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Vol. 11, Issue 5, 1631-1643, May 2000
and
*Department of Genetics, Kassel University, 34132 Kassel, Germany;
and Discoidin I expression was used as a marker to screen for mutants
affected in the growth-differentiation transition (GDT) of
Dictyostelium. By REMI mutagenesis we
have isolated mutant 2-9, an overexpressor of discoidin I. It displays
normal morphogenesis but shows premature entry into the developmental
cycle. The disrupted gene was denominated gdt1. The
mutant phenotype was reconstructed by disruptions in different parts of
the gene, suggesting that all had a complete loss of function.
gdt1 was expressed in growing cells; the levels of
protein and mRNA appear to increase with cell density and rapidly
decrease with the onset of development. gdt1 encodes a
175-kDa protein with four putative transmembrane domains. In the C
terminus, the derived amino acid sequence displays some
similarity to the catalytic domain of protein kinases. Mixing experiments demonstrate that the gdt1
Abteilung Zellbiologie, Max-Planck-Institut
für Biochemie, D-82512 Martinsried, Germany
phenotype is cell autonomous. Prestarvation factor is secreted at
wild-type levels. The response to folate, a negative regulator of
discoidin expression, was not impaired in gdt1 mutants.
Cells that lack the G protein
2 display a loss of discoidin
expression and do not aggregate.
gdt1
/G
2
double mutants show no aggregation but strong discoidin expression. This suggests that gdt1 is a negative regulator of the GDT downstream of or in a parallel pathway to G
2.
Corresponding author. E-mail address:
nellen{at}hrz.uni-kassel.de.
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