Birgit Millauer
Max Planck Society
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Featured researches published by Birgit Millauer.
Cell | 1993
Birgit Millauer; Susanne Wizigmann-Voos; Harald Schnürch; Ricardo Martinez; Niels Peter H. Møller; Werner Risau; Axel Ullrich
Examination of flk-1 receptor tyrosine kinase mRNA expression by in situ hybridization analysis revealed specific association with endothelial cells at all stages of mouse development, including the blood islands in the yolk sac of day 8.5-10.5 embryos, in which the early progenitors of this lineage originate. flk-1 transcripts were abundant in proliferating endothelial cells of vascular sprouts and branching vessels of embryonic and early postnatal brain, but were drastically reduced in adult brain, where proliferation has ceased. Identification of the angiogenic mitogen, vascular endothelial growth factor (VEGF), as the high affinity ligand of Flk-1 and correlation of the temporal and spatial expression pattern of Flk-1 and VEGF suggest a major role of this ligand-receptor signaling system in vasculogenesis and angiogenesis.
Molecular and Cellular Biology | 1992
Klaus Seedorf; Birgit Millauer; Günter Kostka; Joseph Schlessinger; Axel Ullrich
Chimeric receptors composed of the human epidermal growth factor receptor (EGF-R) extracellular domain fused to wild-type and truncated platelet-derived growth factor receptor (PDGF-R) intracellular sequences were stably expressed in NIH 3T3 cells devoid of endogenous EGF-Rs. This experimental system allowed us to investigate the biological activity of PDGF-R cytoplasmic-domain mutants in PDGF-R-responsive NIH 3T3 cells by activating PDGF-specific signaling pathways with EGF. Deletion of 74 carboxy-terminal amino acids severely impaired the ability of the PDGF-R cytoplasmic domain to associate with cellular substrates in vitro. This deletion also inhibited receptor and substrate phosphorylation, reduced the receptors mitogenic activity, and completely abolished its oncogenic signaling potential. Surprisingly, removal of only six additional amino acids, including Tyr-989, restored substantial receptor and substrate phosphorylation capacity as well as transforming potential and yielded a receptor with wild-type levels of ligand-induced mitogenic activity. However, the ability of this chimera to bind phospholipase C gamma was severely impaired in comparison with the ability of the wild-type receptor, while the association with other cellular proteins was not affected. Further deletion of 35 residues, including Tyr-977, nearly abolished all PDGF-R cytoplasmic-domain biological signaling activities. None of the three C-terminal truncations completely abolished the mitogenic potential of the receptors or had any influence on ligand binding or receptor down regulation. Together, these data implicate the 80 C-terminal-most residues of the PDGF-R, and possibly Tyr-989, in phospholipase C gamma binding, while receptor sequences upstream from Asp-988 appear to be essential for specific interactions with other cellular polypeptides such as ras GTPase-activating protein and phosphatidylinositol 3-kinase. Thus, the mutants described here allow the separation of distinct PDGF-activated signaling pathways and demonstrate that phospholipase C gamma phosphorylation is not required for mitogenesis and transformation.
Nature | 1994
Birgit Millauer; Laura Kay Shawver; Karl H. Plate; Werner Risau; Axel Ullrich
Cancer Research | 1993
Karl H. Plate; Georg Breier; Birgit Millauer; Axel Ullrich; Werner Risau
Cancer Research | 1996
Birgit Millauer; Michael P. Longhi; Karl H. Plate; Laura Kay Shawver; Werner Risau; Axel Ullrich; Laurie M. Strawn
Oncogene | 1995
F. Alves; Wolfgang F. Vogel; Kevin Mossie; Birgit Millauer; Heinz Höfler; Axel Ullrich
Oncogene | 1995
Thomas Ciossek; Birgit Millauer; Axel Ullrich
Archive | 1994
Axel Ullrich; Werner Risau; Birgit Millauer
Journal of Biological Chemistry | 1991
Klaus Seedorf; Stephen Felder; Birgit Millauer; Joseph Schlessinger; Axel Ullrich
Archive | 2002
Thomas Ciossek; Axel Ullrich; Birgit Millauer