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Drug
Enzyme
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Gene/Protein
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Target Concepts:
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Query: EC:3.4.24.17 (
MMP-3
)
3,419
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
TEL
is a member of the ETS family of transcription factors that interacts with the mSin3 and SMRT corepressors to regulate transcription.
TEL
is biallelically disrupted in acute leukemia, and loss of heterozygosity at the
TEL
locus has been observed in various cancers. Here we show that expression of
TEL
in Ras-transformed NIH 3T3 cells inhibits cell growth in soft agar and in normal cultures. Unexpectedly, cells expressing both Ras and
TEL
grew as aggregates. To begin to explain the morphology of Ras-plus
TEL
-expressing cells, we demonstrated that the endogenous matrix metalloproteinase
stromelysin
-1 was repressed by
TEL
.
TEL
bound sequences in the
stromelysin
-1 promoter and repressed the promoter in transient-expression assays, suggesting that it is a direct target for
TEL
-mediated regulation. Mutants of
TEL
that removed a binding site for the mSin3A corepressor but retained the ETS domain failed to repress
stromelysin
-1. When BB-94, a matrix metalloproteinase inhibitor, was added to the culture medium of Ras-expressing cells, it caused a cell aggregation phenotype similar to that caused by
TEL
expression. In addition,
TEL
inhibited the invasiveness of Ras-transformed cells in vitro and in vivo. Our results suggest that
TEL
acts as a tumor suppressor, in part, by transcriptional repression of
stromelysin
-1.
...
PMID:TEL, a putative tumor suppressor, modulates cell growth and cell morphology of ras-transformed cells while repressing the transcription of stromelysin-1. 1091 66
TEL
(Translocation-ETS-Leukemia or ETV 6) is disrupted by multiple chromosomal translocations in acute leukemia. The loss of heterozygosity at the
TEL
locus in leukemias and the hemizygous deletion of
TEL
that is observed in various tumors, suggests that
TEL
is a tumor suppressor. Overexpression of
TEL
alters cellular morphology and represses the expression of the matrix metalloproteinase
stromelysin
-1. Based on these studies, deletion analysis was used to define the minimal repression domains of
TEL
.
TEL
-mediated repression required both the N-terminal pointed domain and a central region composed of amino acids 268-303. The mSin3A and N-CoR corepressors bind to the pointed domain and the central repression domain of
TEL
, respectively. Unexpectedly, histone deacetylase-3, but not other histone deacetylases, also associates with the central region of
TEL
. Histone deacetylase-3 interacts with a
TEL
mutant that cannot bind N-CoR, suggesting that this is a direct interaction with
TEL
. In addition, histone H3 was under-acetylated near the
TEL
-binding sites in the endogenous
stromelysin
-1 promoter when
TEL
was expressed. Furthermore, trichostatin A, a potent histone deacetylase inhibitor, impaired
TEL
-dependent repression of the
stromelysin
-1 promoter. Finally, while
TEL
-expression induced cellular aggregation of Ras-transformed cells, Trichostatin A reversed the
TEL
-induced cellular aggregation phenotype. Thus, the cumulative data suggests that histone deacetylase-3 activity is required for the transcriptional functions of
TEL
.
...
PMID:TEL contacts multiple co-repressors and specifically associates with histone deacetylase-3. 1143 34
