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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
) plays a key role in transcription initiation. Several negative cofactors (NC1,
NC2
, and Dr1) are known to interact with
TBP
in a manner that prevents productive interactions of transcription factors TFIIA and TFIIB with promoter-bound
TBP
. To gain insights into the regulatory interplay on the surface of
TBP
, we have employed mutant forms of
TBP
to identify amino acid residues important for interactions with the negative regulatory cofactor
NC2
and the general factor TFIIB. The results show the involvement of distinct domains of
TBP
in these interactions. Residues (Lys-133, Lys-145, and Lys-151) in the basic repeat region are important for interactions with
NC2
, as well as with TFIIA (Buratowski, S., and Zhou, H. (1992) Science 255, 1130-1132; Lee, D. K., DeJong, J., Hashimoto, S., Horikoshi, M., and Roeder, R. G. (1992) Mol. Cell. Biol. 12, 5189-5196), whereas a residue (Leu-189) in the second stirrup-like loop spanning S2' and S3' is required for interaction with TFIIB. In addition, we demonstrate that
NC2
is identical to the previously cloned negative cofactor Dr1. The implications of these results for
TBP
structure and function are discussed.
...
PMID:TATA-binding protein residues implicated in a functional interplay between negative cofactor NC2 (Dr1) and general factors TFIIA and TFIIB. 773 39
The human general co-factors were discovered during biochemical fractionation of mammalian nuclear extracts in functional in vitro assays. They appear to act in concert with other co-activators that bind tightly to the
TATA-binding protein
and RNA polymerase II. Several co-factors have been shown to interact with general transcription factors, leading either to activation or repression of transcription. At least one subgroup of co-factors that enhance the effects of activators on transcription are DNA-binding proteins located in the chromatin. In fact, one co-factor, the repressor
NC2
, is structurally related to histones. The understanding of the molecular interplay of such components of the initiation complex in the chromatin-including general co-factors, other co-factors, general factors and activators-will be a major challenge in the future.
...
PMID:The human general co-factors. 887 Apr 94
Using a genetic screen, we isolated three
TATA-binding protein
(
TBP
) mutants that increase transcription from promoters that are repressed by the Cyc8-Tup1 or Sin3-Rpd3 corepressors or that lack an enhancer element, but not from an equivalently weak promoter with a mutated TATA element. Increased transcription is observed when the
TBP
mutants are expressed at low levels in the presence of wild-type
TBP
. These
TBP
mutants are unable to support cell viability, and they are toxic in strains lacking Rpd3 histone deacetylase or when expressed at higher levels. Although these mutants do not detectably bind TATA elements in vitro, genetic and chromatin immunoprecipitation experiments indicate that they act directly at promoters and do not increase transcription by titration of a negative regulatory factor(s). The
TBP
mutants are mildly defective for associating with promoters responding to moderate or strong activators; in addition, they are severely defective for RNA polymerase (Pol) III but not Pol I transcription. These results suggest that, with respect to Pol II transcription, the
TBP
mutants specifically increase expression from core promoters. Biochemical analysis indicates that the
TBP
mutants are unaffected for TFIID complex formation, dimerization, and interactions with either the general negative regulator
NC2
or the N-terminal inhibitory domain of TAF130. We speculate that these
TBP
mutants have an unusual structure that allows them to preferentially access TATA elements in chromatin templates. These
TBP
mutants define a criterion by which promoters repressed by Cyc8-Tup1 or Sin3-Rpd3 resemble enhancerless, but not TATA-defective, promoters; hence, they support the idea that these corepressors inhibit the function of activator proteins rather than the Pol II machinery.
...
PMID:TATA-binding protein mutants that increase transcription from enhancerless and repressed promoters in vivo. 1066 25
The assembly of transcription complexes at eukaryotic promoters involves a number of distinct steps including chromatin remodeling, and recruitment of a
TATA-binding protein
(
TBP
)-containing complexes, the RNA polymerase II holoenzyme. Each of these stages is controlled by both positive and negative factors. In this review, mechanisms that regulate the interactions of
TBP
with promoter DNA are described. The first is autorepression, where
TBP
sequesters its DNA-binding surface through dimerization. Once
TBP
is bound to DNA, factors such as TAF(II)250 and Mot1 induce
TBP
to dissociate, while other factors such as
NC2
and the NOT complex convert the
TBP
/DNA complex into an inactive state. TFIIA antagonizes these
TBP
repressors but may be effective only in conjunction with the recruitment of the RNA polymerase II holoenzyme by promoter-bound activators. Taken together, the ability to induce a gene may depend minimally upon the ability to remodel chromatin as well as alleviate direct repression of
TBP
and other components of the general transcription machinery. The magnitude by which an activated gene is expressed, and thus repeatedly transcribed, might depend in part on competition between
TBP
inhibitors and the holoenzyme for access to the
TBP
/TATA complex.
...
PMID:Control of gene expression through regulation of the TATA-binding protein. 1097 59
Histones are among the most conserved proteins in evolution, sharing a histone fold motif. A number of additional histonic proteins exist and are involved in the process of transcriptional regulation. We describe here the identification, cloning and characterization of two small members of the H2A-H2B sub-family (YBL1 and YCL1) related to the NF-YB and NF-YC subunits of the CCAAT-binding activator NF-Y and to the
TATA-binding protein
(
TBP
) binding repressor
NC2
. Unlike the latters, YBL1 and YCL1 have no intrinsic CCAAT or TATA-binding capacity. In nucleosome reconstitution assays, they can form complexes with histones in solution and on DNA and they are part of relatively large complexes, as determined by glycerol gradient experiments. Our data support the idea that YBL1 and YCL1 are divergent with respect to NF-YB and NF-YC for specific functions, but have coevolved the capacity to interact with nucleosomal structures.
...
PMID:Cloning and characterization of the histone-fold proteins YBL1 and YCL1. 1100 Feb 77
NC2
(Dr1-Drap1 or Bur6-Ydr1) has been characterized in vitro as a general negative regulator of RNA polymerase II (Pol II) transcription that interacts with
TATA-binding protein
(
TBP
) and inhibits its function. Here, we show that
NC2
associates with promoters in vivo in a manner that correlates with transcriptional activity and with occupancy by basal transcription factors.
NC2
rapidly associates with promoters in response to transcriptional activation, and it remains associated under conditions in which transcription is blocked after assembly of the Pol II preinitiation complex.
NC2
positively and negatively affects approximately 17% of Saccharomyces cerevisiae genes in a pattern that resembles the response to general environmental stress. Relative to
TBP
,
NC2
occupancy is high at promoters where
NC2
is positively required for normal levels of transcription. Thus,
NC2
is associated with the Pol II preinitiation complex, and it can play a direct and positive role at certain promoters in vivo.
...
PMID:Yeast NC2 associates with the RNA polymerase II preinitiation complex and selectively affects transcription in vivo. 1128 53
Mot1 is an essential yeast Snf2/Swi2-related ATPase that exerts both positive and negative effects on gene expression. In vitro, Mot1 can disrupt
TATA-binding protein
-DNA complexes in an ATP-dependent reaction. This activity can explain Mot1-mediated transcriptional repression, but how Mot1 activates transcription is unknown. We demonstrate that, remarkably, Mot1 is localized in vivo to promoters for both Mot1-repressed and Mot1-activated genes. Moreover, Mot1 ATPase activity is required for both activation and repression of gene activity. These findings suggest a novel function for the Mot1 ATPase at activated genes, perhaps involving ATP-driven reorganization of the preinitiation complex. Mot1 regulates the expression of approximately 3% of yeast genes in cells grown in rich medium. Most of these genes are repressed by Mot1, consistent with Mot1's ATP-dependent
TATA-binding protein
-DNA dissociating activity. Additionally, approximately 77% of the Mot1-repressed genes are involved in the diauxic shift, stress response, mating, or sporulation. The gene sets controlled by
NC2
and Srb10 are strongly correlated with the Mot1-controlled set, suggesting that these factors cooperate in transcriptional control on a global scale.
...
PMID:Mot1 activates and represses transcription by direct, ATPase-dependent mechanisms. 1188 Jun 21
Mot1 stably associates with the
TATA-binding protein
(
TBP
), and it can dissociate
TBP
from DNA in an ATP-dependent manner. Mot1 acts as a negative regulator of
TBP
function in vitro, but genome-wide transcriptional profiling suggests that Mot1 positively affects about 10% of yeast genes and negatively affects about 5%. Unexpectedly, Mot1 associates with active RNA polymerase (Pol) II and III promoters, and it is rapidly recruited in response to activator proteins. At Pol II promoters, Mot1 association requires
TBP
and is strongly correlated with the level of
TBP
occupancy. However, the Mot1/
TBP
occupancy ratio at both Mot1-stimulated and Mot1-inhibited promoters is high relative to that at typical promoters, strongly suggesting that Mot1 directly affects transcriptional activity in a positive or negative manner, depending on the gene. The effect of Mot1 at the HIS3 promoter region depends on the functional quality and DNA sequence of the TATA element. Unlike
TBP
, Mot1 association is largely independent of the Srb4 component of Pol II holoenzyme, and it also can occur downstream of the promoter region. Mot1 removes
TBP
, but not
TBP
complexes or preinitiation complexes, from inappropriate genomic locations. Mot1 inhibits the association of
NC2
with promoters, suggesting that the
TBP
-Mot1 and
TBP
-
NC2
complexes compete for promoter occupancy in vivo. We speculate that Mot1 does not form transcriptionally active
TBP
complexes but rather regulates transcription in vivo by modulating the activity of free
TBP
and/or by affecting promoter DNA structure.
...
PMID:Mot1 associates with transcriptionally active promoters and inhibits association of NC2 in Saccharomyces cerevisiae. 1241 16
Mot1 is an essential Snf2/Swi2-related Saccharomyces cerevisiae protein that binds the
TATA-binding protein
(
TBP
) and removes
TBP
from DNA using ATP hydrolysis. Mot1 functions in vivo both as a repressor and as an activator of transcription. Mot1 catalysis of
TBP
.DNA disruption is consistent with its function as a repressor, but the Mot1 mechanism of activation is unknown. To better understand the physiologic role of Mot1 and its enzymatic mechanism, MOT1 mutants were generated and tested for activity in vitro and in vivo. The results demonstrate a close correlation between the
TBP
.DNA disruption activity of Mot1 and its essential in vivo function. Previous results demonstrated a large overlap in the gene sets controlled by Mot1 and
NC2
. Mot1 and
NC2
can co-occupy
TBP
.DNA in vitro, and
NC2
binding does not impair Mot1-catalyzed disruption of the complex. Residues on the DNA-binding surface of
TBP
are important for Mot1 binding and the Mot1.
TBP
binary complex binds very poorly to DNA and does not dissociate in the presence of ATP. However, the binary complex binds DNA well in the presence of the transition state analog ADP-AlF(4). A model for Mot1 action is proposed in which ATP hydrolysis causes the Mot1 N terminus to displace the TATA box, leading to ejection of Mot1 and
TBP
from DNA.
...
PMID:Mot1 regulates the DNA binding activity of free TATA-binding protein in an ATP-dependent manner. 1257 Dec 41
Transcriptional activity of the
TATA-binding protein
(
TBP
) is controlled by a variety of proteins. The BTAF1 protein (formerly known as TAF(II)170/TAF-172 and the human ortholog of Saccharomyces cerevisiae Mot1p) and the
NC2
complex composed of NC2alpha (DRAP1) and NC2beta (Dr1) are able to bind to
TBP
directly and regulate RNA polymerase II transcription both positively and negatively. Here, we present evidence that the NC2alpha subunit interacts with BTAF1. In contrast, the NC2beta subunit is not able to associate with BTAF1 and seems to interfere with the BTAF1-
TBP
interaction. Addition of NC2alpha or the
NC2
complex can stimulate the ability of BTAF1 to interact with
TBP
. This function is dependent on the presence of ATP in cell extracts but does not involve the ATPase activity of BTAF1 nor phosphorylation of NC2alpha. Together, our results constitute the first evidence of the physical cooperation between BTAF1 and NC2alpha in
TBP
regulation and provide a framework to understand transcription functions of NC2alpha and NC2beta in vivo.
...
PMID:NC2alpha interacts with BTAF1 and stimulates its ATP-dependent association with TATA-binding protein. 1550 7
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