Awardee OrganizationSCRIPPS RESEARCH INSTITUTE, THE
Description
Abstract Text
A number of genes including those for the major degradative
enzymes of Bacillus subtilis appear to be controlled by several
regulatory genes which may comprise a global regulatory system.
The regulatory genes, sacU, sacQ, prtR, and hpr pleiotropically
affect the synthesis of several enzymes including levansucrase,
sacB, and alkaline protease, aprE. The target of these regulatory
genes on either sacB or aprE is at least 100 basepairs upstream of
the promoter for the genes and they stimulate transcription from
the normal start site. Studies are proposed to isolate the only
remaining uncloned regulatory gene, sacU and characterize
mutations in the gene. The molecular basis for the phenotypes of
mutations in each gene will be probed. Other genes in which
mutation leads to an alteration of this regulatory network will be
isolated and characterized. The site of action of the regulatory
genes will be determined for the aprE (subtilisin) promoter.
Extensive deletion analyses from both directions will be used to
define the target sites. Site-directed and cassette mutagenesis
experiments will further implicate important bases. Messenger
RNA will be isolated from mutant strains and transcription start
sites found by primer extension to determine if all the regulatory
mutations stimulate transcription from the normal start site.
Northern analysis will ascertain if messenger RNA levels in all
mutants are elevated. Large quantities of purified proteins will
be produced in expression vectors. These proteins will be used in
binding studies and footprints analyses to determine which
proteins bind to the targets and where. Studies are proposed using
lac fusions to each regulatory gene to uncover the regulatory
interactions among them. The relationship between these genes
and catabolite repression will be probed.
No Sub Projects information available for 5R01GM039442-03
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