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Query: UNIPROT:P20226 (
TATA-binding protein
)
1,297
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
The
TATA-binding protein
(
TBP
) is a principal component of the general factor TFIID and is required for specific transcription by
RNA polymerase II
. We have shown that
TBP
is also a general factor for RNA polymerase III.
...
PMID:The TATA-binding protein is a general transcription factor for RNA polymerase III. 129 45
Initiation of transcription by
RNA polymerase II
requires a TFIID factor, which can recognize the TATA element common to many promoters. Two distinct multisubunit TFIID factors can be resolved from extracts of mammalian cells, and both of them contain the well-characterized
TATA-binding protein
(
TBP
) and are capable of supporting
RNA polymerase II
transcription in an in vitro reaction system. The smaller complex, B-TFIID, was purified and its subunit composition was determined. B-TFIID consists of two subunits: the
TBP
and a TBP-associated factor (TAF) of 170 kDa. This TAF is specific for B-TFIID and appears not to be present in the D-TFIID complex. Furthermore, it was found that the highly purified B-TFIID fractions have (d)ATPase activity.
...
PMID:Composition of transcription factor B-TFIID. 138 11
A critical regulatory element in many promoters transcribed by
RNA polymerase II
is the "TATA" box, which is located 25-30 nucleotides upstream of the transcription initiation site. TFIID is a biochemically defined HeLa cell nuclear fraction containing a transcription factor activity that binds specifically to the TATA box and is critical in determining both basal and regulated promoter activity. Recently, the gene for a
TATA-binding protein
was cloned and found to bind to various TATA elements and to substitute for TFIID in stimulating basal gene expression in in vitro transcription systems. However, it is possible that additional cellular factors can bind to the TATA element and influence the level of gene expression. By using lambda gt11 expression cloning with oligonucleotides corresponding to the human immunodeficiency virus 1 TATA element, we report the identification of a cellular protein with a calculated molecular mass of 123 kDa that we designate TATA element modulatory factor (TMF). TMF binds to the human immunodeficiency virus 1 TATA element in gel-retardation assays and inhibits activation of the viral long terminal repeat by the
TATA-binding protein
in in vitro transcription assays. TMF contains leucine-zipper amino acid motifs and exhibits homology in its DNA binding domain with the phage-encoded DNA binding protein Ner. Chromosomal mapping localizes the TMF gene to human chromosome 3p12-p21, which is a site of frequent rearrangements in lung and renal carcinomas. Thus, TMF is a transcription factor that likely regulates the expression of both viral and cellular genes.
...
PMID:Cloning and chromosomal mapping of a human immunodeficiency virus 1 "TATA" element modulatory factor. 140 43
The TDS4 gene of S. cerevisiae was isolated as an allele-specific high copy suppressor of mutations within the basic region of the
TATA-binding protein
(
TBP
). The gene is essential for viability and encodes a 596 aa protein. The first 300 aa of the TDS4 protein exhibit significant sequence similarity to the
RNA polymerase II
transcription factor TFIIB. However, TDS4 is required for RNA polymerase III transcription in vivo and in vitro. Antibodies specific for TDS4 or
TBP
react with the TFIIIB complex, indicating that both proteins are components of the RNA polymerase III initiation complex. These findings suggest that the
RNA polymerase II
and III initiation mechanisms are extremely similar, and they explain how the
TATA-binding protein
can function in both systems.
...
PMID:A suppressor of TBP mutations encodes an RNA polymerase III transcription factor with homology to TFIIB. 142 90
We have previously shown that the
TATA-binding protein
(
TBP
) and multiple
TBP
-associated factors (TAFs) are required for regulated transcriptional initiation by
RNA polymerase II
. Here we report the biochemical properties of the RNA polymerase I promoter selectivity factor, SL1, and its relationship to
TBP
. Column chromatography and glycerol gradient sedimentation indicate that a subpopulation of
TBP
copurifies with SL1 activity. Antibodies directed against
TBP
efficiently deplete SL1 transcriptional activity, which can be restored with the SL1 fraction but not purified
TBP
. Thus,
TBP
is necessary but not sufficient to complement SL1 activity. Analysis of purified SL1 reveals a complex containing
TBP
and three distinct TAFs. Purified TAFs reconstituted with recombinant
TBP
complement SL1 activity, and this demonstrates that
TBP
plus novel associated factors are integral components of SL1. These findings suggest that
TBP
may be a universal transcription factor and that the
TBP
-TAF arrangement provides a unifying mechanism for promoter recognition in animal cells.
...
PMID:The TATA-binding protein and associated factors are integral components of the RNA polymerase I transcription factor, SL1. 154 96
Using temperature- and proteolytically sensitive derivatives to inactivate the function of the yeast
TATA-binding protein
(
TBP
) in vivo, we investigated the requirement of
TBP
for transcription by the three nuclear RNA polymerases in yeast cells.
TBP
is required for
RNA polymerase II
(pol II) transcription from promoters containing conventional TATA elements as well as functionally distinct promoters that lack TATA-like sequences.
TBP
is also required for transcription of the U6 snRNA and two different tRNA genes mediated by RNA pol III as well as transcription of ribosomal RNA mediated by RNA pol I. For all promoters tested, transcription decreases rapidly and specifically upon inactivation of
TBP
, strongly suggesting that
TBP
is directly involved in the transcription process. These observations suggest that
TBP
is required for transcription of all nuclearly encoded genes in yeast, although distinct molecular mechanisms are probably involved for the three RNA polymerase transcription machineries.
...
PMID:The TATA-binding protein is required for transcription by all three nuclear RNA polymerases in yeast cells. 158 47
The adenovirus type 2 IVa2 promoter lacks a conventional TATA element yet directs transcription from two closely spaced initiation sites. To define elements required for in vitro transcription of this promoter, IVa2 templates carrying 5' deletions or linker-scanning mutations were transcribed in HeLa whole-cell extracts and the transcripts were analyzed by primer extension. Mutation of the sequence centered on position -47, which is specifically recognized by a cellular factor, reduced the efficiency of IVa2 transcription two- to threefold, whereas mutation of the sequence centered on position -30 selectively impaired utilization of the minor in vivo initiation site. Utilization of the major in vivo site was decreased no more than fivefold by deletion of all sequences upstream of position -15. By contrast, mutation of the region from +13 to +19 or of the initiation region severely impaired IVa2 transcription. The sequence spanning the initiation sites was sufficient to direct accurate initiation by
RNA polymerase II
from the major in vivo site. Thus, the two initiation sites of the IVa2 promoter are specified by independent elements, and a downstream element is the primary determinant of efficient transcription from both of these sites. The downstream element identified by mutational analysis altered the TATA element-like sequence TATAGAAA lying at positions +21 to +14 in the coding strand. Transcription from the wild-type IVa2 promoter was severely inhibited when endogenous TFIID was inactivated by mild heat treatment. Exogenous human
TATA-binding protein
(
TBP
) synthesized in Escherichia coli restored specific IVa2 transcription from both initiation sites when added to such heat-treated extracts. Although efficient IVa2 transcription requires both the downstream TATA sequence and active TFIID, bacterially synthesized
TBP
also stimulated the low level of IVa2 transcription observed when the TATA sequence was mutated to a sequence that failed to bind
TBP
.
...
PMID:Anatomy of an unusual RNA polymerase II promoter containing a downstream TATA element. 158 75
Fractionation of a transcription-competent HeLa cell extract on a column containing one copy of the heptamer repeat (YSPTSPS) present in the carboxy-terminal domain (CTD) of the largest subunit of
RNA polymerase II
resulted in the loss of transcriptional activity. Fractionation of the extracts on columns containing mutations of the heptamer repeat was without effect. Such transcriptionally inactive extracts regained their ability to specifically transcribe different class II promoters upon the addition of human TFIID, recombinant yeast
TATA-binding protein
(
TBP
), or proteins bound to the column. Fractionation of
RNA polymerase II
on columns containing human or yeast
TBP
resulted in the specific retention of the nonphosphorylated form of
RNA polymerase II
. The phosphorylated form of the enzyme was unable to interact with
TBP
. The specific interaction of
RNA polymerase II
with
TBP
was mediated by the CTD of
RNA polymerase II
.
...
PMID:Specific interaction between the nonphosphorylated form of RNA polymerase II and the TATA-binding protein. 159 81
The
RNA polymerase II
large subunit carboxy-terminal domain (CTD) plays a role in transcription initiation, but its mechanism of action is not well understood. We have investigated the function of the SRB2 gene, which was isolated as a dominant suppressor of CTD truncation mutations. The allele specificity of this suppressor indicates that SRB2 and the CTD are involved in the same function. Indeed, cells lacking SRB2 and cells lacking a large portion of the CTD exhibit the same set of conditional growth phenotypes and exhibit very similar defects in gene expression in vivo. The SRB2 protein is a novel transcription factor that has an important role in basal and activated transcription in vitro and is essential for efficient establishment of the transcription initiation apparatus. Template commitment experiments suggest that SRB2 becomes physically associated with the transcription initiation complex. We find that SRB2 binds specifically to TFIID. As SRB2 and the
RNA polymerase II
CTD are involved in the same function, these results reveal a functional link between the CTD and the
TATA-binding factor
. This study implicates the CTD in recruitment of
RNA polymerase II
to the transcription initiation complex.
...
PMID:A novel transcription factor reveals a functional link between the RNA polymerase II CTD and TFIID. 159 82
Transcription of mammalian genes by
RNA polymerase II
often begins at a specific nucleotide, whose location is determined either by an upstream DNA element known as a TATA box or by an element positioned at the transcription start site called an initiator (Inr). By in vitro analysis of synthetic promoters, we demonstrate here that the TATA and Inr elements are functionally similar and that the Inr is contained between nucleotides -3 and +5 relative to the initiation site. Moreover, we found that a mammalian transcription factor IID (TFIID) protein fraction is required for transcriptional stimulation by an Sp1-dependent activating element placed upstream of either TATA or Inr elements. However, in these assays, the yeast
TATA-binding protein
, which previously was shown to function similarly to mammalian TFIID, could not efficiently substitute for the mammalian TFIID fraction. These results demonstrate that mammalian TFIID is functionally distinct from the yeast
TATA-binding protein
and may contain additional subunits or domains that are important for transcriptional activation from some promoters.
...
PMID:Transcriptional activation by Sp1 as directed through TATA or initiator: specific requirement for mammalian transcription factor IID. 214 Nov 69
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