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Query: EC:3.4.21.5 (
thrombin
)
33,306
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
Tumor growth and metastasis are angiogenesis-dependent and tumor angiogenesis is a result of complex interplay of positive and negative regulators. Vascular endothelial growth factor (VEGF) occupies a particular place among the positive regulators of angiogenesis due to its potency and specificity for endothelial cells. VEGF upregulates several molecules such as growth factors, adhesion molecules, proteases, and protease receptors and it actually induces microvascular hyperpermeability, resulting in activation of
thrombin
from prothrombin.
Osteopontin
(
OPN
) is a secreted arginine-glycine-asparic acid (RGD)-containing phosphoprotein and it contains a predicted
thrombin
cleavage site.
OPN
binds to several integrins and CD44 variants.
OPN
has diverse functions such as cell adhesion, chemoattraction, and immunomodulation, and it induces endothelial cell migration and upregulates endothelial cell migration induced by VEGF.
OPN
expression is upregulated in human carcinomas. This review documents the functional roles of VEGF and
OPN
in angiogenesis and their clinical significance in tumor biology.
...
PMID:Vascular endothelial growth factor and osteopontin in tumor biology. 1100 9
Osteopontin
(
OPN
) is a phosphoprotein secreted by many cells of epithelial, mesenchymal, and hematopoietic origin. In the kidney,
OPN
is expressed in the renal tubules and collecting ducts and is excreted into the urine. A pathophysiologic role for urinary
OPN
has not been established. In this study, urinary excretion of
OPN
was analyzed in patients with primary glomerular diseases, including immunoglobulin A nephropathy (IgAN; n = 32), minimal change nephrotic syndrome (MCNS; n = 16), and membranous nephropathy (MN; n = 18). Compared with normal controls (n = 20), mean +/- SD of urinary
OPN
in IgAN patients was decreased significantly (21.4 +/- 6.2 versus 11.6 +/- 9.6 mg/g creatinine, P: < 0.001). In contrast, the levels of urinary
OPN
in patients with MCNS or MN did not differ significantly from normal values. Immunoblot analysis showed that
OPN
is present as a 55- to 60-kd molecule in normal urine. A 34-kd fragment of
OPN
was the major immunoreactive band in samples from IgAN patients. This fragment also was detectable in the urine from some patients with MCNS or MN but was absent in normal subjects.
OPN
has a
thrombin
-cleavage site near its central portion. Thrombin treatment of the urine from normal controls could result in 34-kd
OPN
fragments. Although the underlying mechanisms remain to be determined, these data provide evidence that secretion or processing (or both) of urinary
OPN
is altered in patients with IgAN.
...
PMID:Reduced urinary excretion of intact osteopontin in patients with IgA nephropathy. 1115 80
The integrin alpha9beta1 mediates neutrophil migration across several ligands that are enriched at sites of inflammation. In one of these ligands, the acidic phosphoprotein
osteopontin
, the alpha9beta1 binding site is cryptic, but is revealed after
thrombin
cleavage. We have recently mapped the alpha9beta1 binding site in
osteopontin
to the linear peptide sequence, SVVYGLR, immediately adjacent to the
thrombin
cleavage site. Interestingly, this site is also adjacent to a sequence (RGD) through which five other integrins bind to
osteopontin
. These findings suggest a novel mechanism by which
thrombin
can modulate integrin signaling at sites of tissue injury.
...
PMID:Mapping of the cryptic integrin-binding site in osteopontin suggests a new mechanism by which thrombin can regulate inflammation and tissue repair. 1123 95
Previous work from our laboratory demonstrates that the alpha(4)beta(1) integrin is an adhesion receptor for
OPN
and that alpha(4)beta(1) binding site(s) are present in the N-terminal
thrombin
fragment of
osteopontin
(
OPN
) (Bayless, K. J., Meininger, G. A., Scholtz, J. M., and Davis, G. E. (1998) J. Cell Sci. 111, 1165-1174). The work presented here identifies two alpha(4)beta(1) binding sites within a recombinantly produced N-terminal
thrombin
fragment of human
OPN
. Initial experiments, using wild-type
OPN
containing an RGD sequence or an
OPN
-RGE mutant, showed identical alpha(4)beta(1)-dependent cell adhesive activity. A strategy to localize alpha(4)beta(1) binding sites within the
thrombin
fragment of
osteopontin
involved performing a series of truncation analyses. Removal of the last 39 amino acids (130) completely eliminated adhesion, indicating all binding activity was present within that portion of the molecule. Combined mutation and deletion analyses of this region revealed the involvement of dual alpha(4)beta(1) binding sites. Synthetic peptides for both regions in
OPN
, ELVTDFPTDLPAT (131) and SVVYGLR (162), were found to block alpha(4)beta(1)-dependent adhesion. The first peptide when coupled to Sepharose bound the alpha(4)beta(1) integrin directly whereas a mutated ELVTEFPTELPAT peptide showed a dramatically reduced ability to bind. These data collectively demonstrate that dual alpha(4)beta(1) integrin binding sites are present in a 38 amino acid domain within the N-terminal
thrombin
fragment of
OPN
.
...
PMID:Identification of dual alpha 4beta1 integrin binding sites within a 38 amino acid domain in the N-terminal thrombin fragment of human osteopontin. 1127 97
Osteopontin
(
OPN
) is a secreted phosphoprotein shown to function in wound healing, inflammation, and tumor progression. Expression of
OPN
is often co-localized with members of the matrix metalloproteinase (MMP) family. We report that
OPN
is a novel substrate for two MMPs, MMP-3 (stromelysin-1) and MMP-7 (matrilysin). Three cleavage sites were identified for MMP-3 in human
OPN
, and two of those sites were also cleaved by MMP-7. These include hydrolysis of the human Gly166-Leu167, Ala201-Tyr202 (MMP-3 only), and Asp210-Leu211 peptide bonds. Only the N-terminal Gly-Leu cleavage site is conserved in rat
OPN
(Gly151-Leu152). These sites are distinct from previously reported cleavage sites in
OPN
for the proteases
thrombin
or enterokinase. We found evidence for the predicted MMP cleavage fragments of
OPN
in vitro in tumor cell lines, and in vivo in remodeling tissues such as the postpartum uterus, where
OPN
and MMPs are co-expressed. Furthermore, cleavage of
OPN
by MMP-3 or MMP-7 potentiated the function of
OPN
as an adhesive and migratory stimulus in vitro through cell surface integrins. We predict that interaction of MMPs with
OPN
at tumor and wound healing sites in vivo may be a mechanism of regulation of
OPN
bioactivity.
...
PMID:Osteopontin, a novel substrate for matrix metalloproteinase-3 (stromelysin-1) and matrix metalloproteinase-7 (matrilysin). 1137 93
The
osteopontin
SVVYGLR motif binds the integrins alpha(4)beta(1) and alpha(9)beta(1). We show that alpha(4)beta(7) also interacts with this motif and that an SVVYGLR-OH peptide antagonises the alpha(4)beta(7) MAdCAM interaction. The important elements of this motif required to bind alpha(4)beta(1) and alpha(4)beta(7) were probed using a series of mutated peptides based around SVVYGLR. Leu167 is important for the interaction with alpha(4) integrins, as is the C-terminal carboxylic acid of Arg168 exposed by
thrombin
cleavage. The importance of the acidic group means that SVVYGLR has structural elements in common with other alpha(4) integrin-binding motifs and suggests why
thrombin
cleavage activates this motif.
...
PMID:Structural elements of the osteopontin SVVYGLR motif important for the interaction with alpha(4) integrins. 1151 58
Osteopontin
(
OPN
) is a secreted glycoprotein in both phosphorylated and non-phosphorylated forms. It contains an Arg-Gly-Asp cell-binding sequence and a
thrombin
-cleavage site.
OPN
is mainly present in the loop of Henle and distal nephrons in normal kidneys in animals and humans. After renal damage,
OPN
expression may be significantly up-regulated in all tubule segments and glomeruli. Studies utilizing
OPN
gene-deficient mice, antisense-treated or anti-
OPN
-treated animals have demonstrated that
OPN
promotes accumulation of macrophages, and may play a role in macrophage-mediated renal injury, but that the effect may be mild and short-lived. On the other hand,
OPN
has some renoprotective actions in renal injury, such as increasing tolerance to acute ischemia, inhibiting inducible nitric oxide synthase and suppressing nitric oxide synthesis, reducing cell peroxide levels and promoting the survival of cells exposed to hypoxia, decreasing cell apoptosis and participating in the regeneration of cells. In addition,
OPN
is associated with renal stones, but whether it acts as a promoter or inhibitor of stone formation is controversial. It has been demonstrated that
OPN
receptors include two families: integrin and CD44. The
OPN
integrin receptors include alpha(v)beta(3), alpha(v)beta(1), alpha(v)beta(5) and alpha(9)beta(1), and alpha(4)beta(1). In normal human kidneys, standard CD44 is expressed most dominantly. Different
OPN
functions are mediated via distinct receptors. Parathyroid hormone, vitamin D(3), calcium, phosphate and some cytokines increase
OPN
expression in vitro or in vivo, whereas female sex hormones and angiotensin-converting enzyme inhibitors or angiotensin II receptor antagonists decrease
OPN
expression in some renal damage states.
...
PMID:Expression, roles, receptors, and regulation of osteopontin in the kidney. 1170 81
Osteopontin
(
OPN
) is a secreted protein that has been implicated in diverse physiological and pathological processes.
OPN
can bind to integrins, via GRGDS or SVVYGLR amino acid sequences, and to other cell surface receptors, and many of
OPN
's functions are likely mediated via cell adhesion and subsequent signaling. Here we developed and characterized a series of five monoclonal antibodies, raised to distinct internal peptide sequences of human
OPN
, and have used these sequence-specific reagents, along with the previously described anti-
OPN
monoclonal antibody mAb53, to map functional epitopes of
OPN
that are important to cell adhesion and migration. All antibodies were reactive with native as well as recombinant human
OPN
. One antibody (2K1) raised against the peptide VDTYDGRGDSVVYGLRS could inhibit RGD-dependent cell binding to
OPN
, with an efficacy comparable to that of mAb53. Furthermore, 2K1 could inhibit alpha9 integrin-dependent cell binding to
OPN
. The epitope recognized by 2K1 was not destroyed by
thrombin
digestion, whereas mAb53 has been shown to be unable to react with
OPN
following
thrombin
cleavage. The two distinct epitopes defined by 2K1 and mAb53 antibodies are closely related to the SVVYGLR cell-binding domain and the GLRSKS containing
thrombin
cleavage site, respectively, and are involved in cell binding and cell migration.
...
PMID:Mapping of functional epitopes of osteopontin by monoclonal antibodies raised against defined internal sequences. 1178 71
Neutrophil-independent macrophage responses are a prominent part of delayed-type immune and healing processes and depend on T cell-secreted cytokines. An important mediator in this setting is the phosphoprotein
osteopontin
, whose secretion by activated T cells confers resistance to infection by several intracellular pathogens through recruitment and activation of macrophages. Here, we analyze the structural basis of this activity following cleavage of the phosphoprotein by
thrombin
into two fragments. An interaction between the C-terminal domain of
osteopontin
and the receptor CD44 induces macrophage chemotaxis, and engagement of beta(3)-integrin receptors by a nonoverlapping N-terminal
osteopontin
domain induces cell spreading and subsequent activation. Serine phosphorylation of the
osteopontin
molecule on specific sites is required for functional interaction with integrin but not CD44 receptors. Thus, in addition to regulation of intracellular enzymes and substrates, phosphorylation also regulates the biological activity of secreted cytokines. These data, taken as a whole, indicate that the activities of distinct
osteopontin
domains are required to coordinate macrophage migration and activation and may bear on incompletely understood mechanisms of delayed-type hypersensitivity, wound healing, and granulomatous disease.
...
PMID:Phosphorylation-dependent interaction of osteopontin with its receptors regulates macrophage migration and activation. 1237 45
It has been shown that
osteopontin
(
OPN
) plays a pivotal role in the pathogenesis of rheumatoid arthritis (RA). However, the molecular mechanism of
OPN
action is yet to be elucidated. Splenic monocytes obtained from arthritic mice exhibited a significant capacity for cell migration toward
thrombin
-cleaved
OPN
but not toward full-length
OPN
. Migratory monocytes expressed alpha9 and alpha4 integrins. Since cleavage of
OPN
by
thrombin
exposes the cryptic epitope recognized by alpha9 and alpha4 integrins, we investigated the role of the cryptic epitope SLAYGLR in a murine RA model by using a specific antibody (M5) reacting to SLAYGLR sequence. The M5 antibody could abrogate monocyte migration toward the
thrombin
-cleaved form of
OPN
. Importantly, M5 antibody could inhibit the proliferation of synovium, bone erosion, and inflammatory cell infiltration in arthritic joints. Thus, we demonstrated that a cryptic epitope, the SLAYGLR sequence of murine
OPN
, is critically involved in the pathogenesis of a murine model of RA.
...
PMID:Essential role of the cryptic epitope SLAYGLR within osteopontin in a murine model of rheumatoid arthritis. 1286 2
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