Your search keyword '"Iacovoni JS"' showing total 4 results

1. HuR-dependent loading of miRNA RISC to the mRNA encoding the Ras-related small GTPase RhoB controls its translation during UV-induced apoptosis.

Author

Glorian V, Maillot G, Polès S, Iacovoni JS, Favre G, and Vagner S

Subjects

3' Untranslated Regions, Binding Sites, Cell Line, ELAV Proteins antagonists & inhibitors, ELAV Proteins genetics, Humans, Luciferases, Firefly genetics, Luciferases, Firefly metabolism, Protein Binding, RNA Interference, RNA, Small Interfering metabolism, rhoB GTP-Binding Protein genetics, Apoptosis radiation effects, ELAV Proteins metabolism, MicroRNAs metabolism, RNA, Messenger metabolism, Ultraviolet Rays, rhoB GTP-Binding Protein metabolism

Abstract

Of critical importance in the stress response is the post-transcriptional control of the expression of important genes involved in the control of cell survival and apoptosis. Here we report that miR-19, an oncogenic component of the miR-17-92/Oncomir-1 microRNA polycistron, regulates the expression of Ras homolog B (RhoB) in keratinocytes upon exposure to ultraviolet (UV) radiation. Strikingly, we could not find any evidence for deregulated expression of miR-19 during UV treatment. However, we show that miR-19-mediated regulation of antiapoptotic RhoB expression requires the binding of human antigen R (HuR), an AU-rich element binding protein, to the 3'-untranslated region of the rhoB mRNA. We propose that the loss of the interdependent binding between HuR and miR-19 to the rhoB mRNA upon UV exposure relieves this mRNA from miR-19-dependent inhibition of translation and contributes to the apoptotic response.

Published

2011

2. v-Jun targets showing an expression pattern that correlates with the transformed cellular phenotype.

Author

Iacovoni JS, Cohen SB, Berg T, and Vogt PK

Subjects

Animals, Mice, Oligonucleotide Array Sequence Analysis, Phenotype, Protein Array Analysis, Up-Regulation, Cell Transformation, Neoplastic, Proto-Oncogene Proteins c-jun physiology

Abstract

Targets of the oncogenic transcription factor v-Jun in the murine cell line C3H 10T1/2 cells have been identified using DNA microarrays. Two targets, Akap12 and Marcks, are downregulated in transformed cells and are known tumor suppressor genes. Overexpression of either Akap12 or Marcks in v-Jun-transformed cells reverses the transformed phenotype and leads to the re-expression of the other tumor suppressor gene, suggesting that these two genes cooperate in the establishment of the nontransformed state. Reverted cells continue to express v-Jun at high levels and also re-express c-Jun, which is normally repressed by v-Jun. A panel of six cell lines has been generated to evaluate the expression levels of other v-Jun targets in 10T1/2 cells. With these cells, we find that the upregulated target Sprr1a has an expression pattern that correlates with the transformed phenotype., (Copyright 2004 Nature Publishing Group)

Published

2004

3. Glutaredoxin is a direct target of oncogenic jun.

Author

Goller ME, Iacovoni JS, Vogt PK, and Kruse U

Subjects

Animals, Chick Embryo, GAP-43 Protein genetics, Gene Expression Regulation, Glutaredoxins, Oncogene Protein p65(gag-jun) genetics, Oxidoreductases, Proteins genetics

Abstract

We have analysed differential gene expression in v-jun-transformed chicken embryo fibroblasts (CEF) compared to normal CEF by using the directional tag PCR subtraction method. From a first generation of putative Jun targets four clones were selected for study; they are upregulated in jun-transformed cells. Three of these clones showed homology to known genes: glutaredoxin, growth associated protein (GAP)-43/neuromodulin, and phenobarbital-induced cytochrome P450. The expression of these genes was analysed in fibroblasts transformed by various oncogenes. Expression of the glutaredoxin mRNA could be induced by a Jun-estrogen receptor chimaera in the absence of de novo protein biosynthesis. Based on this observation we conclude that glutaredoxin is a direct target of v-Jun.

Published

1998

4. Avian winged helix proteins CWH-1, CWH-2 and CWH-3 repress transcription from Qin binding sites.

Author

Freyaldenhoven BS, Freyaldenhoven MP, Iacovoni JS, and Vogt PK

Subjects

Binding Sites, DNA metabolism, Avian Proteins, DNA-Binding Proteins physiology, Repressor Proteins physiology, Transcription Factors physiology

Abstract

The chicken winged helix proteins, CWH-1, CWH-2 and CWH-3, were isolated and identified by homology cloning using the winged helix sequence of the retroviral oncogene qin as a probe. The CWH proteins act as growth stimulators in chicken embryo fibroblasts and in this activity resemble the Qin protein. Qin is a transcriptional regulator that functions as a repressor, and its oncogenic potential is correlated with the ability to repress transcription. In this communication we show that CWH proteins are localized in the cell nucleus, recognize the Qin DNA binding site and also function as transcriptional repressors. The repression activity of CWH-3 was mapped to the region of amino acids 211 to 311, a domain that is homologous to the major repression domain of Qin.

Published

1997