons cytology, Neurons enzymology, Neurotoxins, Phenotype, Rats, Rats, Sprague-Dawley, Sciatic Nerve surgery, Stem Cells chemistry, Stem Cells cytology, Nerve Tissue Proteins, Neurons transplantation, Spinal Cord surgery, Stem Cell Transplantation

Abstract

Denervation of CNS neurons and peripheral organs is a consequence of traumatic SCI. Intraspinal transplantation of embryonic CNS neurons is a potential strategy for reinnervating these targets. Neural progenitor cell lines are being investigated as alternates to embryonic CNS neurons. RN33B is an immortalized neural progenitor cell line derived from embryonic rat raphe nuclei following infection with a retrovirus encoding the temperature-sensitive mutant of SV40 large T-antigen. Transplantation studies have shown that local epigenetic signals in intact or partially neuron-depleted adult rat hippocampal formation or striatum direct RN33B cell differentiation to complex multipolar morphologies resembling endogenous neurons. After transplantation into neuron-depleted regions of the hippocampal formation or striatum, RN33B cells were relatively undifferentiated or differentiated with bipolar morphologies. The present study examines RN33B cell differentiation after transplantation into normal spinal cord and under different lesion conditions. Adult rats underwent either unilateral lesion of lumbar spinal neurons by intraspinal injection of kainic acid or complete transection at the T10 spinal segment. Neonatal rats underwent either unilateral lesion of lumbar motoneurons by sciatic nerve crush or complete transection at the T10 segment. At 2 or 6-7 wk postinjury, lacZ-labeled RN33B cells were transplanted into the lumbar enlargement of injured and age-matched normal rats. At 2 wk posttransplantation, bipolar and some multipolar RN33B cells were found throughout normal rat gray matter. In contrast, only bipolar RN33B cells were seen in gray matter of kainic acid lesioned, sciatic nerve crush, or transection rats. These observations suggest that RN33B cell multipolar morphological differentiation in normal adult spinal cord is mediated by direct cell-cell interaction through surface molecules on endogenous neurons and may be suppressed by molecules released after SCI. They also indicate that the fate of immortalized neural progenitor cell lines in injured CNS must be stringently characterized.

Published

1997

36. Growth properties of neural cell lines immortalized with the tsA58 allele of SV40 large T antigen.

Author

Truckenmiller ME, Dillon-Carter O, Tornatore C, Kulaga H, Takashima H, and Freed WJ

Subjects

Alleles, Animals, Antigens, Polyomavirus Transforming analysis, Base Sequence, Blood Proteins pharmacology, Cell Cycle physiology, Cell Division physiology, Cell Line, Transformed chemistry, Cell Line, Transformed cytology, Cell Line, Transformed drug effects, Cell Survival physiology, Culture Media, Serum-Free pharmacology, Fetus cytology, Flow Cytometry, Immunohistochemistry, Molecular Sequence Data, Neurons chemistry, Neurons drug effects, Point Mutation, Rats, S Phase physiology, Sequence Analysis, DNA, Temperature, Antigens, Polyomavirus Transforming genetics, Corpus Striatum cytology, Neurons cytology

Abstract

In vitro growth properties of three CNS-derived cell lines were compared under a variety of culture conditions. The M213-20 and J30a cell lines were each derived from embryonic CNS culture with the temperature-sensitive (ts) allele of SV40 large T antigen, tsA58, while the A7 cell line was immortalized using wild-type SV40 large T antigen. Cells immortalized with tsA58 SV40 large T proliferate at the permissive temperature, 33 degrees C, while growth is expected to be suppressed at the nonpermissive temperature, 39.5 degrees C. Both the M213-20 and J30a cell lines were capable of proliferating at 39.5 degrees C continuously for up to 6 mo. All three cell lines showed no appreciable differences in growth rates related to temperature over a 7-day period in either serum-containing or defined serum-free media. The percentage of cells in S-phase of the cell cycle did not decrease or was elevated at 39.5 degrees C for all three cell lines. After 3 wk at 39.5 degrees C, the three cell lines also showed positive immunostaining using two monoclonal antibodies reacting with different epitopes of SV40 large T antigen. Double strand DNA sequence analyses of a 300 base pair (bp) fragment of the large T gene from each cell line, which included the ts locus, revealed mutations in both the J30a and M213-20 cell lines. The J30a cell line ts mutation had reverted to wild type, and two additional loci with bp substitutions with predicted amino acid changes were also found. While the ts mutation of the M213-20 cells was retained, an additional bp substitution with a predicted amino acid change was found. The A7 cell line sequence was identical to the reference wild-type sequence. These findings suggest that (a) nucleic acid sequences in the temperature-sensitive region of the tsA58 allele of SV40 large T are not necessarily stable, and (b) temperature sensitivity of cell lines immortalized with tsA58 is not necessarily retained.

Published

1997

37. Two distinct P2 purinergic receptors, P2Y and P2U, are coupled to phospholipase C in mouse pineal gland tumor cells.

Author

Suh BC, Son JH, Joh TH, and Kim KT

Subjects

Adenosine Diphosphate analogs & derivatives, Adenosine Diphosphate pharmacology, Adenosine Triphosphate analogs & derivatives, Adenosine Triphosphate pharmacology, Animals, Antigens, Polyomavirus Transforming, Arylamine N-Acetyltransferase metabolism, Biomarkers, Calcium metabolism, Carcinogens pharmacology, Cell Line, Transformed chemistry, Cell Line, Transformed drug effects, Cell Line, Transformed enzymology, Dose-Response Relationship, Drug, Inositol 1,4,5-Trisphosphate metabolism, Magnesium pharmacology, Mice, Pertussis Toxin, Pineal Gland chemistry, Receptors, Purinergic P2 chemistry, Tetradecanoylphorbol Acetate pharmacology, Thionucleotides pharmacology, Tryptophan Hydroxylase metabolism, Uridine Triphosphate pharmacology, Virulence Factors, Bordetella pharmacology, Pineal Gland cytology, Receptors, Purinergic P2 metabolism, Type C Phospholipases metabolism

Abstract

We found that extracellular ATP can increase the intracellular Ca2+ concentration ([Ca2+]i) in mouse pineal gland tumor (PGT-beta) cells. Studies of the [Ca2+]i rise using nucleotides and ATP analogues established the following potency order: ATP, adenosine 5'-O-(3-thiotriphosphate) > or = UTP > 2-chloro-ATP > 3'-O-(4-benzoyl)benzoyl ATP, GTP > or = 2-methylthio ATP, adenosine 5'-O-(2-thiodiphosphate) (ADP beta S) > CTP. AMP, adenosine, alpha,beta-methyleneadenosine 5'-triphosphate, beta,gamma-methyleneadenosine 5'-triphosphate, and UMP had little or no effect on the [Ca2+]i rise. Raising the extracellular Mg2+ concentration to 10 mM decreases the ATP- and UTP-induced [Ca2+]i rise, because the responses depend on the ATP4- and UTP4- concentrations, respectively. The P2U purinoceptor-selective agonist UTP and the P2Y purinoceptor-selective agonist ADP beta S induce inositol 1,4,5-trisphosphate generation in a concentration-dependent manner with maximal effective concentrations of approximately 100 microM. In sequential stimulation, UTP and ADP beta S do not interfere with each other in raising the [Ca2+]i. Costimulation with UTP and ADP beta S results in additive inositol 1,4,5-trisphosphate generation to a similar extent as is achieved with ATP alone. Pretreatment with pertussis toxin inhibits the action of UTP and ATP by maximally 45-55%, whereas it has no effect on the ADP beta S response. Treatment with 1 microM phorbol 12-myristate 13-acetate inhibits the ADP beta S-induced [Ca2+]i rise more effectively than the ATP- and UTP-induced responses. These results suggest that P2U and P2Y purinoceptors coexist on PGT-beta cells and that both receptors are linked to phospholipase C.

Published

1997

38. Expression of estrogen receptors in a normal human breast epithelial cell type with luminal and stem cell characteristics and its neoplastically transformed cell lines.

Author

Kang KS, Morita I, Cruz A, Jeon YJ, Trosko JE, and Chang CC

Subjects

Adult, Animals, Blotting, Western, Cell Cycle Proteins metabolism, Cell Line, Transformed chemistry, Cell Line, Transformed metabolism, DNA metabolism, Epithelium chemistry, Female, Humans, Mice, Mice, Nude, Neoplastic Stem Cells, Polymerase Chain Reaction, Receptors, Estrogen metabolism, Simian virus 40, Tumor Cells, Cultured chemistry, Tumor Cells, Cultured metabolism, Breast chemistry, Breast Neoplasms chemistry, Receptors, Estrogen analysis

Abstract

Although approximately two-thirds of breast cancers are estrogen receptor (ER)-positive, only a small proportion of epithelial cells in the mammary gland express the ER. The origin of the ER-positive breast cancers is unknown. Recently, we have developed a culture method to grow two morphologically and antigenically distinguishable types of normal human breast epithelial cells (HBEC) derived from reduction mammoplasty. In this report, we studied the expression of ER in these two types of cells and their transformed cell lines. The results indicate that Type I HBEC with luminal and stem cell characteristics expressed a variant ER (approximately 48 kd) by Western blot analysis. This variant ER contains a deletion in the DNA binding domain (exon 2) as revealed by RT-PCR analysis. The lack of the DNA-binding domain of the variant ER was also confirmed by the ER-estrogen responsive element binding assay, as well as by the immunofluorescence staining of the ER using anti-ER antibodies which recognize either the C-terminal or N-terminal region. In contrast, Type II HBEC with basal epithelial phenotype are ER-negative. Simian virus 40 (SV40) transformed Type I and Type II HBEC lines also expressed the variant ER. Tumors formed in athymic nude mice by in vitro transformed tumorigenic Type I cell lines, however, expressed a high level of wild type ER which was undetectable in these cells grown in vitro before and after tumor formation. Thus, there appears to be a differential ER mRNA splicing between the in vitro and in vivo mileu.

Published

1997

39. Receptors for natriuretic peptides in a human cortical collecting duct cell line.

Author

Millul V, Ardaillou N, Placier S, Baudouin B, and Ronco PM

Subjects

Atrial Natriuretic Factor pharmacology, Binding Sites physiology, Binding, Competitive physiology, Blotting, Northern, Cell Line, Transformed chemistry, Cell Line, Transformed metabolism, Cyclic GMP metabolism, Humans, Iodine Radioisotopes, Kidney Cortex cytology, Kidney Cortex ultrastructure, Kidney Tubules, Collecting chemistry, Polymerase Chain Reaction, RNA, Messenger analysis, Receptors, Atrial Natriuretic Factor chemistry, Transcription, Genetic physiology, Kidney Tubules, Collecting cytology, Receptors, Atrial Natriuretic Factor analysis, Receptors, Atrial Natriuretic Factor genetics

Abstract

The aim of the present study was to analyze the expression of natriuretic peptide receptors in human collecting duct, by using a newly established SV40 cell line (HCD). ANP and C-type natriuretic peptide (CNP) induced a concentration-dependent increase in cGMP suggesting the presence of type-A (NPR-A) and type-B (NPR-B) receptors, respectively. Threshold concentrations were 1 pM and 1 nM, respectively, and stimulated over basal cGMP ratios were 500 and 160 at 0.1 microM ANP and CNP. The urodilatin concentration-response curve was similar to that of ANP. [125I]-ANP bound specifically to HCD cells in a time-dependent fashion, reaching a plateau-phase between one and two hours at 4 degrees C. Equilibrium saturation binding curves suggested a single group of receptor sites (Kd = 421 +/- 55 pM, Bmax = 49.2 +/- 8.8 fmol/mg protein, Hill coefficient = 1.44 +/- 0.1, N = 6). Binding of [125I]-ANP was not displaced by CNP or by C-ANP (4-23), a specific ligand of clearance receptors (NPR-C), and thus occurred mainly via NPR-A. Neither Northern blot analysis nor RT-PCR could detect NPR-C mRNA, although the latter was clearly identified in control human glomerular visceral epithelial cells. In contrast, PCR products with the expected lengths were obtained for NPR-A and NPR-B. In conclusion, HCD cells express both NPR-A and NPR-B, as demonstrated by mRNA and cGMP production studies, but fail to produce NPR-C. This suggests that the human cortical collecting duct is a target for ANP, CNP and urodilatin.

Published

1997

40. Re-expression of interleukin 1 in human papillomavirus 18 immortalized keratinocytes inhibits their tumorigenicity in nude mice.

Author

Merrick DT, Winberg G, and McDougall JK

Subjects

Animals, Blotting, Northern, Carcinogenicity Tests, Cell Line, Transformed chemistry, Cell Line, Transformed physiology, Cell Line, Transformed transplantation, Enzyme-Linked Immunosorbent Assay, Female, Gene Expression Regulation, Neoplastic physiology, Humans, Interleukin-1 metabolism, Male, Mice, Mice, Inbred BALB C, Mice, Nude, Neoplasm Transplantation, Neoplasms, Glandular and Epithelial, Plasmids, RNA, Messenger analysis, Uterine Cervical Neoplasms, Interleukin-1 genetics, Keratinocytes cytology, Papillomaviridae

Abstract

The ability to form tumors in nude mice developed spontaneously in the human papillomavirus (HPV)-18 immortalized keratinocyte cell line, 18-11, and is shown here to be accompanied by a loss of interleukin 1 (IL-1) alpha and beta expression at both the RNA and protein level. In addition, a separate tumorigenic 18-11 derivative and two cervical carcinoma-derived cell lines, HeLa and Caski, were found to have significantly decreased or lost IL-1 alpha and IL-1 beta expression. Using retroviral expression vectors, we re-established IL-1 expression in tumorigenic 18-11 cells (18-11S3) in an effort to evaluate whether loss of IL-1 expression represented an important phenotypic change in the development of tumorigenicity in these cells. IL-1-expressing 18-11S3 cells showed a range of tumorigenic potential, depending on the type and combination of IL-1 alpha and IL-1 beta expressed. Although 18-11S3 expressing the precursor forms of both IL-1 alpha and IL-1 beta normally found in keratinocytes showed moderate inhibition of tumorigenicity, other IL-1-expressing lines showed complete inhibition of tumor formation. Co-injection of nontumorigenic, IL-1-expressing 18-11S3 with parental 18-11S3 also inhibited tumor formation. These results suggest that maintenance of IL-1 expression may play an important role in preventing progression to tumorigenicity in cervical carcinoma and other epithelial cancers.

Published

1996

41. Differentiation modulates the balance of positive and negative Jun/AP-1 DNA binding activities to regulate cellular proliferative potential: different effects in nontransformed and transformed cells.

Author

Wang H, Xie Z, and Scott RE

Subjects

3T3 Cells chemistry, Adipocytes cytology, Adipocytes physiology, Animals, Cell Differentiation physiology, Cell Division physiology, Cell Line, Transformed chemistry, Cell Line, Transformed cytology, DNA, Antisense pharmacology, DNA-Binding Proteins physiology, Gene Expression physiology, Mice, Protein Binding physiology, Proto-Oncogene Proteins c-jun analysis, Proto-Oncogene Proteins c-jun genetics, Transcription Factor AP-1 analysis, Transformation, Genetic, 3T3 Cells cytology, Transcription Factor AP-1 genetics

Abstract

Differentiation of 3T3T cells into adipocytes results in the progressive repression of growth factor responsiveness. This is associated with the transcriptional repression of the inducibility of c-jun and junB expression by serum. In contrast, differentiation of SV-40 large T antigen-transformed 3T3T cells (CSV3-1) does not repress growth factor responsiveness nor c-jun or junB inducibility even though CSV3-1 cells can differentiate into adipocytes. To better explain these observations, we have studied compositional changes in AP-1 DNA binding activity attributed to c-Jun, JunB, and JunD during the differentiation process in 3T3T and CSV3-1 cells. The results show that in nontransformed 3T3T cells, differentiation represses AP-1 DNA binding activity via a proportionate downregulation of c-Jun, JunB, and JunD. In contrast, in CSV3-1 cells, AP-1 DNA binding activity increases twofold during differentiation, which is accounted for by an increase in JunD with no change in c-Jun and JunB. If c-Jun and JunB serve as positive regulators and JunD serves as a negative regulator for cell proliferation as suggested by previous studies, the repression of JunD expression in differentiating CSV3-1 cells should be mitogenic because decreasing JunD/AP-1 DNA binding activity would allow c-Jun/AP-1 and JunB/AP-1 DNA binding activities to be dominant. The results confirm this prediction showing that antisense junD oligodeoxyribonucleotides are mitogenic for differentiating CSV3-1 cells whereas antisense c-jun and junB inhibit mitogenesis. These data support the conclusion that differentiation can regulate cellular proliferative potential by modulating the balance of positive and negative Jun/AP-1 DNA binding activities in distinct ways in nontransformed and transformed cells.

Published

1996

42. Characterization of antisera specific to NK1, NK2, and NK3 neurokinin receptors and their utilization to localize receptors in the rat gastrointestinal tract.

Author

Grady EF, Baluk P, Böhm S, Gamp PD, Wong H, Payan DG, Ansel J, Portbury AL, Furness JB, McDonald DM, and Bunnett NW

Subjects

Animals, Antibody Formation, Antibody Specificity, Blotting, Western, CHO Cells chemistry, Cell Line, Transformed chemistry, Cricetinae, Digestive System cytology, Enzyme-Linked Immunosorbent Assay, Epithelial Cells, Female, Fluorescent Antibody Technique, Immunohistochemistry, Kidney cytology, Male, Microscopy, Confocal, Muscle, Smooth cytology, Muscle, Smooth innervation, Rabbits, Rats, Receptors, Neurokinin-1 immunology, Receptors, Neurokinin-2 immunology, Receptors, Neurokinin-3 immunology, Tachykinins analysis, Tachykinins immunology, Transfection, Digestive System innervation, Neurons chemistry, Receptors, Tachykinin analysis, Receptors, Tachykinin immunology

Abstract

Understanding the physiological role of tachykinins requires precise cellular and subcellular localization of their receptors. We raised antisera by immunizing rabbits with peptides corresponding to portions of the intracellular tails of the rat neurokinin 1, 2, and 3 receptors (NK1-R, NK2-R, NK3-R). Receptors were localized by immunofluorescence and confocal microscopy. NK1-R, NK2-R, and NK3-R were detected at the plasma membrane of transfected cells with minimal intracellular stores. Staining was abolished by preabsorption of the antisera with the peptides used for immunization. Nontransfected cells were unstained. Each antiserum only stained cells transfected with the appropriate receptor and did not stain cells transfected with the other receptors. Therefore, the antisera are specific and do not cross-react with other neurokinin receptors. We examined the distribution of the neurokinin receptors in the gastrointestinal tract of the rat. NK1-R was detected in myenteric and submucosal neurons and in interstitial cells of Cajal. NK2-R was localized to circular and longitudinal muscle cells and to nerve endings in the plexuses. NK3-R was detected in numerous myenteric and submucosal neurons. Some neurons expressed both NK1-R and NK3-R. Receptors were detected at the plasma membrane and in endosomes. Cells expressing the receptors were closely associated with tachykinin-containing nerve fibers. Thus, NK1-R and NK3-R mediate neurotransmission by tachykinins within enteric nerve plexuses, and NK1-R and NK2-R mediate the effects of tachykinins on interstitial and smooth muscle cells, respectively.

Published

1996

43. Calcium binding proteins in normal and transformed cells, Perugia, May 1996.

Author

Williams RJ

Subjects

Cell Line chemistry, Cell Line, Transformed chemistry, Calcium-Binding Proteins physiology

Published

1996

44. Identification of resting cells by dual-parameter flow cytometry of statin expression and DNA content.

Author

Pellicciari C, Mangiarotti R, Bottone MG, Danova M, and Wang E

Subjects

3T3 Cells chemistry, Animals, Antigens, Neoplasm, Apoptosis drug effects, Biomarkers, Breast Neoplasms chemistry, Bromodeoxyuridine, Cell Cycle Proteins, Cell Division drug effects, Cell Division physiology, Cell Line, Transformed chemistry, Estrogen Antagonists pharmacology, Estrogens pharmacology, Female, Fixatives, Fluorescent Antibody Technique, Formaldehyde, Gene Expression, Glioma chemistry, Humans, Ki-67 Antigen, Mice, Neoplasm Proteins, Nuclear Proteins, Polymers, Proliferating Cell Nuclear Antigen, Propidium, Proteins genetics, Rats, Tamoxifen pharmacology, Thymus Gland cytology, DNA, Neoplasm analysis, Flow Cytometry, Proteins analysis, Resting Phase, Cell Cycle physiology

Abstract

Statin, a 57-kDa nuclear protein, has been recognized as a unique marker of quiescent (G0) cells; specific monoclonal antibodies (MoAb) against statin have been produced and used to label resting cells in tissue sections and in cultured cells. We present an improved method for the identification of G0 cells by dual-parameter flow cytometry of statin expression and DNA content. The appropriate technical conditions were set up by using resting and cycling human fibroblasts as a model cell system. Several fixatives proved to be suitable for the immunocytochemical detection of statin; among them, 70% ethanol was selected because this fixation procedure is suitable for DNA staining with intercalating dyes and is routinely used for the immunolabeling of proliferation markers (such as proliferating cell nuclear antigen [PCNA] and Ki-67) and of bromodeoxyuridine (BrdUrd) incorporation. Following cell permeabilization with detergent, exposure to the antistatin antibody (S-44), and indirect fluorescein isothiocyanate immunolabeling, cells were counterstained for DNA with propidium iodide and analyzed by dual-parameter flow cytometry. In cells from several animal sources (rat thymocytes and C6 glioma cells, mouse 3T3 cells, and human MCF-7 cells), under different experimental conditions, the expression of statin was found to correlate inversely with that of PCNA and Ki-67, and with the BrdUrd labeling index. In dual-parameter flow scattergrams, G0 (statin positive) cells can be discriminated from the potentially cycling (statin negative) G1 cells, i.e., within a cell fraction having the same DNA content. This approach can be envisaged as a powerful tool both for monitoring changes in the resting cell fraction and for investigating the process of G0-G1 transition in unperturbed and drug-treated cell populations.

Published

1995

45. Correlation between complementation group for immortality and the cellular distribution of mortalin.

Author

Wadhwa R, Pereira-Smith OM, Reddel RR, Sugimoto Y, Mitsui Y, and Kaul SC

Subjects

Animals, Carrier Proteins, Cell Line, Transformed cytology, Cell Survival, Genetic Complementation Test, Humans, Mice, Mitochondrial Proteins, Tumor Cells, Cultured cytology, Cell Line, Transformed chemistry, Cellular Senescence physiology, HSP70 Heat-Shock Proteins, Heat-Shock Proteins analysis, Tumor Cells, Cultured chemistry

Abstract

The dominance of cellular senescence over the immortal phenotype has been demonstrated by cell fusion experiments utilizing human and mouse cells. Mortalin, a novel 66-kDa member of the murine hsp70 family of proteins, has recently been identified as a marker of the mortal phenotype by virtue of its characteristic cytosolic distribution in mortal cells. Here we report the mortalin immunostaining observations on 21 human cell lines. These cell lines have previously been assigned by somatic cell hybridization analysis to one (18 lines) or more than one (3 lines) of the four complementation groups (A, B, C, and D) for immortalization. Four patterns of mortalin immunostaining were observed: granular-juxtanuclear cap, granular-gradient from nuclear to cell membrane, granular-juxtanuclear arch, and fibrous-perinuclear. In 17 of 18 cell lines assigned to a single complementation group, the mortalin staining corresponded with the complementation group. In two of the three cell lines previously assigned to multiple complementation groups, the mortalin staining corresponded to one of the assigned groups. Two cell lines, however, exhibited staining patterns which did not match to their assigned complementation groups. The basis of correlation between cellular distribution of mortalin and the complementation group remains unclear at present. However, the data (i) suggest that the intracellular distribution of mortalin can be used to distinguish mortal and immortal cells, confirming the association of mortalin with senescence; (ii) provide supportive evidence for the existence of at least four different pathways of immortalization in human cells; and (iii) indicate that mortalin is involved in processes that result in immortalization.

Published

1995

46. Establishment of a human retinal cell line by transfection of SV40 T antigen gene with potential to undergo neuronal differentiation.

Author

Dutt K, Scott M, Wang M, Semple E, Sharma GP, and Srinivasan A

Subjects

Cell Differentiation, Cell Division, Cell Line, Transformed chemistry, Cell Line, Transformed drug effects, Cyclic AMP pharmacology, Embryo, Mammalian, Eye Proteins analysis, Humans, Nerve Tissue Proteins analysis, Phorbol Esters pharmacology, Simian virus 40 genetics, Transfection, Antigens, Polyomavirus Transforming genetics, Cell Line, Transformed cytology, Retina cytology

Abstract

Recently, a number of laboratories have been interested in developing cell lines of ocular tissues to understand the pathogenesis of ocular diseases. Toward this end, we report here the generation of cell lines of human retina by transfection of simian virus SV40 T antigen gene. Established retinal cells grow as a monolayer and exhibit limited serum dependence. Phase-contrast and electron microscopic studies revealed distinct morphological cell types. Immunofluorescence studies showed that the established retinal cells were positive for neuron-specific enolase, neurofilament protein, glycine receptor, synaptophysin, and secretogranin. Cells were negative for glial fibrillary acidic protein, glutamine synthetase, galactocerebroside, and carbonic anhydrase II. In addition to neuronal features, a small percentage of flat cells were, however, positive for cellular retinaldehyde binding protein, and cells with the phenotype of rod and cone photoreceptor coexpressed opsin and interphotoreceptor retinoid-binding protein. An important feature of this cell line is that addition of phorbol ester and cAMP induced dramatic changes, with 100% of the cells extending long, thin neuritic processes. Thus, the established retinal cells would be useful for studies dealing with differentiation and plasticity of the cells of the nervous system.

Published

1994

47. Transformation and immortalization of Leydig cells from the Sprague-Dawley rat by an early genetic region of simian virus 40 DNA.

Author

Nagpal ML, Wang D, Calkins JH, and Lin T

Subjects

Animals, Carrier Proteins genetics, Cell Division, Cell Line, Transformed chemistry, Cell Line, Transformed cytology, DNA, Viral analysis, Gene Expression, Insulin-Like Growth Factor Binding Protein 2, Insulin-Like Growth Factor I genetics, Leydig Cells chemistry, Male, RNA, Messenger analysis, RNA, Viral analysis, Rats, Rats, Sprague-Dawley, Receptors, LH genetics, Receptors, Somatomedin genetics, Somatomedins genetics, Antigens, Polyomavirus Transforming genetics, Cell Transformation, Viral, Leydig Cells cytology, Simian virus 40 genetics

Abstract

Two transformed cell lines of rat Leydig cells were established by transfection of primary cells with the transforming region of simian virus (SV40) DNA. Normal adult Leydig cells are non-proliferating cells and cease to grow after the first trypsinization for cell culturing. The cell lines, NWL2 and NWL15, continued to proliferate and subsequently needed subculturing every 2 weeks (split ratio 1:2). No crisis was observed after 35 passages for 18 months. Nile red staining showed the presence of lipid droplets in both normal and transformed cells, although the transformed cells had 2-3-fold higher amounts than the normal cells. The integration of T-antigen DNA has taken place in at least 2 and 1 sites in NWL2 and NWL15, respectively. Both cell lines expressed T-antigen mRNA. The cell lines expressed luteinizing hormone receptor (LH-R) (a Leydig cell-specific gene), insulin-like growth factor-I, insulin-like growth factor-I receptor (IGF-I-R) and insulin-like growth factor binding protein-2 (IGFBP-2) genes. The amounts of transcripts of LH-R were lower in the transformed cells as compared to the normal cells. The IGF-I-R mRNA levels were comparable to those of the normal Leydig cells. NWL2 and NWL15 cells also expressed IGF-I mRNA although to a lesser extent than the normal Leydig cells. IGFBP-2 mRNA levels were much higher in both the transformed cell lines than in the normal Leydig cells. The transformed cells were evaluated for the expression of P450scc, which catalyzes the conversion of cholesterol to pregnenolone.(ABSTRACT TRUNCATED AT 250 WORDS)

Published

1994

48. Characterization of immortalized mouse granulosa cell lines.

Author

Briers TW, van de Voorde A, and Vanderstichele H

Subjects

17-Hydroxysteroid Dehydrogenases metabolism, 3-Hydroxysteroid Dehydrogenases metabolism, Activins, Animals, Cell Division drug effects, Cell Line, Transformed chemistry, Cell Line, Transformed cytology, Culture Media, Conditioned, Female, Granulosa Cells chemistry, Granulosa Cells cytology, Growth Substances pharmacology, Inhibins metabolism, Karyotyping, Mice, Prostaglandins metabolism, Proto-Oncogene Proteins c-myc analysis, Steroids analysis, Transforming Growth Factor beta metabolism, Cell Line, Transformed physiology, Granulosa Cells physiology

Abstract

Cell cultures of primary mouse granulosa cells were transfected with a v-myc-containing plasmid, and the resulting stable cell lines were tested for their steroidogenic properties and physiologic status. Granulosa cells were obtained from 22-day-old NMRI mice injected with 8 IU pregnant mare serum gonadotropin i.p. 2 days earlier. In Passage 1 the cells were transfected with pSVv-myc using calcium phosphate precipitation or lipofectin. The 3 beta- and 17 beta-hydroxy steroid dehydrogenase activity was visualized in control cultures. The three cell lines obtained have been in culture for over 1 yr and have been subcultured for more than 90 passages. The cell line GRM01, with a doubling time of 37 +/- 3 h and a diploid modal chromosome number, produced progesterone, estradiol, as well as inhibinlike and activinlike material under basal conditions. A combination of follicle-stimulating hormone and luteinizing hormone was able to increase the secretion of progesterone. GRM01L, a fast growing clone of the GRM01 line with a doubling time of 10 +/- 1 h, retained only the capacity to produce activinlike material and transforming growth factor-beta, and it was the only one with a tumorigenic capacity. Epidermal growth factor, insulin, and interleukin-6 were able to induce the [3H]thymidine incorporation into DNA in these two cell lines. GRM02, with a doubling time of 36 +/- 2 h and a hypertriploid modal chromosome number, produced progesterone and activinlike and inhibinlike material. Follicle-stimulating hormone and luteinizing hormone were able to enhance the secretion of progesterone. For this cell line, only insulin was shown to induce [3H]thymidine incorporation into DNA.

Published

1993

49. Malignant cells have increased levels of common glycoprotein ligands of the endogenous cerebellar soluble lectin CSL.

Author

Maschke S, Robert J, Coindre JM, Kuchler S, Vincendon G, and Zanetta JP

Subjects

Animals, Cells, Cultured, Concanavalin A metabolism, Glycoproteins metabolism, Humans, Ligands, Neoplasm Proteins metabolism, Cell Line, Transformed chemistry, Glycoproteins analysis, Lectins metabolism, Neoplasm Proteins analysis, Tumor Cells, Cultured chemistry

Abstract

The glycoprotein composition of various transformed cells or malignant tumors was analyzed and compared to their respective non-malignant control cells or tissues of several species, including man, using an endogenous carbohydrate-binding protein, the cerebellar soluble lectin CSL (Zanetta et al., J. Neurochem. 49, 1250-1257 (1987). A large variety of transformed cells contain a much higher number and larger quantity of glycoprotein ligands of CSL than the control cells or normal tissues. The glycoprotein profiles were, in most cases, independent of the nature of the cell transformation of the degree of differentiation, of the tissue and species. Thus, it is suggested that many transformed cells have, as a common anomaly, the increased synthesis of the special type of glycan recognized by CSL, expressed on the same polypeptide chains.

Published

1993

50. Lipid composition and synthesis of HaCaT cells, an immortalized human keratinocyte line, in comparison with normal human adult keratinocytes.

Author

Schürer N, Köhne A, Schliep V, Barlag K, and Goerz G

Subjects

Adult, Calcium pharmacology, Cell Differentiation, Cell Division, Cell Line, Transformed chemistry, Cholesterol metabolism, Contact Inhibition, Fatty Acids metabolism, Humans, Keratinocytes chemistry, Lipids analysis, Phospholipids metabolism, Receptors, LDL metabolism, Sphingolipids metabolism, Cell Line, Transformed metabolism, Keratinocytes metabolism, Lipids biosynthesis

Abstract

Cultured keratinocytes are frequently employed for studies of epidermal lipid metabolism. Interpretation of experimental data may be complicated by donor to donor variability, the relatively short culture lifetime and variations between passages, problems that are not encountered to the same extent with immortalized cell lines. The present study was undertaken to compare the lipid composition and synthesis of normal human adult keratinocytes (NHAK) with HaCaT cells, a long-lived, spontaneously immortalized human keratinocyte line, in relation to proliferation and differentiation. No differences between the two cell types were observed: a) in total lipid content; b) in the distribution of major lipid classes during growth at 50%, 75% and 100% confluence; c) in cultures grown at 0.6 mM calcium, at which differentiation is retarded, or at 1.6 mM calcium, at which some differentiation takes place; d) in the incorporation of [14C] acetate into cellular lipids at confluence, or e) in the fatty acid composition of major cellular lipid classes. At 100% confluence NHAK and HaCaT cells differ in their cholesterol metabolism. At all stages of growth, cholesterol synthesis in HaCaT cells is more LDL-dependent than in NHAK. Furthermore, NHAK become less LDL-dependent at confluence whereas HaCaT cells do not. HaCaT cells also revealed a significantly larger fraction of phosphatidyl-ethanolamine, -serine and -inositol at 0.6 mM calcium concentration than NHAK. These findings suggest that HaCaT cells do not differentiate as well as NHAK in vitro and may therefore serve as a model for the study of lipid metabolism in cells defective in terminal differentiation.

Published

1993