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Query: EC:2.7.10.1 (
ERK
)
95,504
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
Scatter factor/hepatocyte growth factor (SF/
HGF
) is a pleiotrophic cytokine that stimulates motility and invasion of several cancer cell types and induces angiogenesis. Its receptor
MET
is a transmembrane tyrosine kinase encoded by the C-MET proto-oncogene. To assess the potential relevance of SF/
HGF
in gliomas we performed functional studies in vivo and in vitro, expression analyses and correlative studies. We showed that both SF/
HGF
and
MET
are expressed in gliomas in vivo and are upregulated during transition from low grade to malignant glioma. When SF/
HGF
cDNA was transfected into glioma cells that expressed the
MET
receptor the cells formed considerably larger and more vascularized intracranial tumors in vivo than SF/
HGF
negative control clones. In other glioma cells, which constitutively expressed both SF/
HGF
and
MET
, we abolished SF/
HGF
expression by antisense ribozyme-targeting, which led to a significant decrease in tumorigenicity and tumor growth. In vitro SF/
HGF
strongly stimulated glioma cell motility and to a lesser degree proliferation. SF/
HGF
also strongly increased endothelial cell motility in vitro and extracts of tumors derived from SF/
HGF
-transfected glioma cells were more mitogenic for endothelial cells and more angiogenic in the rat cornea angiogenesis assay than extracts from control tumors. In a three-dimensional in vitro angiogenesis assay basic fibroblast growth factor (bFGF) was found to synergize with either SF/
HGF
or vascular endothelial growth factor (VEGF) in inducing endothelial capillary-like tubes, whereas neither SF/
HGF
nor VEGF alone or in combination were effective. Interestingly, while both VEGF and SF/
HGF
levels appeared to be increased in malignant gliomas compared with low grade ones, this was not the case for bFGF of which biologically relevant levels were already present in low grade gliomas. It thus seems that bFGF alone is insufficient to induce angiogenesis in gliomas but may act synergistically with either VEGF and/or SF/
HGF
when these become upregulated during malignant progression. In conclusion, we showed that SF/
HGF
may contribute to glioma progression by stimulating tumor invasiveness, proliferation and neovascularization.
...
PMID:Scatter factor/hepatocyte growth factor (SF/HGF) content and function in human gliomas. 1057 13
Hepatocyte Growth Factor, also known as Scatter Factor, is a polypeptide that shows structural homology with enzymes of the blood coagulation cascade. It is a biologically inactive single chain precursor that is then cleaved by specific serine proteases to a fully active alphabeta heterodimer. All the biological responses induced by
HGF
/SF are elicited by binding to its receptor, a transmembrane tyrosine kinase encoded by the
MET
proto-oncogene. The signaling cascade triggered by
HGF
begins with the autophosphorylation of the receptor and is mediated by concomitant activation of different cytoplasmic effectors that bind to the same multifunctional docking site. During development,
HGF
function is essential: knock-out mice for both ligand and receptor show an embryonic lethal phenotype.
HGF
/SF displays a unique feature in inducing "branching morphogenesis", a complex program of proliferation and motogenesis in a number of different cell types. Moreover,
HGF
is involved in the invasive behaviour of several tumor cells both in vivo and in vitro. The role of
HGF
as putative therapeutical agent in pathologies characterized by massive cell loss or deregulated cell proliferation is under investigation.
...
PMID:HGF: a multifunctional growth factor controlling cell scattering. 1064 89
The
MET
proto-oncogene, encoding the tyrosine kinase receptor for
HGF
, controls genetic programs leading to cell growth, invasiveness, and protection from apoptosis. Recently,
MET
mutations have been identified in hereditary and sporadic forms of papillary renal carcinoma (PRC). Introduction of different naturally occurring mutations into the
MET
cDNA results in the acquisition of distinct biochemical and biological properties of transfected cells. Some mutations result in a high increase in tyrosine kinase activity and confer transforming ability in focus forming assays. These mutants hyperactivate the Ras signaling pathway. Other mutations are devoid of transforming potential but are effective in inducing protection from apoptosis and sustaining anchorage-independent growth. These Met(PRC) receptors interact more efficiently with the intracellular transducer Pi3Kinase. The reported results show that
MET
(PRC) mutations can be responsible for malignant transformation through different mechanisms, either by increasing the growth ability of cells or by protecting cells from apoptosis and allowing accumulation of other genetic lesions.-Giordano, S., Maffe, A., Williams, T. A., Artigiani, S., Gual, P., Bardelli, A., Basilico, C., Michieli, P., Comoglio, P. M. Different point mutations in the met oncogene elicit distinct biological properties.
...
PMID:Different point mutations in the met oncogene elicit distinct biological properties. 1065 96
Overexpression of the hepatocyte growth factor receptor (Met/HGF receptor), a transmembrane tyrosine kinase encoded by the
MET
proto-oncogene, is involved in transformation and invasive behavior of human carcinomas and sarcomas. We have previously found that bone sarcomas express high levels of Met/HGF receptor while in some cases the ligand
HGF
is co-expressed with the receptor, activating an autocrine loop. In this study, we analyzed 40 biopsy samples of a collection of giant cell tumors and other rare benign tumors of bone for expression of the
MET
proto-oncogene. These included nonossifying fibromas, osteoblastomas, desmoplastic fibromas of bone, chondroblastomas, and giant cell tumors of bone. Snap frozen samples were tested for the
MET
and
HGF
gene expression by immuno-histochemistry and Western blotting with anti-
MET
antibodies and RT-PCR. Over 50% of all cases scored positive for
MET
expression being constantly positive in recurrent or locally aggressive lesions. Sporadic co-expression of the Met/HGF receptor and ligand is also demonstrated. Met/HGF receptor expression in benign bone neoplasms suggests its early involvement in sarcomagenesis.
...
PMID:The expression of Met/hepatocyte growth factor receptor gene in giant cell tumors of bone and other benign musculoskeletal tumors. 1086 43
Scatter Factors control a complex genetic program known as 'invasive growth'.
HGF
(Scatter factor 1) and MSP (Scatter Factor 2) bind to tyrosine kinase receptors encoded by the proto-oncogenes
MET
and
RON
. Using the appropriate 'kinase inactive' mutant receptors, we show that ligand-induced activation of Met results in transphosphorylation of Ron, and vice versa. Transphosphorylation is direct, as it occurs in Met or Ron receptors lacking the docking sites for signal transducers. Phosphate groups are transferred to the tyrosine phosphorylation sites responsible both for kinase up-regulation (Met: Y1234/Y1235 and Ron: Y1238/Y1239) and for generation of signal transducer docking sites (Met: Y1349/Y1356 and Ron Y1353/Y1360). The transphosphorylation specifically takes place for the receptor subfamily, as it is not observed between Met or Ron and ErbB1, ErbB2 or TrkA. Cross-linking experiments show that non-covalent Met-Ron complexes are present on the cell surface, before ligand-induced dimerization. Co-expression of a kinase inactive Ron receptor with naturally-occurring oncogenic Met mutants suppresses the transforming phenotype, suggesting a dominant negative role for the inefficient kinase partner. These data show that, while specific for their ligands, scatter factor receptors cross-talk and cooperate in intracellular signaling.
...
PMID:Cross-talk between the proto-oncogenes Met and Ron. 1087 56
Satellite cells are the myogenic precursors in postnatal muscle and are situated beneath the myofiber basement membrane. We previously showed that fibroblast growth factor 2 (FGF2, basic FGF) stimulates a greater number of satellite cells to enter the cell cycle but does not modify the overall schedule of a short proliferative phase and a rapid transition to the differentiated state as the satellite cells undergo myogenesis in isolated myofibers. In this study we investigated whether other members of the FGF family can maintain the proliferative state of the satellite cells in rat myofiber cultures. We show that FGF1, FGF4, and FGF6 (as well as hepatocyte growth factor,
HGF
) enhance satellite cell proliferation to a similar degree as that seen with FGF2, whereas FGF5 and FGF7 are ineffective. None of the growth factors prolongs the proliferative phase or delays the transition of the satellite cells to the differentiating, myogenin(+) state. However, FGF6 retards the rapid exit of the cells from the myogenin(+) state that routinely occurs in myofiber cultures. To determine which of the above growth factors might be involved in regulating satellite cells in vivo, we examined their mRNA expression patterns in cultured rat myofibers using RT-PCR. The expression of all growth factors, excluding FGF4, was confirmed. Only FGF6 was expressed at a higher level in the isolated myofibers and not in the connective tissue cells surrounding the myofibers or in satellite cells dissociated away from the muscle. By Western blot analysis, we also demonstrated the presence of FGF6 protein in the skeletal musle tissue. Our studies therefore suggest that the myofibers serve as the main source for the muscle FGF6 in vivo. We also used RT-PCR to analyze the expression patterns of the four tyrosine kinase FGF receptors (
FGFR1
-
FGFR4
) and of the HGF receptor (c-met) in the myofiber cultures. Depending on the time in culture, expression of all receptors was detected, with
FGFR2
and
FGFR3
expressed only at a low level. Only
FGFR4
was expressed at a higher level in the myofibers but not the connective tissue cell cultures.
FGFR4
was also expressed at a higher level in satellite cells compared to the nonmyogenic cells when the two cell populations were released from the muscle tissue and fractionated by Percoll density centrifugation. The unique localization patterns of FGF6 and
FGFR4
may reflect specific roles for these members of the FGF signaling complex during myogenesis in adult skeletal muscle.
...
PMID:Gene expression patterns of the fibroblast growth factors and their receptors during myogenesis of rat satellite cells. 1089 1
CrkII, a 40 kDa adaptor possessing a Src homology (SH)2 domain followed by two SH3 domains, although not endowed with catalytic activity, participates in intracellular signalling, presumably by activating the Ras pathway. CrkII was found to be phosphorylated in response to hepatocyte growth factor/scatter factor (
HGF
/SF) and to associate with the beta-subunit of the HGF receptor (
MET
). CrkII associated with p(145betaMET) via its SH2 domain. Growth-factor-receptor-bound protein 2 (Grb2) co-immunoprecipitated with CrkII species. By transient transfection of A431 human epidermoid carcinoma cells with wild-type and dominant-negative Grb2 expression constructs lacking either the SH2 or SH3 domains, we have concluded that Grb2 does not contribute to the 'presentation' of CrkII to p(145betaMET). Overexpression of wild-type CrkII in A431 cells enhanced
HGF
/SF-induced proliferation, while a CrkII dominant-negative mutant lacking the SH2 domain prevented a similar proliferating response to
HGF
/SF. The effect of CrkII on
HGF
/SF-induced proliferation was also abolished in cells co-expressing CrkII and Son-of-sevenless lacking the guanine exchange domain, suggesting that CrkII is likely to induce cell proliferation partly via the Ras/mitogen-activated protein kinase route.
...
PMID:The beta-subunit of the hepatocyte growth factor/scatter factor (HGF/SF) receptor phosphorylates and associates with CrkII: expression of CrkII enhances HGF/SF-induced mitogenesis. 1097 Aug 10
We review here signalling complexes that we have defined using X-ray analysis in our laboratory. They include growth factors and their receptors: nerve growth factor (NGF) and its hetero-hexameric 7S NGF storage complex, hepatocyte growth factor/scatter factor (
HGF
/SF) NK1 dimers and fibroblast growth factor (FGF1) in complex with its receptor (
FGFR2
) ectodomain and heparin. We also review our recent structural studies on intracellular signalling complexes, focusing on phosducin transducin GPry, CK2 protein kinase and its complexes, and the cyclin D-dependent kinase, Cdk6, bound to the cell cycle inhibitor p19INK4d. Comparing the structures of these complexes with others we show that the surface area buried in signalling interactions does not always give a good indication of the strength of the interactions. We show that conformational changes are often important in complexes with intermediate buried surface areas of 1500 to 2000 A2, such as Cdk6INK4 interactions. Some interactions involve recognition of continuous epitopes, where there is no necessity for a tertiary structure and very often the binding conformation is induced during the process of interaction, for example phosducin binding to the betagamma subunits (Gtbetagamma) of the heterotrimeric G protein transducin.
...
PMID:Protein-protein interactions in receptor activation and intracellular signalling. 1107 27
Scatter factor/hepatocyte growth factor (SF/
HGF
) is a pleiotropic cytokine that has been implicated in glioma invasion and angiogenesis. The SF/HGF receptor,
MET
, has been found to be expressed in neoplastic astrocytes as well as in endothelial cells of the tumor vasculature. Both SF/
HGF
and
MET
expression have also been described to correlate with the malignancy grade of human gliomas. However, most glioblastoma cell lines lack SF/
HGF
expression, raising the question of the cellular origin of SF/
HGF
in vivo. Using in situ hybridization, we analyzed glioblastomas, anaplastic astrocytomas, diffuse astrocytomas, pilocytic astrocytomas, and normal brain for the expression of SF/
HGF
mRNA. We detected strong SF/
HGF
expression by the majority of the tumor cells and by vascular endothelial cells in all glioblastoma specimens analyzed. Combined use of in situ hybridization with fluorescence immunohistochemistry confirmed the astrocytic origin of the SF/
HGF
-expressiong cells. In contrast, CD68-immunoreactive microglia/macrophages, as well as vascular smooth muscle cells reactive to alpha-smooth muscle actin, lacked SF/
HGF
expression. In anaplastic, diffuse, and pilocytic astrocytomas, SF/
HGF
expression was confined to a subset of tumor cells, and signals were less intense than in glioblastomas. In addition, we detected SF/
HGF
mRNA in cortical neurons. SF/
HGF
expression was not up regulated around necroses or at tumor margins.
MET
immunoreactivity was observed in GFAP-expressing astrocytic tumor cells and endothelial cells as well as in a subset of microglia/macrophages. We conclude that in vivo, both autocrine and paracrine stimulation of tumor cells and endothelium through the SF/
HGF
-
MET
system are likely to contribute to tumor invasion and angiogenesis. Lack of SF/
HGF
expression by most cultured glioblastoma cells is not representative of the in vivo situation and most likely represents a culture artifact.
...
PMID:Expression and localization of scatter factor/hepatocyte growth factor in human astrocytomas. 1129 84
Signal transduction by HGF receptor, the tyrosine kinase encoded by the
MET
oncogene, switches on a genetic program called 'invasive growth' inducing epithelial cell dissociation, migration, growth, and ultimately leading to differentiation into branched tubular structures. Sustained tyrosine phosphorylation of the downstream adaptor protein Gab1 is required for the
HGF
response. Here we show that serine/threonine phosphorylation of Gab1 provides a control mechanism for negative regulation. Treatment with okadaic acid, a potent inhibitor of the serine/threonine protein phosphatases PP1 and PP2A, was followed by activation of a number of serine/threonine kinases, hyper-phosphorylation in serine and threonine of Gab1 and severe inhibition of the
HGF
-induced biological responses. Under these conditions, Gab1 was found to be concomitantly hypo-phosphorylated in tyrosine, and thus endowed with reduced ability to recruit SH2 containing signal transducers such as PI3 kinase. Among the serine-threonine kinases activated by PP1 and PP2A inhibition, we found that PKC-alpha and PKC-beta1 are required for negative regulation of Gab1. These data provide a novel negative mechanism for the HGF receptor signaling pathways and highlight a potentially useful target for inhibitors of invasive growth.
...
PMID:Gab1 phosphorylation: a novel mechanism for negative regulation of HGF receptor signaling. 1131 45
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