Identification of a second Grb2 binding site in the v-Fms tyrosine kinase

Mancini, Annalisa; Niedenthal, Rainer; Joos, Hans; Koch, Alexandra; Trouliaris, Sylvia; Niemann, Heiner; Tamura, Teruko

doi:10.1038/sj.onc.1201518

Cited by 50 publications

(53 citation statements)

References 24 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…The reduced binding capacity of this latter mutant is likely, however, to be caused by a diminished tyrosine kinase activity in yeast cells which was observed exclusively with this mutant. In keeping with this notion, PI-3' kinase and Grb2 also showed about 50% reduced binding to this mutant (Mancini et al, 1997). Since it is unclear which of the remaining ten tyrosine residues of the cytoplasmic domain of Fms become also phosphorylated, additional extensive experiments will be required to solve the issue whether the interaction between FMIP and Fms depends on one or more phosphotyrosine residues.…”

Section: Fmip Forms a Complex With Fms Molecules In Fdc-p1mac11 Cellsmentioning

confidence: 81%

“…The bait consisted of the cytoplasmic domain of mouse c-Fms fused to the C terminus of the DNA-binding and dimerization domain of LexA. Upon expression of the fusion protein in yeast cells, dimerization leads to interchain tyrosine phosphorylation of the two Fms receptor segments (Mancini et al, 1997), thus allowing us to screen a mouse embryo cDNA library with a Fms molecule representing the activated receptor phenotype. A total of 157 cDNA clones of various length were obtained, together encoding seven di erent proteins.…”

Section: Detection Of Fmip a Novel Binding Partner Of C-fmsmentioning

confidence: 99%

“…These mutants included Y543F devoid of the p55 binding site (Joos et al, 1996), Y558/568F in which the reported Src attachment sites were mutated (Courtneidge et al, 1993), Y705F lacking the binding site for Stat1 (Novak et al, 1996), Y720F with a mutation of the PI-3'-kinase binding site (Reedijk et al, 1992, Y807F lacking the putative binding site of p120RasGAP (Trouliaris et al, 1995), and Y696/921F in which the two Grb2 binding sites are destroyed (Mancini et al, 1997). However, with the exception of the Y807F mutant, none of the aforementioned mutations in¯uenced binding of FMIP to a signi®cant extent (Figure 4b).…”

Section: Fmip Forms a Complex With Fms Molecules In Fdc-p1mac11 Cellsmentioning

confidence: 99%

“…The construction of LexA fusion genes encoding the cytoplasmic domains of c-Fms, TrkA, c-Met, and c-Kit downstream of LexA, the expression in E. coli pBTM116 and S. cerevisiae strain L40 were described previously (Weidner et al, 1996;Mancini et al, 1997). Fms-mutants containing tyrosine/phenylalanine replacements have been described (Mancini et al, 1997).…”

Section: Plasmid Constructions Transfection and Yeast Two-hybrid Scmentioning

confidence: 99%

“…Fms-mutants containing tyrosine/phenylalanine replacements have been described (Mancini et al, 1997). Yeast clones were selected in medium lacking uracil and tryptophan.…”

Section: Plasmid Constructions Transfection and Yeast Two-hybrid Scmentioning

confidence: 99%

See 4 more Smart Citations

FMIP, a novel Fms-interacting protein, affects granulocyte/macrophage differentiation

et al. 1999

Self Cite

View full text Add to dashboard Cite

Hematopoietic cell growth, di erentiation, and commitment to a restricted lineage are guided by a set of cytokines acting exclusively on cells expressing the corresponding cytokine receptor. The macrophage colony stimulating factor (M-CSF, also termed CSF-1) and its cognate receptor, the tyrosine kinase c-Fms, are essential for monocyte and macrophage development. The underlying molecular mechanism, however, is poorly understood. Here we identi®ed a novel Fms-interacting protein (FMIP, MW 78 kDa) which binds transiently via its Nterminal 144 residues to the cytoplasmic domain of activated Fms-molecules. Binding of FMIP was paralleled by rapid tyrosine phosphorylation within the binding domain which drastically reduced its ability to associate with Fms. Binding was speci®c as evidenced by co-immunoprecipitation and association with recombinant GST-Fms fusion proteins. No binding was observed with the tyrosine phosphorylated cytoplasmic domains of c-Kit, TrkA, c-Met, and the insulin receptor. The role of FMIP in hematopoietic di erentiation was studied in the bipotential myeloid progenitor cell line, FDC-P1Mac11. Overexpression of FMIP prevented M-CSF induced macrophage di erentiation. Instead, cells di erentiated into granulocytes. Our data suggest that the level of FMIP expression could form a threshold that decides about di erentiation either into macrophages or into granulocytes.

show abstract

Section: Fmip Forms a Complex With Fms Molecules In Fdc-p1mac11 Cellsmentioning

confidence: 81%

Section: Detection Of Fmip a Novel Binding Partner Of C-fmsmentioning

confidence: 99%

Section: Fmip Forms a Complex With Fms Molecules In Fdc-p1mac11 Cellsmentioning

confidence: 99%

Section: Plasmid Constructions Transfection and Yeast Two-hybrid Scmentioning

confidence: 99%

“…Fms-mutants containing tyrosine/phenylalanine replacements have been described (Mancini et al, 1997). Yeast clones were selected in medium lacking uracil and tryptophan.…”

Section: Plasmid Constructions Transfection and Yeast Two-hybrid Scmentioning

confidence: 99%

See 3 more Smart Citations

FMIP, a novel Fms-interacting protein, affects granulocyte/macrophage differentiation

et al. 1999

Self Cite

View full text Add to dashboard Cite

show abstract

fmsProtooncogene

Tamura¹,

Mancini²

2002

Wiley Encyclopedia of Molecular Medicine

View full text Add to dashboard Cite

Fine‐tuning osteoclastogenesis: An insight into the cellular and molecular regulation of osteoclastogenesis

Anwar

Sapra

Gupta

et al. 2023

Journal Cellular Physiology

View full text Add to dashboard Cite

Osteoclasts, the bone-resorbing cells, are essential for the bone remodeling process and are involved in the pathophysiology of several bone-related diseases. The extensive corpus of in vitro research and crucial mouse model studies in the 1990s demonstrated the key roles of monocyte/macrophage colony-stimulating factor, receptor activator of nuclear factor kappa B ligand (RANKL) and integrin αvβ3 in osteoclast biology. Our knowledge of the molecular mechanisms by which these variables control osteoclast differentiation and function has significantly advanced in the first decade of this century. Recent developments have revealed a number of novel insights into the fundamental mechanisms governing the differentiation and functional activity of osteoclasts; however, these mechanisms have not yet been adequately documented. Thus, in the present review, we discuss various regulatory factors including local and hormonal factors, innate as well as adaptive immune cells,noncoding RNAs (ncRNAs), etc., in the molecular regulation of the intricate and tightly regulated process of osteoclastogenesis. ncRNAs have a critical role as epigenetic controllers of osteoclast physiologic activities, including differentiation and bone resorption. The primary ncRNAs, which include micro-RNAs, circular RNAs, and long noncoding RNAs, form a complex network that affects gene transcription activities associated with osteoclast biological activity. Greater knowledge of the involvement of ncRNAs in osteoclast biological activities will contribute to the treatment and management of several skeletal diseases such as osteoporosis, osteoarthritis, rheumatoid arthritis, etc. Moreover, we further outline potential therapies targeting these regulatory pathways of osteoclastogenesis in distinct bone pathologies.

show abstract

Identification of a second Grb2 binding site in the v-Fms tyrosine kinase

Cited by 50 publications

References 24 publications

FMIP, a novel Fms-interacting protein, affects granulocyte/macrophage differentiation

FMIP, a novel Fms-interacting protein, affects granulocyte/macrophage differentiation

fmsProtooncogene

Fine‐tuning osteoclastogenesis: An insight into the cellular and molecular regulation of osteoclastogenesis

Contact Info

Product

Resources

About