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Modifications in host cell cytoskeleton structure and function mediated by intracellular HIV-1 Tat protein are greatly dependent on the second coding exon

Author: A. Dopazo
Albini
Alcami
Amieva
Anand
Aprea
Arenzana-Seisdedos
Bachelerie
Barillari
Bartz
Battaglia
Baumli
Berkhout
Biswas
Borgatti
Bradford
Campioni
Carroll
Chang
Chen
Choe
Churcher
D. Abia
Damsky
Dandekar
de la Fuente
de Mareuil
Demarchi
E. Mateos
Egele
Ensoli
Epie
Fais
Fais
Foy
Garcia
Gautier
Gaynor
Gibellini
Gumienny
Harrich
Hauber
Hidalgo-Estevez
Huigen
Izmailova
J. Alcami
Janardhan
Jeang
Jeang
Jones
Kashiwa
Kim
Klein-Hitpass
Klipper-Aurbach
Kurayoshi
La n de Lera
Lee
Li
Liu
Liu
Liu
M. Coiras
M. R. Lopez-Huertas
Ma
Macian
Magnuson
Marcello
McCloskey
Meyaard
Misumi
Mitola
Northrop
Ortiz
Ott
Ott
Pickl
Pincus
P lopon se
Rhim
S. Callejas
Sabatier
Sali
Sasaki
Schuler
Schwarze
Subramanyam
Verhoef
Viscidi
Vives
Westendorp
Westendorp
Willard-Gallo
Wu
Xiao
Xiao
Yoshida
Zauli
Zhou
Zhu
Publication venue: Oxford University Press
Publication date: 01/01/2010
Field of study

Supplementary Data are available at NAR OnlineThe human immunodeficiency virus type 1 (HIV-1) regulator Tat is essential for viral replication because it achieves complete elongation of viral transcripts. Tat can be released to the extracellular space and taken up by adjacent cells, exerting profound cytoskeleton rearrangements that lead to apoptosis. In contrast, intracellular Tat has been described as protector from apoptosis. Tat gene is composed by two coding exons that yield a protein of 101 amino acids (aa). First exon (1–72aa) is sufficient for viral transcript elongation and second exon (73–101 aa) appears to contribute to non-transcriptional functions. We observed that Jurkat cells stably expressing intracellular Tat101 showed gene expression deregulation 4-fold higher than cells expressing Tat72. Functional experiments were performed to evaluate the effect of this deregulation. First, NF-iB-, NF-AT- and Sp1-dependent transcriptional activities were greatly enhanced in Jurkat-Tat101, whereas Tat72 induced milder but efficient activation. Second, cytoskeleton-related functions as cell morphology, proliferation, chemotaxis, polarization and actin polymerization were deeply altered in Jurkat- Tat101, but not in Jurkat-Tat72. Finally, expression of several cell surface receptors was dramatically impaired by intracellular Tat101 but not by Tat72. Consequently, these modifications were greatly dependent on Tat second exon and they could be related to the anergy observed in HIV-1-infected T cells.Plan Nacional del SIDA (MVI 1434/05–5), FIPSE 36584/ 06 and 36633/07, VIRHORST Network from Comunidad de Madrid (Spain), FIS PI040614 and PI0808752, ISCIII-RETIC RD06/0006, EUROPRISE Network of Excellence of the EU (Grant no. LSHP CT-2006- 037611), and BIO2008-04384 from the Ministerio de Ciencia e Innovacio´ n, Espan˜ a. Funding for open access charge: Instituto de Salud Carlos III, Ministry of Science and Technology, Spain.Peer reviewe

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