Your search keyword '"André, Charlotte"' showing total 6 results

1. Polarized expression of the membrane ASP protein derived from HIV-1 antisense transcription in T cells

Author

Gay Bernard, Arpin-André Charlotte, Vargas Amandine, Borel Sophie, Landry Sébastien, Torresilla Cynthia, Laverdure Sylvain, Clerc Isabelle, Briant Laurence, Gross Antoine, Barbeau Benoît, and Mesnard Jean-Michel

Subjects

Immunologic diseases. Allergy, RC581-607

Abstract

Abstract Background Retroviral gene expression generally depends on a full-length transcript that initiates in the 5' LTR, which is either left unspliced or alternatively spliced. We and others have demonstrated the existence of antisense transcription initiating in the 3' LTR in human lymphotropic retroviruses, including HTLV-1, HTLV-2, and HIV-1. Such transcripts have been postulated to encode antisense proteins important for the establishment of viral infections. The antisense strand of the HIV-1 proviral DNA contains an ORF termed asp, coding for a highly hydrophobic protein. However, although anti-ASP antibodies have been described to be present in HIV-1-infected patients, its in vivo expression requires further support. The objective of this present study was to clearly demonstrate that ASP is effectively expressed in infected T cells and to provide a better characterization of its subcellular localization. Results We first investigated the subcellular localization of ASP by transfecting Jurkat T cells with vectors expressing ASP tagged with the Flag epitope to its N-terminus. Using immunofluorescence microscopy, we found that ASP localized to the plasma membrane in transfected Jurkat T cells, but with different staining patterns. In addition to an entire distribution to the plasma membrane, ASP showed an asymmetric localization and could also be detected in membrane connections between two cells. We then infected Jurkat T cells with NL4.3 virus coding for ASP tagged with the Flag epitope at its C-terminal end. By this approach, we were capable of showing that ASP is effectively expressed from the HIV-1 3' LTR in infected T cells, with an asymmetric localization of the viral protein at the plasma membrane. Conclusion These results demonstrate for the first time that ASP can be detected when expressed from full-length HIV-1 proviral DNA and that its localization is consistent with Jurkat T cells overexpressing ASP.

Published

2011

2. The HBZ-SP1 isoform of human T-cell leukemia virus type I represses JunB activity by sequestration into nuclear bodies

Author

Barbeau Benoit, Robert-Hebmann Véronique, Arpin-André Charlotte, Henaff Daniel, Raymond Frédéric, Basbous Jihane, Hivin Patrick, and Mesnard Jean-Michel

Subjects

Immunologic diseases. Allergy, RC581-607

Abstract

Abstract Background The human T-cell leukemia virus type I (HTLV-I) basic leucine-zipper factor (HBZ) has previously been shown to modulate transcriptional activity of Jun family members. The presence of a novel isoform of HBZ, termed HBZ-SP1, has recently been characterized in adult T-cell leukemia (ATL) cells and has been found to be associated with intense nuclear spots. In this study, we investigated the role of these nuclear bodies in the regulation of the transcriptional activity of JunB. Results Using fluorescence microscopy, we found that the HBZ-SP1 protein localizes to intense dots corresponding to HBZ-NBs and to nucleoli. We analyzed the relative mobility of the EGFP-HBZ-SP1 fusion protein using fluorescence recovery after photobleaching (FRAP) analysis and found that the deletion of the ZIP domain perturbs the association of the HBZ-SP1 protein to the HBZ-NBs. These data suggested that HBZ needs cellular partners, including bZIP factors, to form HBZ-NBs. Indeed, by cotransfection experiments in COS cells, we have found that the bZIP factor JunB is able to target delocalized form of HBZ (deleted in its nuclear localization subdomains) into the HBZ-NBs. We also show that the viral protein is able to entail a redistribution of JunB into the HBZ-NBs. Moreover, by transfecting HeLa cells (known to express high level of JunB) with a vector expressing HBZ-SP1, the sequestration of JunB to the HBZ-NBs inhibited its transcriptional activity. Lastly, we analyzed the nuclear distribution of HBZ-SP1 in the presence of JunD, a Jun family member known to be activated by HBZ. In this case, no NBs were detected and the HBZ-SP1 protein was diffusely distributed throughout the nucleoplasm. Conclusion Our results suggest that HBZ-mediated sequestration of JunB to the HBZ-NBs may be causing the repression of JunB activity in vivo.

Published

2007

3. HTLV-I antisense transcripts initiating in the 3'LTR are alternatively spliced and polyadenylated

Author

Marriott Susan J, Wattel Éric, Thête Julien, Paré Marie-Ève, Hivin Patrick, Arpin-André Charlotte, Audet Brigitte, Landry Sébastien, Cavanagh Marie-Hélène, Mesnard Jean-Michel, and Barbeau Benoit

Subjects

Immunologic diseases. Allergy, RC581-607

Abstract

Abstract Background Antisense transcription in retroviruses has been suggested for both HIV-1 and HTLV-I, although the existence and coding potential of these transcripts remain controversial. Thorough characterization is required to demonstrate the existence of these transcripts and gain insight into their role in retrovirus biology. Results This report provides the first complete characterization of an antisense retroviral transcript that encodes the previously described HTLV-I HBZ protein. In this study, we show that HBZ-encoding transcripts initiate in the 3' long terminal repeat (LTR) at several positions and consist of two alternatively spliced variants (SP1 and SP2). Expression of the most abundant HBZ spliced variant (SP1) could be detected in different HTLV-I-infected cell lines and importantly in cellular clones isolated from HTLV-I-infected patients. Polyadenylation of HBZ RNA occurred at a distance of 1450 nucleotides downstream of the HBZ stop codon in close proximity of a typical polyA signal. We have also determined that translation mostly initiates from the first exon located in the 3' LTR and that the HBZ isoform produced from the SP1 spliced variant demonstrated inhibition of Tax and c-Jun-dependent transcriptional activation. Conclusion These results conclusively demonstrate the existence of antisense transcription in retroviruses, which likely plays a role in HTLV-I-associated pathogenesis through HBZ protein synthesis.

Published

2006

4. Polarized expression of the membrane ASP protein derived from HIV-1 antisense transcription in T cells

Author

Clerc, Isabelle, primary, Laverdure, Sylvain, additional, Torresilla, Cynthia, additional, Landry, Sébastien, additional, Borel, Sophie, additional, Vargas, Amandine, additional, Arpin-André, Charlotte, additional, Gay, Bernard, additional, Briant, Laurence, additional, Gross, Antoine, additional, Barbeau, Benoît, additional, and Mesnard, Jean-Michel, additional

Published

2011

5. The HBZ-SP1 isoform of human T-cell leukemia virus type I represses JunB activity by sequestration into nuclear bodies

Author

Hivin, Patrick, primary, Basbous, Jihane, additional, Raymond, Frédéric, additional, Henaff, Daniel, additional, Arpin-André, Charlotte, additional, Robert-Hebmann, Véronique, additional, Barbeau, Benoit, additional, and Mesnard, Jean-Michel, additional

Published

2007

6. HTLV-I antisense transcripts initiating in the 3'LTR are alternatively spliced and polyadenylated

Author

Cavanagh, Marie-Hélène, primary, Landry, Sébastien, additional, Audet, Brigitte, additional, Arpin-André, Charlotte, additional, Hivin, Patrick, additional, Paré, Marie-Ève, additional, Thête, Julien, additional, Wattel, Éric, additional, Marriott, Susan J, additional, Mesnard, Jean-Michel, additional, and Barbeau, Benoit, additional

Published

2006