Affiliation:
1. Department of Biological Sciences, Stanford University, Stanford, California 94305-5020
Abstract
ABSTRACT
Expression of the tryptophanase (
tna
) operon of
Escherichia coli
is regulated by catabolite repression and by tryptophan-induced transcription antitermination. Tryptophan induction prevents Rho-dependent transcription termination in the leader region of the operon. Induction requires translation of a 24-residue leader peptide-coding region,
tnaC
, containing a single, crucial Trp codon. Studies with a
lacZ
reporter construct lacking the
tnaC-tnaA
spacer region suggest that, in the presence of excess tryptophan, the TnaC leader peptide acts in
cis
on the ribosome translating
tnaC
to inhibit its release. The stalled ribosome is thought to block Rho's access to the transcript. In this paper we examine the roles of the
boxA
sequence and the
rut
site in Rho-dependent termination. Deleting six nucleotides (CGC CCT) of
boxA
or introducing specific point mutations in
boxA
results in high-level constitutive expression. Some constitutive changes introduced in
boxA
do not change the TnaC peptide sequence. We confirm that deletion of the
rut
site results in constitutive expression. We also demonstrate that, in each constitutive construct, replacement of the
tnaC
start codon by a UAG stop codon reduces expression significantly, suggesting that constitutive expression requires translation of the
tnaC
coding sequence. Addition of bicyclomycin, an inhibitor of Rho, to these UAG constructs increases expression, demonstrating that reduced expression is due to Rho action. Combining a
boxA
point mutation with
rut
site deletion results in constitutive expression comparable to that of a maximally induced operon. These results support the hypothesis that in the presence of tryptophan the ribosome translating
tnaC
blocks Rho's access to the
boxA
and
rut
sites, thereby preventing transcription termination.
Publisher
American Society for Microbiology
Subject
Molecular Biology,Microbiology
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4. Catabolite Repression of Tryptophanase in
Escherichia coli
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