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Blood, Vol. 95 No. 11 (June 1), 2000:
pp. 3380-3386
HEMOSTASIS, THROMBOSIS, AND VASCULAR BIOLOGY
From the Sol Sherry Thrombosis Research Center, Temple University
School of Medicine, Philadelphia, PA
The activity of phosphodiesterase (PDE)3A requires divalent cations.
Putative metal-binding sites are expected at 2 highly conserved
metal-binding motifs, HXXXH(X)25E. A functional truncated recombinant PDE3A containing the catalytic domain (PDE3A
An increase of intracellular cyclic adenosine
monophosphate (cAMP) produces potent inhibition of all platelet
functions.1 Cyclic guanosine monophosphate (cGMP)-inhibited
cAMP phosphodiesterase (PDE)3A, the most abundant cyclic nucleotide
phosphodiesterase in platelets,2 hydrolyzes cAMP, lowering
its intracellular concentration. Inhibitors function as potent
antiplatelet agents. Currently, the 2 oral antiplatelet agents with
proven efficacy are aspirin, which inhibits cyclooxygenase-dependent
synthesis of thromboxane A2 (TXA2), and
clopidogrel or ticlopidine, which blocks the ability of adenosine
diphosphate (ADP) to inhibit stimulated adenyl cyclase.3
Controlled trials show that both aspirin and ticlopidine are indicated
in the secondary prevention of stroke, myocardial infarction, and
peripheral vascular occlusion. However, standard antiplatelet drugs do
not alter the impairment of hemostasis seen in cardiopulmonary bypass,
and neither drug appears to prevent reocclusion of coronary arteries
after either thrombolytic therapy or angioplasty. The failure of
aspirin and ticlopidine in these situations largely results from their
inability to inhibit thrombin-induced platelet activation. Although, at
low concentrations of thrombin, platelet aggregation is dependent on
ADP and TXA2, high concentrations of thrombin aggregate and
activate platelets by independent pathways. In contrast, the elevation
of cAMP blocks all activating pathways in platelets The action of naturally occurring inhibitory prostaglandins The existence of distinct families of mammalian cyclic nucleotide PDEs,
which are expressed in a cell-specific manner, has encouraged the
further development of drugs that selectively inhibit specific
cAMP-PDEs. The mammalian PDEs are currently classified into 10 distinct families based on a combination of amino acid sequence
homology and a variety of biochemical properties, including substrate
specificity, response to selective inhibitors, mode of regulation, and
kinetic properties.12 The sequencing of the cDNA from at
least 1 member of each PDE family suggests that the 10 families are
coded for by related but distinct genes. They share a
conserved region of approximately 250 amino acids at the C-terminal end that contains the catalytic domain, which is
enzymatically competent by itself13-15; however,
the extent of homology is only 28% to 40%.16 In contrast,
the N-terminal region of each class is distinct and, in certain cases,
appears to contain the regulatory domain(s).
Native PDE3A purified from human erythroleukemia (HEL) cells in the
presence of chymostatin has a molecular mass of 110 kd17 and hydrolyzes cAMP with a Km of 0.5 µmol/L. The enzyme
is competitively inhibited by cGMP (Ki = 0.06 µmol/L).
When the enzyme is purified in the absence of an inhibitor, the
molecular mass is 61 kd with identical kinetic constants. PDE3A
purified from outdated platelets is a 61-kd catalytically active
hydrolase.18 We cloned HEL cell PDE3A,19
obtained its cDNA sequence, which was identical to a cloned enzyme from
heart,20 and coded for an amino acid sequence obtained from
platelets. We expressed a deletion mutant, PDE3A To elucidate the amino acids important in the active site, we
showed that a pH profile of PDE3A yielded pKa values of 6.5 and 9.0, consistent with histidine and cysteine.21 We then
performed group-specific modification on histidines with diethyl
pyrocarbonate and cysteines with N-ethylmaleimide and
5,5'-dithiobis-(2-nitrobenzoic acid). From difference spectra and
protection studies, 2 histidines were responsible for hydrolysis of
cAMP. However, if cGMP was used to protect against modification, 2 different histidines were protected because the combination of cGMP and
cAMP protected 4 histidine residues.21 A single
cysteine was required for cAMP hydrolysis, but none was needed
for cGMP binding. This study allowed us to formulate the
hypothesis that cAMP and cGMP binding sites are overlapping but not identical.
PDE3A activity is dependent on the presence of a divalent cation,
Mn++ > Mg++ > Co++.
Zn++ is the most potent cation but is
inhibitory.22 The sequence of the enzyme displayed 2 metal-binding motifs, HXXXH (X)25E, which are candidates
for coordinating Mn++, Co++, and
Mg++.23 These motifs are part of 26 perfectly
conserved amino acids in PDE3A, PDE2, PDE4A, and PDE5A.24
Twenty-three of these have been mutated in PDE5. We have previously
mutated 6 of the 26 conserved amino acids. The protein containing C816A
is poorly expressed. The mutation lies in a 44-amino acid insert unique
for PDE3. The protein containing H840A is well expressed, and the
mutation lies in the second metal-binding motif but displays no
catalytic activity. The enzyme containing H869A, outside the 2 motifs,
has kinetics consistent with defective binding for both cAMP and cGMP.
Mutation of amino acids C942A, C945A, and C1013A resulted in enzymes
indistinguishable from PDE3A We have now made 6 new mutations, 5 in the 2 metal-binding motifs, to
test whether these motifs bind divalent cations. The results of our
studies show that both histidines and the glutamate in the first motif
have exceedingly low activity, consistent with impairment of either
catalytic or metal binding. However, E866A has impaired binding for
both cAMP and cGMP. H836 had only decreased cGMP binding, and E971A had
decreased affinity only for cGMP. Neither mutant nor E825A showed loss
of metal-induced activity. We conclude that the second metal-binding
motif functions as a substrate binding region and that cAMP and cGMP
binding involve common and distinct amino acids.
Materials
Expression of a recombinant PDE3A in baculovirus/Sf9 cell system
Site-directed mutagenesis Site-directed mutagenesis of the recombinant PDE3A was performed with a QuikChange kit (Stratagene). Pairs of complementary oligonucleotide primers that contain desired mutants were synthesized as follows: (1) H752A, 5'-GGGATATTCCTTATGCTAACTGAATCCATGCC-3' and 5'-GGCATGGATTCTGTTAGCA-TAAGGAATATCCC-3'; (2) H756A, 5'-CATAACAGAATCGCTGCCACTGATCTTTTACAT-GC-3' and 5'-GCATGTAAAACATCAGTGGCAGCGATTCTGTTATG-3'; (3) E825A, 5'-GGAGTATCCCTGCCTTGGCGTTGATGGCGCTG-3' and 5'-CAGCGCCATCAACGCCAA-GGCAGGGATATTCC-3'; (4) H836, 5'-GGCTGCAGCCATGGCCGATTATGATCATCC-3' and 5'-GGATGATCATAATCATAATCGGCCATGGCTGCAGCC-3'; (5) E866A, 5'-CGATCGTTCAGTTTTGGCGAATCATCACGC-3' and 5'-GCGTGATGATTCGCCAAAACT-GAACGATCG-3'; (6) E971A, 5'-GGACAGATGGTATTGTCAATGCATTTTATGAACAGG-G-3' and 5'-CCCTGTTCATAAAATGCATTGACAATACCATCTGTCC-3'. pBlueBacHis 3031 plasmid DNA was used as a template of polymerase chain reaction (PCR) with plaque-forming unit DNA polymerase. The PCR products were treated with DpnI to digest the parent double-strand DNA chains. The mutated plasmid DNA was transformed in TOP 10 Escherichia coli competent cell (Invitrogen). The sequences of mutants were confirmed by automated DNA sequencing.Preparation of cell extract The Sf9 cells were harvested 96 hours after infection by centrifugation at 3000g for 15 minutes at 4°C, washed by PBS buffer, pH 7.4, and resuspended in a lysis buffer (50 mmol/L Tris-HCl, pH 7.8, 10 mmol/L MgCl2 with 0.5 µg/mL pepstatin, 0.5 µg/mL leupeptin, 2 µmol/L benzamidine, 10 µg/mL soybean trypsin inhibitor, and 50 µmol/L Tosyl phenylalanyl chloromethylketone) at 5 × 107 cells/mL. The cells were disrupted with a sonicator probe at 30-spare pulse for a total time of 2 minutes in ice. Crude cell extracts were centrifuged at 15 000g for 30 minutes at 4°C. The supernatant was either stored at 80°C or further purified.
Purification of the recombinant PDE3A protein and mutant proteins ProBond nickel-chelating resin (Invitrogen) was used for the protein purification; 1 mL resin was added to 2 mL supernatant in a total volume of 8 mL with a binding buffer (50 mmol/L Tris-HCl, pH 8.0, 0.5 mol/L NaCl, and 25 mmol/L imidazole) and rotated for 20 minutes. The resin was washed 3 times with the same binding buffer and packed in a 10-mL column. The purified protein was eluted by the eluted buffer (50 mmol/L Tris-HCl, pH 7.0, 0.5 mol/L NaCl, and 250 mmol/L imidazole), and aliquots were collected at 0.5 mL of each. The purified proteins were further dialyzed against 50 mmol/L Tris-HCl, pH 7.8, 10 mmol/L MgCl2, and 20% glycerol. All procedures were performed at 4°C.Phosphodiesterase activity assay Enzymatic activity was measured as described previously.18 Briefly, 100 µL total reaction volume containing 50 mmol/L Tris-HCl, pH 7.8, 10 mmol/L MgCl, and 1 µmol/L 3H-cAMP (40 000 cpm/assay) was incubated at 24°C for 30 minutes. Reactions were stopped by the addition of 0.2 mL of 0.2 mol/L ZnSO4 and 0.2 mL of 0.2 mol/L Ba(OH)2. Samples were mixed and centrifuged at 10 000g for 3 minutes. Radioactivity in the supernatants was determined by liquid scintillation. Vmax and Km for cAMP were determined by the Lineweaver-Burk plot with various concentrations of cAMP from 0.04 µmol/L to 20 µmol/L by Microsoft Excel program. For studies of enzyme activity inhibition by related inhibitor, compounds were present in the reaction mixture at concentrations that covered 4 orders of magnitude. Reactions were conducted at 24°C for 30 minutes and terminated by the addition of ZnSO4. Enzymatic assays were conducted in the linear range of the reaction, where less than 30% of the initial substrate cAMP was hydrolyzed. For mutants with low intrinsic activity, the amount of protein was increased until the total activity was comparable to the wild type. All assays were repeated 3 times, each on an independent transfection. Data are expressed as mean ± SD. Percentage expression of each recombinant protein was calculated by the following formula:
Western blot analysis Expressed cell lysates or purified recombinant protein and mutant proteins were separated on SDS-polyacrylamide gel electrophoresis using 10% polyacrylamide gels purchased from Fisher Scientific (Houston, TX). Proteins were transferred electrophoretically to nitrocellulose membrane (Bio-Rad, Hercules, CA). The membrane was blocked with 5% nonfat dry milk and 0.05% Tween 20 and incubated for 1.5 hours at room temperature with rabbit antiplatelet PDE3A polyclonal antibody (1:1000 dilution).19 Immunoreactivity was detected with horseradish-conjugated antirabbit IgG. Bands were visualized with substrate system (Bio-Rad) according to the manufacturer's protocol.Effects of divalent metal cations on the purified recombinant PDE3A and mutant proteins Metal-free water and metal-free buffer were made by the method previously described.22 Recombinant and mutant PDE3A were purified by the same method as above except in the metal-free buffer. Purified proteins were dialyzed in metal-free 50 mmol/L Tris-HCl buffer. Enzyme activity in metal-free buffer was assayed as a baseline, and the activity was measured in the presence of 10 µm to 1 mmol/L Mn2+, Mg2+, and Co2+ in chloride salt form. The value taken as 100% activity is the activity of purified recombinant PDE3A before dialysis.Protein concentration determination Protein concentrations in cell lysates and purified proteins were determined by bicinchonic acid (BCA) protein assay reagent (Pierce, Rockford, IL), and bovine serum albumin was used as a standard.
PDE3A
A limiting factor in the study of platelet PDE3A has been the
quantity available. Conventional purification from outdated platelets
requires starting material of 200 U outdated platelets derived from 100 L human blood. After purification of 2500-fold with a yield of
approximately 20%, 100 to 200 µg enzyme is
recovered.18,21 Overexpression of PDE3A in bacteria results
in poor growth of the cells, presumably because of the effects of
increased cAMP. Expression in yeast (S. cerevisiae) strain
GL62, deficient in yeast PDE1 and PDE2, still required a
purification of approximately500-fold with a yield of approximately
10%. The insect cell system first used for human myocardial
PDE3A25 offers many advantages. With the use of a
hexahistidine-containing construct, the purification of the recombinant
enzyme on a Ni column is simple. A 1-step procedure results in a
75-fold purification, with a yield of almost 50% of an
enzyme 90% to 95% homogeneous on SDS gel. The truncated recombinant
enzyme PDE3A
We thank Rita Stewart for skillful article preparation.
Submitted August 23, 1999; accepted January 5, 2000.
Supported in part by grants from the National Heart, Lung, and Blood
Institute (NHLB I) (nos. P01-HL64943 and T32-HL07777).
Reprints: Robert W. Colman, Sol Sherry Thrombosis Research
Center, Temple University School of Medicine, 3400 North Broad St,
Philadelphia, PA 19140; e-mail: colmanr{at}astro.temple.edu.
The publication costs of this
article were defrayed in part by
page charge payment. Therefore,
and solely to indicate this fact,
this article is hereby marked
"advertisement"
in accordance with 18 U.S.C.
section 1734.
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Top
Abstract
Introduction
1) and mutant proteins were expressed in a baculovirus/Sf9 cell system. All
the mutant proteins had decreased catalytic efficiency
(kcat/Km). Mutants H752A, H756A, and E825A had
kcat of less than 0.0008 s
1 to 0.0475 s
among them
increases in intracellular Ca++, shape change, aggregation,
secretion, and the effects of phospholipases A2 and C
1, coding for amino
acids 679 to 1141 in yeast with similar kinetics to the full-length
molecule and a specific activity of 844 nmol cAMP hydrolyzed per minute
per milligram protein. Further deletions led to a complete loss of
activity.
1, 40 times higher than H752A or H756A.
The decrease in specific activity is entirely attributable to a fall in
kcat because Km is unchanged from the truncated
recombinant enzyme. This decrease is therefore not caused by a change
in cAMP binding. There is, however, a modest elevation (5-fold) in the binding site for cGMP as reflected by an increase in Ki.
This change is specific because another inhibitor, milrinone, is not affected. Turko et al
