Your search keyword '"E J, Leonard"' showing total 11 results

1. Macrophage-stimulating protein, a ligand for the RON receptor protein tyrosine kinase, suppresses myeloid progenitor cell proliferation and synergizes with vascular endothelial cell growth factor and members of the chemokine family

Author

David B. Donner, Hal E. Broxmeyer, Li Lu, M.-H. Wang, Andreas H. Sarris, Zhi Hua Li, M.-S. Chang, Scott Cooper, and E. J. Leonard

Subjects

Vascular Endothelial Growth Factor A, Chemokine CXCL5, Chemokine, medicine.medical_specialty, Myeloid, medicine.medical_treatment, Bone Marrow Cells, Receptors, Cell Surface, Endothelial Growth Factors, Ligands, Colony-Forming Units Assay, Proto-Oncogene Proteins, Internal medicine, parasitic diseases, medicine, Humans, Progenitor cell, Growth Substances, Cells, Cultured, Lymphokines, biology, Hepatocyte Growth Factor, Vascular Endothelial Growth Factors, Cell growth, Growth factor, Interleukin-8, Receptor Protein-Tyrosine Kinases, Hematology, General Medicine, Growth Inhibitors, Hematopoiesis, Cell biology, Haematopoiesis, Endocrinology, medicine.anatomical_structure, biology.protein, Chemokines, Stem cell, Chemokines, CXC, Tyrosine kinase

Abstract

Macrophage-stimulating protein (MSP), originally identified as an inducer of murine resident macrophage responsiveness to chemoattractants, is a ligand for human RON/murine STK receptor protein tyrosine kinases. Since STK was cloned from populations enriched for hematopoietic stem cells, we initiated studies on the effects of MSP on colony formation by granulocyte-macrophage (CFU-GM), erythroid (BFU-E), and multipotential (CFU-GEMM) myeloid progenitor cells. MSP alone had no colony stimulating activity. However, MSP caused about a 50% suppression of CFU-GM colony formation induced by synergistic combinations of SLF or Flt-L plus GM-CSF, G-CSF, or IL-3 and of BFU-E and CFU-GEMM colonies induced by SLF or Flt3-L plus Epo or Epo and IL-3. In contrast, MSP had no effect on progenitors stimulated by one growth factor. MSP also suppressed colony formation by stimulated cord blood progenitors, but only after preinduction to a rapidly cycling state. It was previously reported that several members of the chemokine family synergistically suppress myeloid progenitor proliferation. Likewise, synergistic suppression was observed when MSP was paired with VEGF, MIP-1 alpha, IL-8, PF4, MCP-1, IP-10, or ENA-78, or when VEGF was paired with the chemokines; and the required MSP concentration was more than 100-fold less than for MSP alone. Additionally, MSP or VEGF inhibited proliferation of the human myeloid growth factor-dependent cell line, M07e, but a sustained effect required multiple additions over time. At the least, some of the MSP suppressive effects on myeloid progenitors, as assessed on single isolated CD34 marrow cells, appeared to be directly on the progenitors; sustained additions of MSP were required to see this effect. The suppressive action of MSP and its synergism with proteins of the chemokine family may be of relevance to regulation of blood cell production.

Published

1996

2. Anti-apoptotic action of macrophage stimulating protein (MSP)

Author

A, Danilkovitch-Miagkova and E J, Leonard

Subjects

Cell Survival, Hepatocyte Growth Factor, MAP Kinase Signaling System, Apoptosis, Epithelial Cells, Models, Biological, Mice, Proto-Oncogene Proteins, Cell Adhesion, Animals, Humans, Growth Substances, Protein Binding, Signal Transduction

Abstract

MSP is a serum protein belonging to the plasminogen-related kringle domain protein family. In addition to macrophages, epithelial cells are also MSP targets. MSP is a multifunctional factor regulating cell adhesion and motility, growth and survival. MSP mediates its biological activities by activating a transmembrane receptor tyrosine kinase called RON in humans or SKT in mice. MSP can protect epithelial cells from apoptosis by activating two independent signals in the PI3-K/AKT or the MAPK pathway. The MAPK pathway mediates the MSP antiapoptotic effect only if additional signaling pathways are activated through adhesion. This indicates that MSP receptors and integrins, the receptors mediating cell-matrix-dependent adhesion, can collaborate in promotion of cell survival. This adhesion-dependent pathway, which is essential for the MAPK-mediated anti-apoptotic effect, remains to be identified. A hypothesis that Stat3 might represent a key component of the adhesion-induced anti-apoptotic pathway is presented in this review.

Published

2001

3. Cross-talk between RON receptor tyrosine kinase and other transmembrane receptors

Author

A, Danilkovitch-Miagkova and E J, Leonard

Subjects

Integrins, Hepatocyte Growth Factor, Receptor Protein-Tyrosine Kinases, Receptors, Cell Surface, Receptor Cross-Talk, Cadherins, Ligands, Mice, Proto-Oncogene Proteins, Animals, Humans, Receptors, Growth Factor, Receptors, Cytokine, Growth Substances, Protein Binding, Signal Transduction

Abstract

RON is a transmembrane receptor tyrosine kinase that mediates biological activities of Macrophage Stimulating Protein (MSP). MSP is a multifunctional factor regulating cell adhesion, motility, growth and survival. MSP binding to RON causes receptor tyrosine phosphorylation leading to up-regulation of RON catalytic activity and subsequent activation of downstream signaling molecules. Recent studies show that RON is spatially and functionally associated with other transmembrane molecules including adhesion receptors integrins and cadherins, and cytokine and growth factor receptors IL-3 betac, EPOR and MET. For example, MSP-induced cell shape change is mediated via RON-activated IL-3 betac receptor. Activation of integrins causes MSP-independent RON phosphorylation, and the integrin/RON collaboration regulates cell survival. Thus, RON can be activated without MSP by ligand stimulation of RON-associated receptors, and MSP-activated RON can cause ligand-independent activation of RON-associated receptors. As a result of the receptor cross-activation RON-specific pathways become a part of a signal transduction network of other receptors, and conversely signaling pathways activated by other receptors can be used by RON. This receptor collaboration extends the spectrum of cellular responses generated by MSP and by putative ligands of RON-associated receptors. However signaling pathways involved in the receptor cross-talk and underlying activation mechanisms remain to be investigated. The purpose of this review is to summarize data and to discuss a role of cross-talk between RON and other transmembrane receptors.

Published

2001

4. Macrophage stimulating protein

Author

E J, Leonard and A, Danilkovitch

Subjects

Hepatocyte Growth Factor, Macrophages, Osteoclasts, Receptor Protein-Tyrosine Kinases, Bone Marrow Cells, Receptors, Cell Surface, Phosphatidylinositol 3-Kinases, Proto-Oncogene Proteins, ras Proteins, Animals, Humans, Protein Precursors, Growth Substances, Protein Kinases, Signal Transduction

Published

1999

5. Interaction of macrophage-stimulating protein with its receptor. Residues critical for beta chain binding and evidence for independent alpha chain binding

Author

A, Danilkovitch, M, Miller, and E J, Leonard

Subjects

DNA, Complementary, Base Sequence, Sequence Homology, Amino Acid, Hepatocyte Growth Factor, Molecular Sequence Data, Serine Endopeptidases, CHO Cells, Proto-Oncogene Proteins c-met, Cell Line, Dogs, Cricetinae, Proto-Oncogene Proteins, Animals, Amino Acid Sequence, Growth Substances, Protein Binding

Abstract

Macrophage-stimulating protein (MSP) and hepatocyte growth factor/scatter factor (HGF/SF) are plasminogen-related growth and motility factors that interact with cell-surface protein tyrosine kinase receptors. Each one is a heterodimeric protein comprising a disulfide-linked alpha chain and a serine protease-like beta chain. Despite structural similarities between MSP and HGF, the primary receptor binding site is located on the alpha chain of HGF/SF but on the beta chain of MSP. To obtain insight into the structural basis for MSP beta chain binding, beta chain structure was modeled from coordinates of an existing model of the HGF beta chain. The model revealed that the region corresponding to the S1 specificity pocket in trypsin is filled by the Asn(682)/Glu(648) interacting pair, leaving a shallow cavity for possible beta chain interaction with the receptor. Mutants in this region were created, and their binding characteristics were determined. A double mutation of Asn(682)/Glu(648) caused diminished binding of the beta chain to the MSP receptor, and a single mutation of neighboring Arg(683) completely abolished binding. Thus, this region of the molecule is critical for binding. We also found that at equimolar concentrations of free alpha and beta chains, alpha chain binding to receptor was detectable, at levels considerably lower than beta chain binding. The EC(50) values determined by quantitative enzyme-linked immunosorbent assay are 0.25 and 16.9 nM for beta and alpha chain, respectively. The data suggest that MSP has two independent binding sites with high and low affinities located in beta and alpha chain, respectively, and that the two sites together mediate receptor dimerization and subsequent activation.

Published

1999

6. Biological aspects of macrophage-stimulating protein (MSP) and its receptor

Author

E J, Leonard

Subjects

Hepatocyte Growth Factor, Hydrolysis, Macrophages, Proto-Oncogene Proteins, Ectoderm, Animals, Humans, Proteins, Receptor Protein-Tyrosine Kinases, Epithelial Cells, Receptors, Cell Surface, Protein Precursors, Growth Substances

Abstract

Macrophage-stimulating protein (MSP; also known as HGF-like protein [HGFl]) is a 78 kDa plasma protein that is secreted by the liver into the circulation as single-chain, biologically inactive pro-MSP. The presence of conserved triple disulfide loops (kringles) places pro-MSP in a family of coagulation system serine protease zymogens that are activated by proteolytic cleavage. Although pro-MSP has lost enzymic activity, it has retained the activation mechanism, in that proteolytic cleavage at a single site yields biologically active disulfide-linked alpha beta-chain heterodimeric MSP. The MSP receptor is a transmembrane protein tyrosine kinase. MSP causes phosphorylation of the receptor cytoplasmic domain, association of phosphatidylinositol (PI)-3 kinase with the receptor, and phosphorylation of receptor-bound PI-3 kinase. Inhibition of PI-3 kinase by wortmannin prevents MSP action on cells. MSP stimulates motility of murine resident peritoneal macrophages. However, it does not act on exudate macrophages or blood monocytes, since these earlier maturational stages of the lineage do not express the receptor. MSP also stimulates keratinocyte cell lines, causing either chemotactic responses or increased cell numbers in culture. We suggest that pro-MSP diffuses into local tissue sites, where proteolytic cleavage to MSP results in stimulation of keratinocytes and macrophages. It possibly plays a role in tissue injury or wound healing.

Published

1997

7. Requirement of phosphatidylinositol-3 kinase for epithelial cell migration activated by human macrophage stimulating protein

Author

M H, Wang, F A, Montero-Julian, I, Dauny, and E J, Leonard

Subjects

Phosphatidylinositol 3-Kinases, Phosphotransferases (Alcohol Group Acceptor), Cell Movement, Hepatocyte Growth Factor, Proto-Oncogene Proteins, Humans, Receptor Protein-Tyrosine Kinases, Tyrosine, Epithelial Cells, Receptors, Cell Surface, Phosphorylation, Growth Substances, Signal Transduction

Abstract

Macrophage stimulating protein (MSP) is a ligand for the RON receptor protein tyrosine kinase. Activation of RON in murine resident macrophages results in cell shape change and migration. We studied cell movement induced by MSP in different types of human epithelial cells and the possible role of phosphatidylinositol-3 (PI-3) kinase in RON-mediated signal transduction. We observed specific and saturable binding of 125I-MSP to RON on several epithelial cell lines. In addition to activation and phosphorylation of RON, MSP also induced tyrosine phosphorylation of the PI-3 kinase p85 subunit in a time-dependent manner, with a peak at 15 min. Moreover, phosphorylated RON formed a complex with PI-3 kinase in both HK-NOC keratinocyte and RON cDNA-transfected MDCK cells. An in vitro protein interaction assay confirmed that PI-3 kinase from a lysate of MSP-activated cells bound to pure RON protein. MSP, at a concentration range of 1 to 5 nM, induced migration of three epithelial cell lines. This effect was inhibited by wortmannin, a specific inhibitor for PI-3 kinase, with an IC50 of 10 nM. MSP-induced shape change in murine resident peritoneal macrophages was also abolished by wortmannin. These data suggest that activation of PI-3 kinase is required for MSP-induced epithelial cell migration. The stimulation by MSP of epithelial cell movement may have implications for tissue repair, wound healing, and tumor metastasis.

Published

1996

8. Macrophage-stimulating protein inhibits induction of nitric oxide production by endotoxin- or cytokine-stimulated mouse macrophages

Author

M H, Wang, G W, Cox, T, Yoshimura, L A, Sheffler, A, Skeel, and E J, Leonard

Subjects

Mice, Inbred C3H, Hepatocyte Growth Factor, Macrophage Activation, Nitric Oxide, Endotoxins, Kinetics, Mice, Proto-Oncogene Proteins, Macrophages, Peritoneal, Animals, Cytokines, Humans, Amino Acid Oxidoreductases, RNA, Messenger, Nitric Oxide Synthase, Growth Substances

Abstract

Human serum macrophage-stimulating protein (MSP) is a disulfide-linked heterodimer that induces motile and phagocytic activity of mouse resident peritoneal macrophages. In this work, we found that MSP blocked the increase in macrophage nitric oxide synthase mRNA, as well as the associated increase in nitric oxide production, that occurred in response to several stimuli. These included bacterial products and mammalian cytokines: endotoxin, and interferon-gamma plus endotoxin, interleukin-2, or tumor necrosis factor-alpha. The inhibition by MSP of induction of nitric oxide synthase mRNA and nitric oxide secretion was concentration-dependent. The concentration of MSP that caused maximal inhibition of nitric oxide production was comparable with the optimum for stimulation of macrophage motile and phagocytic activity. Time course studies showed that nitrite was first detected in culture fluid about 8 h after endotoxin stimulation, and it accumulated at a linear rate during the ensuing 16 h. Inhibition by MSP occurred during the 8-h lipopolysaccharide (LPS) induction period; inhibition was maximal when MSP and LPS were added together and decreased progressively to no inhibition as the interval between LPS and MSP addition increased to 11 h.

Published

1994

9. Action and target cell specificity of human macrophage-stimulating protein (MSP)

Author

A, Skeel and E J, Leonard

Subjects

Mice, Erythrocytes, Sheep, Phagocytosis, Cell Movement, Hepatocyte Growth Factor, Proto-Oncogene Proteins, Macrophages, Peritoneal, Animals, Humans, Complement C5a, In Vitro Techniques, Growth Substances

Abstract

Macrophage-stimulating protein (MSP) induces mouse resident peritoneal macrophages to become responsive to the chemoattractant C5a and to ingest C3bi-coated erythrocytes. We now show that MSP action is not limited to complement-induced responses, because it also induced responsiveness to the noncomplement chemoattractant casein. In addition to stimulating responsiveness to attractants, MSP functioned alone as a chemoattractant for resident peritoneal macrophages, with an optimal concentration of approximately 0.2 nM. A critical difference between MSP and C5a is that resident macrophages did not migrate to C5a without an additional stimulus such as MSP in the cell suspension, whereas macrophages suspended in medium alone migrated to MSP in the attractant well. Thus, in contrast to C5a, MSP seems capable of a dual role, both activator and attractant. MSP had no effect on responsiveness of mouse peritoneal exudate macrophages to C5a; nor could it attract exudate macrophages or human blood monocytes. Absorption studies showed that resident macrophages have a receptor for MSP, but exudate macrophages do not. In view of these findings, it seems that the biological role of MSP is not as a recruiter of blood monocytes to sites of inflammation, but as an activator of mature macrophages. The MSP-induced activated state for responsiveness to C5a or C3bi was transient, and decayed at a first order rate with a t 1/2 of approximately 1 h. This is a new example of the transience of activation induced in macrophages by proinflammatory stimuli.

Published

1994

10. Proteolytic conversion of single chain precursor macrophage-stimulating protein to a biologically active heterodimer by contact enzymes of the coagulation cascade

Author

M H, Wang, T, Yoshimura, A, Skeel, and E J, Leonard

Subjects

Serine Proteinase Inhibitors, Leupeptins, Macromolecular Substances, Enzyme-Linked Immunosorbent Assay, CHO Cells, Factor XIIa, Transfection, Factor XIa, Mice, Aprotinin, Cricetinae, Proto-Oncogene Proteins, Animals, Humans, Cysteine, Cloning, Molecular, Protein Precursors, Growth Substances, Cells, Cultured, Hepatocyte Growth Factor, Chemotaxis, Macrophages, Blood Coagulation Factors, Recombinant Proteins, Molecular Weight, Kinetics, Kallikreins, Protein Processing, Post-Translational

Abstract

Human serum macrophage stimulating protein (MSP) is a disulfide-linked heterodimer that induces motile and phagocytic activity of mouse resident peritoneal macrophages. It is a member of the family of kringle proteins, which typically exist in extracellular fluid as single chain precursors that are activated by proteolytic cleavage. In this work, we expressed [35S]cysteine-labeled recombinant pro-MSP in MSP cDNA-transfected Chinese hamster ovary cells and studied proteolytic processing of pro-MSP and the requirement of cleavage for biological activity. In media containing heat-inactivated fetal bovine serum, the protein was secreted as single chain pro-MSP, which was cleaved over a period of hours to the mature heterodimer. Cleavage was prevented by serine protease inhibitors such as leupeptin or aprotinin; it did not occur if cells were cultured in serum-free medium. Nanomolar concentrations of coagulation proteases kallikrein, factor XIIa or factor XIa cleaved pro-MSP to MSP within 30 min. Pro-MSP had no biological activity. After cleavage by kallikrein, biological activity was quantitatively comparable to that of natural MSP isolated from human plasma. These results support our hypothesis that MSP circulates as the biologically inactive precursor and can be activated by enzymes of the intrinsic coagulation cascade.

Published

1994

11. Cloning, sequencing, and expression of human macrophage stimulating protein (MSP, MST1) confirms MSP as a member of the family of kringle proteins and locates the MSP gene on chromosome 3

Author

T, Yoshimura, N, Yuhki, M H, Wang, A, Skeel, and E J, Leonard

Subjects

Sheep, Base Sequence, Sequence Homology, Amino Acid, Hepatocyte Growth Factor, Macrophages, Molecular Sequence Data, Chromosome Mapping, Nucleic Acid Hybridization, DNA, Peptide Fragments, Mice, Proto-Oncogene Proteins, Tumor Cells, Cultured, Animals, Humans, Amino Acid Sequence, Chromosomes, Human, Pair 3, Cloning, Molecular, Growth Substances, Cells, Cultured

Abstract

A human hepatoma (HepG2) cell line library was screened with an oligonucleotide probe for macrophage stimulating protein (MSP) to clone an MSP cDNA. Deduced sequences of isolated clones were compared with peptide fragment sequences of MSP. MSP9 cDNA encoded most of the known sequence of MSP except for a small segment of the 5' end of the open reading frame. Consequently, a hybrid 2300-base pair cDNA that encoded the complete MSP amino acid sequence was constructed from 2 clones. Culture fluid from COS-7 cells transfected with this full-length MSP cDNA had MSP biological activity, and the expressed MSP was detected by immunoprecipitation with antibody against native MSP. The deduced amino acid sequence of MSP includes 4 kringle domains, which have been found in hepatocyte growth factor and several proteins of the blood coagulation system. Among them, MSP has the highest sequence similarity to hepatocyte growth factor (45% identity). The MSP cDNA hybridized strongly to mRNA from liver, and to a lesser extent to mRNA from kidney and pancreas, suggesting that a cell type in the liver is the source of MSP. Several cloned and sequenced MSP cDNAs had insertions or deletions, suggesting that alternatively spliced MSP mRNAs may occur. This was reflected in Northern blots probed with an MSP cDNA, which showed more than one mRNA species. Furthermore, although the gene coding for MSP is on chromosome 3, the sequence of one of the cDNAs was identical with a unique sequence in chromosome 1, indicating that there may be a family of MSP genes, located on chromosomes 3 and 1.

Published

1993