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Molecular and Cellular Biology, October 1999, p. 6803-6814, Vol. 19, No. 10
0270-7306/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.
Cytomegalovirus IE2 Protein Stimulates Interleukin
1
Gene Transcription via Tethering to Spi-1/PU.1
Nawarat
Wara-aswapati,1,2,
Zhiyong
Yang,1,3
Wayne R.
Waterman,1
Yoshinobu
Koyama,1,3
Sotirios
Tetradis,1,
Bob K.
Choy,1,3
Andrew C.
Webb,4 and
Philip E.
Auron1,3,*
The New England Baptist Bone & Joint Institute, Beth Israel
Deaconess Medical Center,1 Department of
Periodontology, Harvard School of Dental
Medicine,2 and Department of Medicine,
Harvard Medical School,3 Boston,
Massachusetts 02115, and Department of Biological Sciences,
Wellesley College, Wellesley, Massachusetts 021814
Received 23 March 1999/Returned for modification 17 May
1999/Accepted 28 July 1999
Potent induction of the gene coding for human prointerleukin 1
(il1b) normally requires a far-upstream inducible enhancer in addition to a minimal promoter located between positions
131 and
+12. The transcription factor Spi-1 (also called PU.1) is necessary for
expression and binds to the minimal promoter, thus providing an
essential transcription activation domain (TAD). In contrast, infection
by human cytomegalovirus (HCMV) can strongly activate il1b
via the expression of immediate early (IE) viral proteins and
eliminates the requirement for the upstream enhancer. Spi-1 has been
circumstantially implicated as a host factor in this process. We report
here the molecular basis for the direct involvement of Spi-1 in HCMV
activation of il1b. Transfection of Spi-1-deficient HeLa
cells demonstrated both the requirement of Spi-1 for IE activity and
the need for a shorter promoter (
59 to +12) than that required in the
absence of IE proteins. Furthermore, in contrast to normal,
enhancer-dependent il1b expression, which absolutely
requires both the Spi-1 winged helix-turn-helix (wHTH) DNA-binding
domain and the majority of the Spi-1 TAD, il1b expression in the presence of IE proteins does not require the Spi-1 TAD, which
plays a synergistic role. In addition, we demonstrate that a single IE
protein, IE2, is critical for the induction of il1b. Protein-protein interaction experiments revealed that the wing motif
within the Spi-1 wHTH domain directly recruits IE2. In turn, IE2
physically associates with the Spi-1 wing and requires the integrity of
at least one region of IE2. Functional analysis demonstrates that both
this region and a carboxy-terminal acidic TAD are required for IE2
function. Therefore, we propose a protein-tethered transactivation mechanism in which the il1b promoter-bound Spi-1 wHTH
tethers IE2, which provides a TAD, resulting in the transactivation of il1b.
*
Corresponding author. Mailing address: Harvard
Institutes of Medicine, Room 245, 77 Avenue Louis Pasteur, Boston, MA
02115-5727. Phone: (617) 667-0741. Fax: (617) 975-5299. E-mail:
pauron{at}caregroup.med.harvard.edu.
Present address: Khon Kaen University, Faculty of Dentistry, Khon
Kaen 40002, Thailand.

Present address: UCLA School of Dentistry, Los Angeles, CA
90095.
Molecular and Cellular Biology, October 1999, p. 6803-6814, Vol. 19, No. 10
0270-7306/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.
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