Affiliation:
1. Department of Plant and Microbial Biology, University of California, Berkeley, Berkeley, California 94720-3102
2. Oregon Health and Science University, Beaverton, Oregon 97006-8921
Abstract
ABSTRACT
Identifying and characterizing transcriptional regulatory networks is important for guiding experimental tests on gene function. The characterization of regulatory networks allows comparisons among both closely and distantly related species, providing insight into network evolution, which is predicted to correlate with the adaptation of different species to particular environmental niches. One of the most intensely studied regulatory factors in the yeast
Saccharomyces cerevisiae
is the bZIP transcription factor Gcn4p. Gcn4p is essential for a global transcriptional response when
S. cerevisiae
experiences amino acid starvation. In the filamentous ascomycete
Neurospora crassa
, the ortholog of
GCN4
is called the
c
ross
p
athway
c
ontrol-1 (
cpc-1
) gene; it is required for the ability of
N. crassa
to induce a number of amino acid biosynthetic genes in response to amino acid starvation. Here, we deciphered the CPC1 regulon by profiling transcription in wild-type and
cpc-1
mutant strains with full-genome
N. crassa
70-mer oligonucleotide microarrays. We observed that at least 443 genes were direct or indirect CPC1 targets; these included 67 amino acid biosynthetic genes, 16 tRNA synthetase genes, and 13 vitamin-related genes. Comparison among the
N. crassa
CPC1 transcriptional profiling data set and the Gcn4/CaGcn4 data sets from
S. cerevisiae
and
Candida albicans
revealed a conserved regulon of 32 genes, 10 of which are predicted to be directly regulated by Gcn4p/CPC1. The 32-gene conserved regulon comprises mostly amino acid biosynthetic genes. The comparison of regulatory networks in species with clear orthology among genes sheds light on how gene interaction networks evolve.
Publisher
American Society for Microbiology
Subject
Molecular Biology,General Medicine,Microbiology
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