Your search keyword '"Pouponnot C"' showing total 58 results

51. Comparison of maf gene expression patterns during chick embryo development.

Author

Lecoin L, Sii-Felice K, Pouponnot C, Eychène A, and Felder-Schmittbuhl MP

Subjects

Animals, Chick Embryo, Gastrula metabolism, Gene Expression Regulation, Developmental, In Situ Hybridization, Limb Buds embryology, Limb Buds metabolism, MafF Transcription Factor, MafK Transcription Factor, Mesoderm metabolism, Nuclear Proteins genetics, Pancreas embryology, Pancreas metabolism, Peripheral Nervous System embryology, Peripheral Nervous System metabolism, Proto-Oncogene Proteins c-maf, Repressor Proteins genetics, Retina embryology, Retina metabolism, Spinal Cord embryology, Spinal Cord metabolism, DNA-Binding Proteins genetics, Gene Expression Profiling, Proto-Oncogene Proteins genetics

Abstract

Maf proteins are basic-leucine zipper transcription factors belonging to the AP1 superfamily. Several developmental processes require Maf proteins yet, the redundancy or complementarity of their respective roles in common processes has been only partially investigated. We present for the first time a complete comparative analysis of maf gene expression patterns in vertebrates. Expression of c-maf, mafB/kreisler, mafA/L-maf, mafF, mafG and mafK was analyzed by whole-mount in situ hybridization within chick embryos and their extraembryonic tissues ranging from embryonic day (E) 1 to 7. We carefully examined the extent of overlap between distinct maf genes and report that the developing lens, kidney, pancreas and apoptotic zones of limb buds show sustained co-expression of large maf genes. Small maf genes also exhibit overlap, for example in the dermomyotome. We also describe so far unidentified sites of maf gene expression. mafA is found in the developing neural tube and dorsal root ganglia. c-maf hybridization is detected in the neuroretina, the notochord and the endothelium of extraembryonic blood vessels.

Published

2004

52. Mutation of B-Raf in human choroidal melanoma cells mediates cell proliferation and transformation through the MEK/ERK pathway.

Author

Calipel A, Lefevre G, Pouponnot C, Mouriaux F, Eychène A, and Mascarelli F

Subjects

Cell Cycle Proteins analysis, Cell Division, Gene Expression Profiling, Humans, MAP Kinase Kinase 1, Mitogen-Activated Protein Kinase 3, Oncogene Proteins analysis, Oncogene Proteins metabolism, Proto-Oncogene Proteins B-raf, RNA, Small Interfering pharmacology, Signal Transduction genetics, Tumor Cells, Cultured, ras Proteins, Choroid Neoplasms pathology, Melanoma pathology, Mitogen-Activated Protein Kinase Kinases metabolism, Mitogen-Activated Protein Kinases metabolism, Mutation, Oncogene Proteins genetics, Protein Serine-Threonine Kinases metabolism

Abstract

The BRAF gene, encoding a mitogen-activated protein kinase kinase kinase, is mutated in several human cancers, with the highest incidence occurring in cutaneous melanoma. The activating V599E mutation accounted for 80% of all mutations detected in cutaneous melanoma cell lines. Reconstitution experiments have shown that this mutation increases ectopically expressed B-Raf kinase activity and induces NIH3T3 cell transformation. Here we used tumor-derived cell lines to characterize the activity of endogenous mutated B-Raf protein and assess its specific role in transformation. We show that three cell lines (OCM-1, MKT-BR, and SP-6.5) derived from human choroidal melanoma, the most frequent primary ocular neoplasm in humans, express B-Raf containing the V599E mutation. These melanoma cells showed a 10-fold increase in endogenous B-RafV599E kinase activity and a constitutive activation of the MEK/ERK pathway that is independent of Ras. This, as well as melanoma cell proliferation, was strongly diminished by siRNA-mediated depletion of the mutant B-Raf protein. Moreover, blocking B-RafV599E-induced ERK activation by different experimental approaches significantly reduced cell proliferation and anchorage-independent growth of melanoma cells. Finally, quantitative immunoblot analysis allowed us to identify signaling and cell cycle proteins that are differentially expressed between normal melanocytes and melanoma cells. Although the expression of signaling molecules was not sensitive to U0126 in melanoma cells, the expression of a cluster of cell cycle proteins remained regulated by the B-RafV599E/MEK/ERK pathway. Our results pinpoint this pathway as an important component in choroidal melanoma cell lines.

Published

2003

53. TGFbeta influences Myc, Miz-1 and Smad to control the CDK inhibitor p15INK4b.

Author

Seoane J, Pouponnot C, Staller P, Schader M, Eilers M, and Massagué J

Subjects

Animals, Base Sequence, COS Cells, Chlorocebus aethiops, Cyclin-Dependent Kinase Inhibitor p15, DNA-Binding Proteins genetics, Gene Silencing, Humans, Kruppel-Like Transcription Factors, Mice, Molecular Sequence Data, Promoter Regions, Genetic, Proto-Oncogene Mas, Proto-Oncogene Proteins c-myc genetics, Response Elements, Smad2 Protein, Smad3 Protein, Smad4 Protein, Smad7 Protein, Trans-Activators genetics, Transcription Factors, Transcriptional Activation, Carrier Proteins genetics, Cell Cycle Proteins, Cyclin-Dependent Kinase Inhibitor p16, Cyclin-Dependent Kinases antagonists & inhibitors, DNA-Binding Proteins metabolism, Proto-Oncogene Proteins c-myc metabolism, Trans-Activators metabolism, Transforming Growth Factor beta metabolism, Tumor Suppressor Proteins, Zinc Fingers

Abstract

Transforming growth factor-beta (TGFbeta) is a cytokine that arrests epithelial cell division by switching off the proto-oncogene c-myc and rapidly switching on cyclin-dependent kinase (CDK) inhibitors such as p15INK4b. Gene responses to TGFbeta involve Smad transcription factors that are directly activated by the TGFbeta receptor. Why downregulation of c-myc expression by TGFbeta is required for rapid activation of p15INK4b has remained unknown. Here we provide evidence that TGFbeta signalling prevents recruitment of Myc to the p15INK4b transcriptional initiator by Myc-interacting zinc-finger protein 1 (Miz-1). This relieves repression and enables transcriptional activation by a TGFbeta-induced Smad protein complex that recognizes an upstream p15INK4b promoter region and contacts Miz-1. Thus, two separate TGFbeta-dependent inputs - Smad-mediated transactivation and relief of repression by Myc - keep tight control over p15INK4b activation.

Published

2001

54. Inhibition of the transforming growth factor beta 1 signaling pathway by the AML1/ETO leukemia-associated fusion protein.

Author

Jakubowiak A, Pouponnot C, Berguido F, Frank R, Mao S, Massague J, and Nimer SD

Subjects

3T3 Cells, Animals, Base Sequence, COS Cells, Core Binding Factor Alpha 2 Subunit, DNA Primers, Mice, RUNX1 Translocation Partner 1 Protein, Oncogene Proteins, Fusion metabolism, Signal Transduction, Transcription Factors metabolism, Transforming Growth Factor beta metabolism

Abstract

The t(8;21) translocation, found in adult acute myelogenous leukemia, results in the formation of an AML1/ETO chimeric transcription factor. AML1/ETO expression leads to alterations in hematopoietic progenitor cell differentiation, although its role in leukemic transformation is not clear. The N-terminal portion of AML1, which is retained in AML1/ETO, contains a region of homology to the FAST proteins, which cooperate with Smads to regulate transforming growth factor beta1 (TGF-beta1) target genes. We have demonstrated the physical association of Smad proteins with AML1 and AML1/ETO by immunoprecipitation and have mapped the region of interaction to the runt homology domain in these AML1 proteins. Using confocal microscopy, we demonstrated that AML1, and ETO and/or AML1/ETO, colocalize with Smads in the nucleus of t(8;21)-positive Kasumi-1 cells, in the presence but not the absence of TGF-beta1. Using transient transfection assays and a reporter gene construct that contains both Smad and AML1 consensus binding sequences, we demonstrated that overexpression of AML1B cooperates with TGF-beta1 in stimulating reporter gene activity, whereas AML1/ETO represses basal promoter activity and blocks the response to TGF-beta1. Considering the critical role of TGF-beta1 in the growth and differentiation of hematopoietic cells, interference with TGF-beta1 signaling by AML1/ETO may contribute to leukemogenesis.

Published

2000

55. Characterization of a novel quiescence responsive element downregulated by v-Src in the promoter of the neuroretina specific QR1 gene.

Author

Provot S, Pouponnot C, Lecoq O, Calothy G, and Felder-Schmittbuhl MP

Subjects

Animals, Avian Sarcoma Viruses genetics, Base Sequence, Binding Sites, Coturnix genetics, Culture Media, Serum-Free pharmacology, DNA genetics, DNA metabolism, Gene Expression Regulation genetics, Macromolecular Substances, Recombinant Fusion Proteins biosynthesis, Retina metabolism, Temperature, Transcription, Genetic, Transfection, Cell Division genetics, Eye Proteins genetics, Oncogene Protein pp60(v-src) physiology, Promoter Regions, Genetic genetics, Regulatory Sequences, Nucleic Acid

Abstract

The neuroretina is a functional unit of the central nervous system which arises through successive steps of division, growth arrest and differentiation of neuroectodermal precursors. Postmitotic quail neuroretina (QNR) cells are conditionally induced to divide upon infection with temperature sensitive mutants of Rous sarcoma virus (RSV), since QNR cell division can be arrested by either inactivating p60v-Src at the nonpermissive temperature (41 degrees C) or by serum deprivation at 37 degrees C. We are studying the transcriptional control of QR1, a neuroretina specific gene, whose expression is down-regulated in proliferating cells at 37 degrees C and is fully restored when these cells are made quiescent. We previously showed that this quiescence specific upregulation implicates a promoter region named A box, which binds Maf transcription factors. We report the identification of the C box, a second promoter sequence that activates QR1 transcription in non dividing cells. This sequence is able to form two DNA-protein complexes, one of which (C4) is predominantly detected in growth arrested NR cells. We identified the DNA binding site for C4 and described mutations that abolish both C4 binding and promoter activity in quiescent cells. Moreover, we show that a multimerized C box is able to stimulate a heterologous promoter in non dividing cells and constitutes, therefore, a novel quiescence responsive enhancer. Finally, we report that QR1 transcriptional response to cell quiescence requires cooperation between the C box and A box.

Published

2000

56. Transforming growth factor beta -inducible independent binding of SMAD to the Smad7 promoter.

Author

Denissova NG, Pouponnot C, Long J, He D, and Liu F

Subjects

Base Sequence, Humans, Molecular Sequence Data, RNA, Messenger analysis, Smad3 Protein, Smad4 Protein, Smad7 Protein, DNA-Binding Proteins genetics, DNA-Binding Proteins metabolism, Promoter Regions, Genetic, Trans-Activators genetics, Trans-Activators metabolism, Transforming Growth Factor beta pharmacology

Abstract

SMAD proteins can mediate transforming growth factor beta (TGF-beta)-inducible transcriptional responses. Whereas SMAD can recognize specific DNA sequences, it is usually recruited to a promoter through interaction with a DNA-binding partner. In an effort to search for TGF-beta-inducible genes, we used a subtractive screening method and identified human Smad7, which can antagonize TGF-beta signaling and is rapidly up-regulated by TGF-beta. In this report, we show that TGF-beta can stabilize Smad7 mRNA and activate Smad7 transcription. The Smad7 promoter is the first TGF-beta responsive promoter identified in vertebrates that contains the 8-bp palindromic SMAD-binding element (SBE), an optimal binding site previously identified by a PCR-based selection from random oligonucleotides by using recombinant Smad3 and Smad4. We demonstrate that on TGF-beta treatment, endogenous SMAD complex can bind to a Smad7 promoter DNA as short as 14 or 16 bp that contains the 8-bp SBE in gel mobility shift and supershift assays. Our studies provide strong evidence that SMAD proteins can bind to a natural TGF-beta responsive promoter independent of other sequencespecific transcription factors. We further show that, whereas recombinant Smad3 binds to the SBE, endogenous or even transfected Smad3 cannot bind to the SBE in the absence of Smad4. These findings have important implications in the identification of target genes of the TGF-beta/SMAD signaling pathways.

Published

2000

57. mafA, a novel member of the maf proto-oncogene family, displays developmental regulation and mitogenic capacity in avian neuroretina cells.

Author

Benkhelifa S, Provot S, Lecoq O, Pouponnot C, Calothy G, and Felder-Schmittbuhl MP

Subjects

Amino Acid Sequence, Animals, Base Sequence, DNA-Binding Proteins metabolism, Dimerization, Eye Proteins biosynthesis, Eye Proteins genetics, Mitogens genetics, Molecular Sequence Data, Oncogene Protein v-maf, Oncogene Proteins metabolism, Oncogene Proteins, Viral metabolism, Promoter Regions, Genetic, Proto-Oncogene Proteins genetics, Proto-Oncogene Proteins c-fos metabolism, Proto-Oncogene Proteins c-jun metabolism, Sequence Homology, Amino Acid, Trans-Activators genetics, Transcriptional Activation, Avian Proteins, Gene Expression Regulation, Neurons cytology, Proto-Oncogene Proteins metabolism, Quail genetics, Retina cytology, Trans-Activators metabolism, Transcription Factors, Viral Proteins

Abstract

Transcription factors of the Maf proto-oncogene family have been shown to participate in the regulation of several differentiation specific genes. We previously reported that a member(s) of this family is involved in the regulation of the neuroretina specific gene, QR1, through a promoter region, designated the A box, that is closely related to the Maf recognition element (MARE). We undertook an identification of Maf family genes expressed in the quail neuroretina (QNR) and we report the isolation of mafA, a gene encoding a novel member of the large Maf proteins subgroup. Expression of this gene is developmentally regulated in the neuroretina. MafA is able to bind to MARE sequence and to heterodimerize with v-Maf, MafB, Jun and Fos, but not with the small MafF and MafK proteins. Accordingly, it is able to transactivate the QR1 promoter A box. We also show that increased expression of mafA induces sustained proliferation of postmitotic QNR cells.

Published

1998

58. QRI, a retina-specific gene, encodes an extracellular matrix protein exclusively expressed during neural retina differentiation.

Author

Casado FJ, Pouponnot C, Jeanny JC, Lecoq O, Calothy G, and Pierani A

Subjects

Animals, Cell Differentiation genetics, Cell Division genetics, Retina cytology, Retina metabolism, Coturnix embryology, Eye Proteins genetics, Gene Expression Regulation, Developmental, Retina embryology

Abstract

Neural retina development results from growth arrest of neuroectodermal precursors and differentiation of postmitotic cells. The QRI gene is specifically expressed in Müller retinal glial cells. Its expression coincides with the stage of withdrawal from the cell cycle and establishment of differentiation and is repressed upon induction of retinal cell proliferation by the v-src gene product. In this report, we show that the QR1 gene encodes several glycosylated proteins that are secreted and can either associate with the extracellular matrix or remain diffusible in the medium. By using pulse-chase experiments, the 100-103 kDa forms seem to appear first and are specifically incorporated into the extracellular matrix, whereas the 108 and 60 kDa polypeptides appear later and are detected as soluble forms in the culture medium. We also report that expression of the QR1 gene is developmentally regulated in the chicken. Its mRNA is first detectable at embryonic day 10, reaches a maximal level at embryonic day 15 and is no longer detected at embryonic day 18. Immunolocalization of the QR1 protein in chicken retina sections during development shows that expression of the protein parallels the differentiation pattern of post-miotic cells (in particular Müller cells and rods), corresponding to the two differentiation gradients in the retina: from the ganglion cell layer to the inner nuclear layer and outer nuclear layer, and from the optic nerve to the iris. At embryonic day 10, expression of the QR1 protein(s) is restricted to the optic nerve region and the inner nuclear layer, colocalizing with Müller cell bodies. As development proceeds, QR1 protein localization spreads towards the iris and towards the outer nuclear layer, following Müller cell elongations towards the photoreceptors. Between embryonic days 16 and 18, the QR1 protein is no longer detectable in the optic nerve region and is concentrated around the basal segment of the photoreceptors in the peripheral retina. Our results suggest a role for the QR1 gene product in the process of growth arrest and establishment of photoreceptor differentiation.

Published

1996