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Query: EC:3.1.4.1 (
phosphodiesterase
)
18,767
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
Autotaxin
(
ATX
), an exo-nucleotide pyrophosphatase and
phosphodiesterase
, was originally isolated as a potent stimulator of tumor cell motility. In order to study whether
ATX
expression affects motility-dependent processes such as invasion and metastasis, we stably transfected full-length
ATX
cDNA into two non-expressing cell lines, parental and ras-transformed NIH3T3 (clone7) cells. The effect of
ATX
secretion on in vitro cell motility was variable. The ras-transformed,
ATX
-secreting subclones had enhanced motility to
ATX
as chemoattractant, but there was little difference in the motility responses of NIH3T3 cells transfected with atx, an inactive mutant gene, or empty vector. In MatrigelTM invasion assays, all subclones, which secreted enzymatically active
ATX
, demonstrated greater spontaneous and
ATX
-stimulated invasion than appropriate controls. This difference in invasiveness was not caused by differences in gelatinase production, which was constant within each group of transfectants. In vivo studies with athymic nude mice demonstrated that injection of atx-transfected NIH3T3 cells resulted in a weak tumorigenic capacity with few experimental metastases. Combination of
ATX
expression with ras transformation produced cells with greatly amplified tumorigenesis and metastatic potential compared to ras-transformed controls. Thus,
ATX
appears to augment cellular characteristics necessary for tumor aggressiveness.
...
PMID:Autotaxin (ATX), a potent tumor motogen, augments invasive and metastatic potential of ras-transformed cells. 1064 2
Autotaxin
(
ATX
) is a 125-kD ectonucleotide pyrophosphate/
phosphodiesterase
, which was initially isolated and cloned from human melanoma cells as a potent stimulator of tumour cell motility.
ATX
shows 44% identity to the plasma cell membrane marker PC-1. Recently, we described the decreased expression of
ATX
mRNA in cultured fibroblast-like synoviocytes (SFC) of patients with RA by interferon-gamma. In this study using a competitive reverse transcriptase-polymerase chain reaction, we show an increased
ATX
mRNA expression in SFC from patients with RA in comparison with synoviocytes from non-RA patients. The median
ATX
mRNA amount in SFC of RA patients (440 pg/microg total RNA) was five-fold higher than the expression in synoviocytes from non-RA patients (80 pg/microg total RNA) or foreskin fibroblasts (MRHF cells, 90 pg/microg total RNA). In contrast to the elevated
ATX
mRNA expression in SFC of patients with RA, we did not measure increased mRNA amounts of PC-1 in these cells. Both the
ATX
mRNA amount and the
5'-nucleotide phosphodiesterase
(
PDE
) activity of SFC lysate were reduced after treatment of SFC with the cytokines IL-1beta or IL-4. IL-1beta and IL-4 induced a down-regulation of PC-1 mRNA and protein expression in SFC. In SFC treated with transforming growth factor-beta the expression of PC-1 mRNA and protein was increased, whereas no significant effect on
ATX
mRNA expression was detectable. Pharmacological drugs used in therapy for RA, such as dexamethasone, cyclosporin, methotrexate and indomethacin, did not show a statistically significant effect on either
ATX
mRNA or PC-1 mRNA expression. Only pentoxifylline suppressed
ATX
mRNA as well as PC-1 mRNA expression. In conclusion, we show a tight regulation of
ATX
and PC-1 gene expression by cytokines detectable in the inflamed tissue of RA. Further investigations will deal with the regulation of
ATX
protein expression as well as with the function of
ATX
in RA.
...
PMID:IL-1 beta- and IL-4-induced down-regulation of autotaxin mRNA and PC-1 in fibroblast-like synoviocytes of patients with rheumatoid arthritis (RA). 1116 12
Autotaxin
(
ATX
) is a recently described member of the nucleotide pyrophosphatase/
phosphodiesterase
(NPP) family of proteins with potent tumor cell motility-stimulating activity. Like other NPPs,
ATX
is a glycoprotein with peptide sequences homologous to the catalytic site of bovine intestinal
alkaline phosphodiesterase
(
PDE
) and the loop region of an EF-hand motif. The
PDE
active site of
ATX
has been associated with the motility-stimulating activity of
ATX
. In this study, we examined the roles of the EF-hand loop region and of divalent cations on the enzymatic activities of
ATX
. Ca(2+) or Mg(2+) was each demonstrated to increase the
PDE
activity of
ATX
in a concentration-dependent manner, whereas incubation of
ATX
with chelating agents abolished this activity, indicating a requirement for divalent cations. Non-linear regression analysis of enzyme kinetic data indicated that addition of these divalent cations increases reaction velocity predominantly through an effect on V(max.) Three mutant proteins, Ala(740)-, Ala(742)-, and Ala(751)-
ATX
, in the EF-hand loop region of
ATX
had enzymatic activity comparable to that of the wild-type protein. A deletion mutation of the entire loop region resulted in slightly reduced
PDE
activity but normal motility-stimulating activity. However, the
PDE
activity of this same deletion mutant remained sensitive to augmentation by cations, strongly implying that cations exert their effect by interactions outside of the EF-hand loop region.
...
PMID:Enzymatic activation of autotaxin by divalent cations without EF-hand loop region involvement. 1138 81
Autotaxin
[ATX (NPP-2)], originally isolated as a tumor motility-stimulating protein, has recently been shown to augment tumor aggressiveness. Specifically, atx-transfected, ras-transformed NIH3T3 cell lines have been shown to be more invasive, tumorigenic, and metastatic than mock-transfected ras-transformed control cells. In addition, the atx-transfected ras-transformed cell lines appeared to produce tumors that were much more hyperemic than those formed by appropriate control cells. This observation led to the present study, in which we demonstrate that ATX modulates angiogenesis both directly and indirectly. We have used a murine in vivo angiogenesis model in which treated Matrigel plugs are injected s.c. into athymic nude BALB/c mice. Using the same transfected cell lines as before, we found that mixing atx-transfected ras-transformed NIH3T3 cells into the Matrigel resulted in greater new blood vessel formation than control cells. Similarly, mixing purified ATX into the Matrigel resulted in new blood vessel formation within the plug, similar to that produced by vascular endothelial growth factor. Mechanistically, ATX is not a strong chemoattractant for human endothelial cells (HUVECs); however, it strongly stimulates motility in human coronary artery smooth muscle cells. In addition, ATX stimulates HUVECs grown on Matrigel to form tubules, much like vascular endothelial growth factor. Both of these normal cell types are shown to express and secrete ATX. In HUVECs, ATX expression is up-regulated by basic fibroblast growth factor in a time-dependent manner. This up-regulation also extends to secretion of enzymatically active protein, as demonstrated by Western blot analysis and quantification of type-1
phosphodiesterase
activity. These results establish the presence of ATX in HUVECs and coronary artery smooth muscle cells and specify ATX as a novel angiogenic factor, suggesting that ATX could contribute to the metastatic cascade through multiple mechanisms, perhaps by supporting an invasive microenvironment for both normal and tumor cells.
...
PMID:Autotaxin (NPP-2), a metastasis-enhancing motogen, is an angiogenic factor. 1155 73
Cofactor-independent phosphoglycerate mutase (iPGM) has been previously identified as a member of the alkaline phosphatase (AlkP) superfamily of enzymes, based on the conservation of the predicted metal-binding residues. Structural alignment of iPGM with AlkP and cerebroside sulfatase confirmed that all these enzymes have a common core structure and revealed similarly located conserved Ser (in iPGM and AlkP) or Cys (in sulfatases) residues in their active sites. In AlkP, this Ser residue is phosphorylated during catalysis, whereas in sulfatases the active site Cys residues are modified to formylglycine and sulfatated. Similarly located Thr residue forms a phosphoenzyme intermediate in one more enzyme of the AlkP superfamily,
alkaline phosphodiesterase
/nucleotide pyrophosphatase PC-1 (
autotaxin
). Using structure-based sequence alignment, we identified homologous Ser, Thr, or Cys residues in other enzymes of the AlkP superfamily, such as phosphopentomutase, phosphoglycerol transferase, phosphonoacetate hydrolase, and GPI-anchoring enzymes (glycosylphosphatidylinositol phosphoethanolamine transferases) MCD4, GPI7, and GPI13. We predict that catalytical cycles of all the enzymes of AlkP superfamily include phosphoenzyme (or sulfoenzyme) intermediates.
...
PMID:Conserved core structure and active site residues in alkaline phosphatase superfamily enzymes. 1174 79
Autotaxin
(
ATX
), an exo-nucleotide pyrophosphatase and
phosphodiesterase
, stimulates tumor cell motility at sub-nanomolar levels and augments invasiveness and angiogenesis. We investigated the role of G protein-coupled phosphoinositide 3-kinase gamma (PI3Kgamma) in
ATX
-mediated tumor cell motility stimulation. Pretreatment of human melanoma cell line A2058 with wortmannin or LY294002 inhibited
ATX
-induced motility.
ATX
increased the PI3K activity in p110gamma, but not p85, immunoprecipitates. This effect was abrogated by PI3K inhibitors or inhibited by pertussis toxin. Furthermore, stimulation of tumor cell motility by
ATX
was inhibited by catalytically inactive form of PI3Kgamma, strongly indicating the crucial role of PI3Kgamma for
ATX
-mediated motility in human melanoma cells
...
PMID:Autotaxin promotes motility via G protein-coupled phosphoinositide 3-kinase gamma in human melanoma cells. 1194 9
Autotaxin
(
ATX
) is a tumor cell motility-stimulating factor, originally isolated from melanoma cell supernatants.
ATX
had been proposed to mediate its effects through 5'-nucleotide pyrophosphatase and
phosphodiesterase
activities. However, the
ATX
substrate mediating the increase in cellular motility remains to be identified. Here, we demonstrated that lysophospholipase D (lysoPLD) purified from fetal bovine serum, which catalyzes the production of the bioactive phospholipid mediator, lysophosphatidic acid (LPA), from lysophosphatidylcholine (LPC), is identical to
ATX
. The Km value of
ATX
for LPC was 25-fold lower than that for the synthetic nucleoside substrate, p-nitrophenyl-tri-monophosphate. LPA mediates multiple biological functions including cytoskeletal reorganization, chemotaxis, and cell growth through activation of specific G protein-coupled receptors. Recombinant
ATX
, particularly in the presence of LPC, dramatically increased chemotaxis and proliferation of multiple different cell lines. Moreover, we demonstrate that several cancer cell lines release significant amounts of LPC, a substrate for
ATX
, into the culture medium. The demonstration that
ATX
and lysoPLD are identical suggests that autocrine or paracrine production of LPA contributes to tumor cell motility, survival, and proliferation. It also provides potential novel targets for therapy of pathophysiological states including cancer.
...
PMID:Autotaxin has lysophospholipase D activity leading to tumor cell growth and motility by lysophosphatidic acid production. 1213 81
We purified human
plasma lysophospholipase D
that produces physiologically active lysophosphatidic acid and showed that it is a soluble form of
autotaxin
, an ecto-nucleotide pyrophosphatase/
phosphodiesterase
, originally found as a tumor cell motility-stimulating factor. Its lower K(m) value for a lysophosphatidylcholine than that for a synthetic substrate of nucleotide suggests that lysophosphatidylcholine is a more likely physiological substrate for
autotaxin
and that its predicted physiological and pathophysiological functions could be mediated by its activity to produce lysophosphate acid, an intercellular mediator. Recombinant
autotaxin
was found to have lysophospholipase D activity; its substrate specificity and metal ion requirement were the same as those of the purified plasma enzyme. The activity of lysophospholipase D for exogenous lysophosphatidylcholine in human serum was found to increase in normal pregnant women at the third trimester of pregnancy and to a higher extent in patients in threatened preterm delivery, suggesting its roles in induction of parturition.
...
PMID:Identification of human plasma lysophospholipase D, a lysophosphatidic acid-producing enzyme, as autotaxin, a multifunctional phosphodiesterase. 1217 93
Autotaxin
(NPP2) is a tumor cell motility-stimulating factor that displays both a nucleotide pyrophosphatase/
phosphodiesterase
activity and a recently described lysophospholipase D activity. The hydrolysis of nucleotides is a metal-assisted reaction that occurs via a nucleotidylated threonine in the catalytic site. We show here that the catalytic site threonine and the metal-coordinating residues are also essential for the hydrolysis of lysophospholipids. In comparing the substrate specificity of NPP2 and the closely related NPP1 and NPP3, we found that only NPP2 displayed a lysophospholipase D activity, whereas NPP1 and NPP3 had a much higher nucleotide pyrophosphatase activity.
...
PMID:The hydrolysis of lysophospholipids and nucleotides by autotaxin (NPP2) involves a single catalytic site. 1263 53
Our group has recently demonstrated (Gesta, S., Simon, M., Rey, A., Sibrac, D., Girard, A., Lafontan, M., Valet, P., and Saulnier-Blache, J. S. (2002) J. Lipid Res. 43, 904-910) the presence, in adipocyte conditioned-medium, of a soluble lysophospholipase d-activity (LPLDact) involved in synthesis of the bioactive phospholipid lysophosphatidic acid (LPA). In the present report, LPLDact was purified from 3T3F442A adipocyte-conditioned medium and identified as the type II ecto-nucleotide pyrophosphatase
phosphodiesterase
,
autotaxin
(
ATX
). A unique
ATX
cDNA was cloned from 3T3F442A adipocytes, and its recombinant expression in COS-7 cells led to extracellular release of LPLDact.
ATX
mRNA expression was highly up-regulated during adipocyte differentiation of 3T3F442A-preadipocytes. This up-regulation was paralleled by the ability of newly differentiated adipocytes to release LPLDact and LPA. Differentiation-dependent up-regulation of
ATX
expression was also observed in a primary culture of mouse preadipocytes. Treatment of 3T3F442A-preadipocytes with concentrated conditioned medium from
ATX
-expressing COS-7 cells led to an increase in cell number as compared with concentrated conditioned medium from
ATX
non-expressing COS-7 cells. The specific effect of
ATX
on preadipocyte proliferation was completely suppressed by co-treatment with a LPA-hydrolyzing phospholipase, phospholipase B. Finally,
ATX
expression was found in mature adipocytes isolated from mouse adipose tissue and was substantially increased in genetically obese-diabetic db/db mice when compared with their lean siblings. In conclusion, the present work shows that
ATX
is responsible for the LPLDact released by adipocytes and exerts a paracrine control on preadipocyte growth via an LPA-dependent mechanism. Up-regulations of
ATX
expression with adipocyte differentiation and genetic obesity suggest a possible involvement of this released protein in the development of adipose tissue and obesity-associated pathologies.
...
PMID:Autotaxin is released from adipocytes, catalyzes lysophosphatidic acid synthesis, and activates preadipocyte proliferation. Up-regulated expression with adipocyte differentiation and obesity. 1264 76
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