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Mol Cell Biol, March 1998, p. 1692-1700, Vol. 18, No. 3
0270-7306/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
Polymerase (Pol) III TATA Box-Binding Protein
(TBP)-Associated Factor Brf Binds to a Surface on TBP Also Required for
Activated Pol II Transcription
Yuhong
Shen,1
George A.
Kassavetis,2
Gene O.
Bryant,1 and
Arnold J.
Berk1,*
Molecular Biology Institute and Department of
Microbiology and Molecular Genetics, University of California, Los
Angeles, California 90095-1570,1 and
Department of Biology and Center for Molecular
Genetics, University of California, San Diego, La Jolla, California
92093-06342
Received 23 September 1997/Returned for modification 17 November
1997/Accepted 16 December 1997
The TATA box-binding protein (TBP) plays an essential role in
transcription by all three eukaryotic nuclear RNA polymerases, polymerases (Pol) I, II, and III. In each case, TBP interacts with
class-specific TBP-associated factors (TAFs) to form class-specific transcription initiation factors. For yeast Pol III transcription, TBP
associates with Brf (from TFIIB-related factor) and B", two Pol III
TAFs, to form Pol III transcription factor TFIIIB. Here, we identify
TBP surface residues that are required for interaction with yeast Pol
III TAFs. Ninety-one human TBP surface residue mutants with radical
substitutions were analyzed for the ability to form stable gel shift
complexes with purified Brf and B" and for their activities for in
vitro synthesis of yeast U6 snRNA. Mutations in a large positively
charged epitope extending from the top (that is, on the surface
opposite the DNA-facing "saddle" of TBP) and onto the side of the
first TBP repeat inhibited binding to Brf (residues K181, L185, R186,
E206, R231, L232, R235, K236, R239, Q242, K243, K249, and F250). A
triple-mutant TBP (R231E + R235E + R239S) had greatly reduced
activity for yeast U6 snRNA gene transcription while remaining active
for Pol II basal transcription. Similar results were observed when
selected mutations were introduced into yeast TBP at equivalent
positions. A C-terminal fragment of Brf lacking the region of homology
with TFIIB retains the ability to bind TBP-DNA complexes (G. Kassavetis, C. Bardeleben, A. Kumar, E. Ramirez, and E. P. Geiduschek, Mol. Cell. Biol. 17:5299-5306, 1997); the same TBP
mutations reduced binding by this fragment. Mutations in TBP residues
that interact with TFIIB did not affect Brf binding or U6 gene
transcription. These results indicate that Brf and TFIIB interact
differently with TBP. An extensively overlapping epitope on the top
surface of TBP was found previously to be required for activated Pol II
transcription and has been hypothesized to interact with Pol II TAFs.
Our results map the surface of TBP that interacts with Brf and suggest
that Pol II and Pol III TAFs interact with the same surface of TBP.
*
Corresponding author. Mailing address: Molecular
Biology Institute, 405 Hilgard Ave., University of California, Los
Angeles, CA 90095-1570. Phone: (310) 206-6298. Fax: (310) 206-7286. E-mail: berk{at}mbi.ucla.edu.
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