Gene/Protein
Disease
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Drug
Enzyme
Compound
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Enzyme
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Query: EC:3.6.1.3 (
ATPase
)
65,361
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
Diabetic retinopathy is one of the leading causes of vision loss in industrialized countries. Despite recent advances, the biochemical basis for the development of this diabetic complication is uncertain. Although retinal circulation is unique in that it is readily observable noninvasively, retinal tissue is extremely difficult to study in humans because of the problems inherent in obtaining fresh, appropriate biopsy material. Moreover, because of the difficulties in working with animal models of diabetic retinopathy, such as the dog, many investigators have turned to cell-culture models, especially those using primary cultures of retinal capillary endothelial cells and pericytes. Diabetic retinopathy involves both morphological and functional changes in the retinal capillaries. Morphological changes include basement membrane thickening and pericyte disappearance; functional changes include one important early change--increased permeability--which may be attributable to endothelial cell changes and basement membrane leakiness. Investigators have described major biochemical changes in cellular signaling pathways, including myo-inositol, inositol phosphates, and DAG metabolism, as well as decreased Na(+)-K(+)-
ATPase
and increased
PKC
activity. These defects may be related to the way endothelial cells and pericytes synthesize and interact with the extracellular matrix. Abnormalities in endothelial cell or pericyte interaction with the basement membrane may in turn lead to functional abnormalities, such as increased permeability.
...
PMID:Current hypotheses for the biochemical basis of diabetic retinopathy. 146 44
Recently, one of the authors (K.I.) and other investigators reported that myosin light chain (MLC) of smooth muscle (gizzard, arterial and tracheal) was diphosphorylated by myosin light chain kinase (MLCK) and that diphosphorylated myosin showed a marked increase in the actin-activated myosin ATPase activity in vitro and ex vivo. In this study, we prepared myosin, actin, tropomyosin (human platelet), MLCK (chicken gizzard) and calmodulin (bovine brain) and demonstrated diphosphorylation of MLC of platelet by MLCK in vitro. Our results are as follows. (1) Platelet MLC was diphosphorylated by a relatively high concentration (greater than 20 micrograms/ml) of MLCK in vitro. As a result of diphosphorylation, the actin-activated myosin ATPase activity was increased 3 to 4-fold as compared to the monophosphorylation. (2) Both di- and monophosphorylation reactions showed similar Ca2+, KCl, MgCl2-dependence. Maximal reaction was seen at [Ca2+] greater than 10(-6) M, 60 mM KCl and 2 mM MgCl2. This condition was physiological in activated platelets. (3) Di- and monophosphorylated myosin showed similar Ca2+, KCl-dependence of
ATPase
activity but distinct MgCl2-dependence. Diphosphorylated myosin showed maximal
ATPase
activity at 2 mM MgCl2 and monophosphorylated myosin showed a maximum at 10 mM MgCl2. (4) The addition of tropomyosin stimulated actin-activated
ATPase
activity in both di- and monophosphorylated myosin to the same degree. (5) ML-9, a relatively specific inhibitor of MLCK, inhibited the aggregation of human platelets induced by thrombin ex vivo in a dose-dependent manner. Moreover, this drug also partially inhibited both di- and monophosphorylation reactions and actin-activated
ATPase
activity. On the other hand, H-7, a synthetic inhibitor of
protein kinase C
, had little effect on the aggregation of human platelets induced by thrombin ex vivo. From these results, we conclude that diphosphorylation of platelet myosin by MLCK may play an important role in activated platelets in vivo.
...
PMID:Diphosphorylation of platelet myosin by myosin light chain kinase. 153 1
The role of
protein kinase C
(
PKC
) in regulating the contractile state of smooth muscle was investigated using the constitutively active catalytic fragment of
PKC
(PKM) with skinned (demembranated) chicken gizzard fibres. PKM attenuated a submaximal contraction in gizzard smooth muscle skinned fibres, but not in rabbit cardiac skinned fibres. PKM-mediated relaxation of submaximal contractions of smooth muscle was accompanied by a reduction in the rate of ATP hydrolysis in the fibre and by phosphorylation of the 20 kDa light chain of gizzard myosin at the
PKC
sites (serine-1, serine-2 and threonine-9). In addition, several other endogenous proteins were phosphorylated by PKM. However, the inhibitory effects on tension and
ATPase
are consistent with the biochemical effects of
PKC
-catalysed phosphorylation of myosin, i.e. reduction of the actin-activated MgATPase activity of myosin prephosphorylated at serine-19 by myosin light chain kinase. Pretreatment of skinned fibres with PKM and ATP gamma S in the absence of Ca2+ had no inhibitory effect on the subsequent submaximal Ca(2+)-activation of force. Consistent with this observation,
PKC
was not able to utilize ATP gamma S as a substrate, confirming that the observed effects were the result of PKM-catalysed protein phosphorylation. We suggest that
PKC
may have two distinct effects on smooth muscle contraction: translocation of
PKC
to the sarcolemma on stimulation results in phosphorylation of a protein(s) other than myosin and a slow, sustained contraction; in some circumstances
PKC
may undergo proteolysis to PKM resulting in myosin phosphorylation at
PKC
-specific sites, a reduction in
ATPase
activity and relaxation of the muscle.
...
PMID:Effects of the constitutively active proteolytic fragment of protein kinase C on the contractile properties of demembranated smooth muscle fibres. 153 85
We recently reported that autophosphorylated
protein kinase C
(
PKC
) has an intrinsic Ca(2+)- and phospholipid-dependent
ATPase
activity and that the
ATPase
and histone kinase activities of
PKC
have similar metal-ion cofactor requirements and Km,app(ATP) values. We hypothesized that the intrinsic
ATPase
activity of
PKC
may represent the bond-breaking step of its protein kinase activity. The rate of the
ATPase
reaction is several times slower than the histone kinase reaction rate. At subsaturating concentrations, various peptide and protein substrates stimulate the
ATPase
reaction by as much as 1.5-fold. In contrast, non-phosphorylatable substrate analogs are not stimulatory. These observations support a mechanism of
PKC
catalysis in which the productive binding of phosphoacceptor substrates enhances the rate of phosphodonor substrate (ATP) hydrolysis at the active site of
PKC
. However, this mechanism contains an assumption that the
ATPase
activity of
PKC
is catalyzed at the active site. In fact, sequence analysis indicates that
PKC
contains a potential second nucleotide binding site outside of its active site. In this report, we provide a detailed analysis of the relationship between the active site of
PKC
and the intrinsic
ATPase
activity of the enzyme. We show that the regulatory and catalytic properties of the
ATPase
reactions of three
PKC
isozymes are similar, despite critical differences among the isozymes in their consensus sequences for the potential non-active-site nucleotide binding site in their catalytic domains. We also show that the
ATPase
and histone kinase reactions of each isozyme have similar Km,app(ATP) values.(ABSTRACT TRUNCATED AT 250 WORDS)
...
PMID:The intrinsic ATPase activity of protein kinase C is catalyzed at the active site of the enzyme. 153 19
The role of
protein kinase C
(
PKC
) in the regulation of phosphatidylcholine-hydrolyzing phospholipase D (PLD) was investigated. In membranes from Chinese hamster lung fibroblasts that had been incubated with [14C]choline to label endogenous phosphatidylcholine, phorbol 12-myristate 13-acetate (PMA) failed to stimulate production of [14C]choline. However, stimulation was observed if fibroblast cytosolic fraction or
PKC
partially purified from this fraction was added. When incubated with membranes in the presence of PMA, pure
PKC
from rat brain stimulated [14C]choline production in a concentration-dependent manner, with a maximal 2-3-fold effect. PMA similarly stimulated [14C]phosphatidylpropanol formation from propanol using membranes from [14C]myristic acid-prelabeled cells, confirming the activation of PLD. None of the effects described required exogenous ATP. To probe the role of phosphorylation in the
PKC
effect, we included high concentrations of apyrase in the assay. This
ATPase
had no effect on the ability of
PKC
to activate PLD, but under exactly the same conditions, it eliminated autophosphorylation of
PKC
. The results provide conclusive evidence for the involvement of
PKC
in the activation of PLD and suggest that ATP-dependent phosphorylation is not required.
...
PMID:Activation of phospholipase D by protein kinase C. Evidence for a phosphorylation-independent mechanism. 155 64
Human platelets were loaded with the fluorescent Na(+)-sensitive dye sodium-binding benzofuran isophtalate (SBFI), and changes in the fluorescence excited at 345 and 385 nm were analyzed after manipulations that evoked predictable changes in the cytosolic Na+ concentration ([Na+]i). Raising [Na+]i by either gramicidin D or monensin specifically increased the fluorescence excited at 345 nm and decreased that excited at 385 nm. Hence, calculation of changes in the 345/385 nm excitation ratio yields an estimate of actual changes in [Na+]i. A transient activation of Na+/H+ exchange evoked by addition of acidified platelets to buffer, pH 7.4, evoked a transient rise in [Na+]i. The re-establishment of basal [Na+]i could be prevented by ouabain, indicating an involvement of the Na+,K(+)-
ATPase
. Upon stimulation by 0.5 unit/ml of thrombin, [Na+]i immediately increased by 16 +/- 4 mM and this rise continued for at least 60 min after addition of agonist, albeit at a lower rate. This latter sustained rise could not be curtailed by scavenging thrombin by means of hirudin. Addition of ouabain or the phorbol ester 12-O-tetradecanoylphorbol-13-acetate induced a comparable slow rise in the 345/385 excitation ratio. This may indicate a
protein kinase C
-mediated inhibition by thrombin of the Na+,K(+)-
ATPase
. In the absence of extracellular Ca2+ (Ca2+o), the [Na+]i gain was augmented to 38 +/- 9 mM. This additional uptake of Na+ was prevented by (i) Mn2+ ions, (ii) La3+ ions, (iii) the blocker of receptor-mediated Ca2+ entry (1-[beta[3-(4-methoxyphenyl)propoxyl]-4-methoxyphenethyl]-1H-im ida zole hydrochloride), and (iv) by hirudin which reversed receptor occupancy by thrombin. These findings suggest that the additional thrombin-induced [Na+]i gain in the absence of Ca2+o is due to Na+ influx through a Ca2+ entry pathway. The increase in [Na+]i in the presence of Ca2+o results from Na+ influx via Na+/H+ exchange.
...
PMID:Further characterization of the mechanisms mediating the rise in cytosolic free Na+ in thrombin-stimulated platelets. Evidence for inhibition of the Na+,K(+)-ATPase and for Na+ entry via a Ca2+ influx pathway. 164 80
This study examines the ontogeny of the regulation of Na+,K(+)-
ATPase
activity in the proximal tubule (PT) by a first messenger, dopamine (DA), and by direct stimulation of a third messenger,
protein kinase C
(
PKC
). PT segments dissected from 10- (PT10), 15-(PT15), 20- (PT20), and 40- (PT40) d-old rats were preincubated with DA 10(-5) M, diacylglycerol (DAG) 10(-5) M (an endogenous activator of
PKC
), or phorbol 12,13-dibutyrate (PDBu) 10(-6) M (an exogenous activator of
PKC
). DA inhibited Na+,K(+)-
ATPase
activity in PT40. In PT20, DA also inhibited Na+,K(+)-
ATPase
activity, but the inhibitory effect in PT20 was less pronounced than in PT40. In PT15, DA had no effect on Na+,K(+)-
ATPase
activity. DAG significantly inhibited Na+,K(+)-
ATPase
activity in PT40. DAG also inhibited Na+,K(+)-
ATPase
activity in PT20, but the inhibition was slightly less pronounced than in PT40. DAG had no effect on Na+,K(+)-
ATPase
activity in PT15. Na+,K(+)-
ATPase
activity in PT40 and PT20 preincubated with PDBu was significantly lower than with vehicle. The inhibitory effect in PT20 was less pronounced than in PT40. When PT40 and PT20 were preincubated with both PDBu and 5 x 10(-5) M sphingosine, an inhibitor of
PKC
activation, the inhibitory effect of PDBu was abolished. In both PT40 and PT20 incubated with 4-alpha-12,13 phorbol didecanoate 10(-7) M, a phorbol ester that will not activate
PKC
, Na+,K(+)-
ATPase
activity was not different from the control. In PT10, Na+,K(+)-
ATPase
activity was the same after PDBu incubation and after vehicle incubation.(ABSTRACT TRUNCATED AT 250 WORDS)
...
PMID:Ontogeny of the regulation of Na+,K(+)-ATPase activity in the renal proximal tubule cell. 165 42
The impaired Na(+)-K(+)-
ATPase
activity in peripheral nerve from diabetic rats is prevented by dietary myo-inositol (MI) supplementation in vivo and corrected by
protein kinase C
(
PKC
) agonists in vitro, suggesting that
PKC
may mediate the effects of nerve MI depletion on Na(+)-K(+)-
ATPase
activity. However, little is known about the effect of diabetes on
PKC
activity or peptide in rat peripheral nerve. Therefore, the effect of streptozocin-induced diabetes and dietary MI supplementation on the activity and distribution of
PKC
in rat sciatic nerve homogenates and cytosolic and particulate fractions was explored with histone phosphorylation assay and Western-blot analysis.
PKC
activity but not peptide was selectively decreased in the cytosolic fraction by streptozocin-induced diabetes, and this abnormality was partially corrected by dietary MI supplementation. These results suggest that altered MI metabolism may affect nerve
PKC
specific activity, and this alteration may play a role in reduced Na(+)-K(+)-
ATPase
activity and blunted regenerative response in diabetic nerve.
...
PMID:Diminished specific activity of cytosolic protein kinase C in sciatic nerve of streptozocin-induced diabetic rats and its correction by dietary myo-inositol. 165 70
Incubation of the murine macrophage tumour cell line PU5-1.8 in K+ (140 mM)-HEPES buffer induced depolarization of the membrane and the translocation of
protein kinase C
(
PKC
) to the subnuclear region. Membrane depolarization also induced an increase of intracellular free Ca2+ levels ([Ca2+]i) which was due to the Ca2+ influx. The amount of K(+)-mediated Ca2+ uptake was dependent on the Ca2+ concentration gradient as measured by indo-1 fluorescence and 45Ca2+ fluxes. The depolarization-mediated Ca2+ influx was suppressed by voltage sensitive Ca2+ channel blockers such as nifedipine and verapamil. Furthermore, in Na(+)-HEPES buffer, incubation of cells with a dihydropyridine agonist [3H]PN200-110 produced a dose-dependent saturable binding. On the other hand, short-term incubation of cells with phorbol 12-myristate 13-acetate (PMA) abolished the early phase of 45Ca2+ influx and the rise of indo-1 fluorescence. Depleting cells of
PKC
or incubating them with
PKC
inhibitors, H7 and sphingosine, enhanced the uptake of 45Ca2+ and the rise of indo-1 fluorescence. These observations suggest that membrane depolarization caused an activation of
PKC
and induced Ca2+ influx through the activation of dihydropyridine-sensitive, voltage-operated Ca2+ channels. Data also show that
PKC
may act as a negative modulator in controlling the Ca2+ response by closing the voltage-operated Ca2+ channel and/or by enhancing the Ca(2+)-
ATPase
activity during membrane depolarization in PU5-1.8 cells.
...
PMID:Membrane depolarization induces protein kinase C translocation and voltage operated calcium channel opening in PU5-1.8 cells. Protein kinase C as a negative feedback modulator for calcium signalling. 165 33
We have examined two distinct protein kinases, cAMP-dependent protein kinase and
protein kinase C
, for their ability to phosphorylate and regulate the activity of three different types of Na+,K(+)-
ATPase
preparation. cAMP-dependent protein kinase phosphorylated purified shark rectal gland Na+,K(+)-
ATPase
to a stoichiometry of approximately 1 mol of phosphate per mol of alpha subunit. Protein kinase C phosphorylated purified shark rectal gland Na+,K(+)-
ATPase
to a stoichiometry of approximately 2 mol of phosphate per mol of alpha subunit. The phosphorylation by each of the kinases was associated with an inhibition of Na+,K(+)-
ATPase
activity of about 40-50%. These two protein kinases also inhibited the activity of a partially purified preparation of Na+,K(+)-
ATPase
from rat renal cortex and the activity of Na+,K(+)-
ATPase
present in preparations of basolateral membrane vesicles from rat renal cortex.
...
PMID:Phosphorylation of the catalytic subunit of Na+,K(+)-ATPase inhibits the activity of the enzyme. 166 94
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