Affiliation:
1. Lehrstuhl für Allgemeine und Molekulare Botanik, Ruhr-Universität, Bochum, Germany
Abstract
ABSTRACT
The homothallic filamentous ascomycete
Sordaria macrospora
possesses genes which are thought to encode two pheromone precursors and two seven-transmembrane pheromone receptors. The pheromone precursor genes are termed
ppg1
and
ppg2.
The putative products derived from the gene sequence show structural similarity to the α-factor precursors and
a
-factor precursors of the yeast
Saccharomyces cerevisiae.
Likewise, sequence similarity has been found between the putative products of the pheromone receptor genes
pre2
and
pre1
and the
S. cerevisiae
Ste2p α-factor receptor and Ste3p
a
-factor receptor, respectively. To investigate whether the α-factor-like pheromone-receptor pair of
S. macrospora
is functional, a heterologous yeast assay was used. Our results show that the
S. macrospora
α-factor-like pheromone precursor PPG1 is processed into an active pheromone by yeast
MATα
cells. The
S. macrospora
PRE2 protein was demonstrated to be a peptide pheromone receptor. In yeast
MAT
a
cells lacking the endogenous Ste2p receptor, the
S. macrospora
PRE2 receptor facilitated all aspects of the pheromone response. Using a synthetic peptide, we can now predict the sequence of one active form of the
S. macrospora
peptide pheromone. We proved that
S. macrospora
wild-type strains secrete an active pheromone into the culture medium and that disruption of the
ppg1
gene in
S. macrospora
prevents pheromone production. However, loss of the
ppg1
gene does not affect vegetative growth or fertility. Finally, we established the yeast assay as an easy and useful system for analyzing pheromone production in developmental mutants of
S. macrospora
.
Publisher
American Society for Microbiology
Subject
Molecular Biology,General Medicine,Microbiology
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