| HOME | HELP | FEEDBACK | SUBSCRIPTIONS | ARCHIVE | SEARCH | TABLE OF CONTENTS |
|
|
|
|||||||
|
|||||||||
J Biol Chem, Vol. 275, Issue 7, 4555-4560, February 18, 2000
From the Fhit, a member of the histidine triad superfamily
of nucleotide-binding proteins, binds and cleaves diadenosine
polyphosphates and functions as a tumor suppressor in human epithelial
cancers. Function of Fhit in tumor suppression does not require
diadenosine polyphosphate cleavage but correlates with the ability to
form substrate complexes. As diadenosine polyphosphates are at lower cellular concentrations than mononucleotides, we sought to quantify interactions between Fhit and competitive inhibitors with the use of
diadenosine polyphosphate analogs containing fluorophores in place of
one nucleoside.
Appp-S-(7-diethylamino-4-methyl-3-(4-succinimidylphenyl)) coumarin (ApppAMC),
Appp-S-(4-4-difluoro-5,7-dimethyl-4-bora-3a,4a-diaza-s-indacine-3-yl) methylaminoacetyl (ApppBODIPY), and GpppBODIPY, synthesized in high yield, are effective Fhit substrates, producing AMP or GMP plus
fluorophore diphosphates. GpppBODIPY cleavage is accompanied by a
5.4-fold increase in fluorescence because BODIPY fluorescence is
quenched by stacking with guanine. Titration of unlabeled diadenosine polyphosphates, inorganic pyrophosphate, mononucleotides, and inorganic
phosphate into fluorescent assays provided values of Km and KI as competitive
inhibitors. The data indicate that Fhit discriminates between good
substrates via kcat and against cellular
competitors in equilibrium binding terms. Surprisingly, pyrophosphate
competes better than purine mononucleotides.
Encoded at 3p14.2 (1), the most fragile site in the human genome
(2), Fhit is a dimeric protein of 147 amino acids with diadenosine
triphosphate (ApppA)1
hydrolase activity (3). Because of the fragility of the FHIT chromosomal location, allele loss at FHIT, the earliest and
most frequent known event in lung carcinogenesis (4, 5), could have
been considered either a cause or a consequence of cancer. Suppression
of tumor formation by reexpression of Fhit protein in kidney, gastric,
and lung cancer cell lines with FHIT deletions demonstrated
that Fhit is an authentic tumor suppressor (6). In lung cancer
suppressor systems, suppression of tumorigenesis is accompanied by
induction of apoptosis (7, 8). In mice, FHIT inactivation
induces stomach and sebaceous tumors that resemble human Muir-Torre
syndrome.2
As anticipated from structural similarity between histidine triad (HIT)
protein dimers and galactose-1-phosphate uridylyltransferase (GalT)
(9), Fhit proceeds through a GalT-like (10), covalent His-96-adenylate
intermediate that is hydrolyzed with retention of configuration (11).
The His-96 To determine the structural consequences of ApnA
substrate binding, stable complexes of wild-type and mutant Fhit proteins bound to nonhydrolyzable ApppA analogs were prepared (16, 17).
Co-crystal structures indicated that the Fhit dimer binds two
ApnA molecules in a manner that fills a large, positively charged groove with substrate phosphates, potentially presenting an altered surface for protein-protein interactions to a
proapoptotic effector (12). Because this model of Fhit function depends
on forming complexes with inabundant substrates, and recognition (and
stabilization) of these complexes by a Fhit effector, it was important
to assay the more abundant cellular mononucleotides as competitive
inhibitors of Fhit. To a first approximation, the cellular abundance of
a Fhit-ApnA complex is expected to be a function
of the equilibrium binding constant of Fhit for that
ApnA, the binding constants of Fhit for
competing compounds, the abundance of Fhit and each compound, and the
lifetimes of these complexes, potentially as modulated by cellular proteins.
In the past, determination of the Km values for
competing substrates would have required assaying products from each substrate. Determination of KI values for
competitive inhibitors would have required measuring rates of
[3H]AMP and [3H]ADP formation from
[3H]ApppA as a function of each inhibitor (18). A
recently reported method of visualizing ApppA reaction products by
staining them with SYBR GREEN II is unsuitable for kinetic measurements
(19). Dietheno-ApppA has also been synthesized and shown to be a Fhit substrate with a 2 µM Km (20). Here,
we synthesized novel fluorescent analogs of ApppA by joining
thiol-reactive derivatives of 7-diethylamino-4-methylcoumarin (AMC) and
4,4-difluoro-5,7-dimethyl-4-bora-3a,4a-diaza-s-indacine-3-yl (BODIPY
FL) to ATP Having developed fluorescent and fluorogenic assays for the Fhit
active site, we titrated unlabeled competitive inhibitors into these
assay to determine the Km of Fhit for ApppA, AppppA,
ApppppA, ATP Synthesis of ApppAMC, ApppBODIPY, and GpppBODIPY--
ATP Fluorescent Thin Layer Enzyme Assays--
Fluorescent substrates
at 1-30 µM were incubated with purified Fhit protein
(16) in reactions at 37 °C containing 20 mM Na HEPES, pH
7.0, 0.5 mM MnCl2, and 0.2 mg/ml bovine serum
albumin. Competitive compounds, when indicated, were mixed with
fluorescent substrate at 8-10 concentrations, surrounding the
Km or KI values of the
competitor. Reaction samples ( Fluorogenic Enzyme Assays--
Reactions in black 96-well plates
containing GpppBODIPY at 1.25-40 µM in 60 µl of 20 mM Na HEPES, pH 7.0, 0.5 mM MnCl2,
and 0.2 mg/ml bovine serum albumin were initiated with addition of 167 fmol of Fhit and incubated for 300-360 s at 37 °C. Duplicate reactions were stopped by addition of 60 µl of 200 mM
sodium citrate, pH 3.0, and read with a Wallach Victor2
Multilabel Counter 1420 with a 485-nm excitation filer and a 535-nm
emission filter. At each substrate concentration, mock reactions were
created by mixing 0%, 5%, and 10% volumes of acid-stopped complete
hydrolysates with acid-stopped mock reactions (100%, 95%, and 90%).
Fluorescent emissions of experimental and mock reactions were counted
and plotted to calculate ppBODIPY production per active site per second
at each concentration of GpppBODIPY. To prove that ApppA,
pyrophosphate, and AMP are competitive inhibitors, these compounds were
titrated into 96-well GpppBODIPY assays at four concentrations at each
of five concentrations of GpppBODIPY (2, 4, 8, 16, and 32 µM). Initial rates as a function of GpppBODIPY and
inhibitor concentration were plotted by the method of Eadie and Hofstee
(24).
Design Criteria for Fluorescent Fhit Substrates--
HIT proteins
are a superfamily of homodimeric nucleotide-binding proteins with a
unique mode of nucleotide recognition (14). Each monomer contributes 5 strands to a 10-stranded anti-parallel Fluorescent ApppA Analogs Are Good Fhit Substrates--
At
substrate concentrations below Km, reactions proceed
with first-order kinetics such that the negative slope of a plot of
log[remaining substrate] against time equals
kcat/Km times the enzyme
concentration (24). To test whether Fhit would tolerate substitution of
one adenosine in a fluorescent ApppA analog, we incubated 0.5-2.5
nM Fhit with 1.5-5 µM ApppAMC and ApppBODIPY. Time courses of such reactions, analyzed by TLC and digitally imaged upon UV illumination, made it clear that Fhit cleaves
each substrate, generating one fluorescent product with reduced
chromatographic mobility (Fig. 2,
A and B). One thousand times more concentrated
substrates were required to visualize the nonfluorescent product by UV
shadowing on TLC plates with fluorescent indicator (12) and, as
expected, that product was indistinguishable from AMP (data not shown).
Thus, Fhit cleaves ApppAMC and ApppBODIPY to produce AMP + ppAMC and
AMP + ppBODIPY, respectively.
At an initial substrate concentration of 3 µM ApppAMC
([enzyme] = 2.5 nM) or 1.5 µM ApppBODIPY
([enzyme] = 1.2 nM), the first-order decay kinetics of
ApppAMC and ApppBODIPY were examined. As shown in Fig.
3 (A and B) and
Table I, calculated
kcat/Km values for each
substrate were 1.2 × 106 s The BODIPY Substitution Affects kcat--
ApppBODIPY
is an effective and useful substrate for Fhit with a quantitative
disadvantage in cleavage
(kcat/Km for ApppBODIPY = 2.3 × 106 s GpppBODIPY Is a Stacked and Quenched Fluorogenic
Substrate--
Cleavage of ApppG by Fhit yielded a two-thirds mixture
of AMP + GDP with a one-third mixture of GMP + ADP (3). Thus, the guanine in GpppBODIPY was expected to be an acceptable substitution for
adenine in ApppBODIPY. Upon synthesis, GpppBODIPY was found to have
only 11% of the fluorescence in aqueous solution of the parental dye.
Because guanine does not absorb photons in the visible range,
fluorescent resonance energy transfer was ruled out as the mechanism of
quenching. In methanol, the yield of GpppBODIPY fluorescence rose to
60% that of BODIPY fluorescence, suggesting that a solvent-sensitive
binding interaction between guanine and BODIPY is responsible for
quenching. The NMR signal in D2O for the guanine C-8 proton
was shifted from 8.2 ppm (GTP) to 7.9 ppm (GpppBODIPY), indicating that
guanine is bound in the electron-rich BODIPY environment. No proton NMR
shift or alteration of fluorescence was observed with ApppBODIPY. By
analogy to fluorescent uridine nucleotide analogs (21), we conclude
that GpppBODIPY is quenched by stacking.
The TLC assay of 2 µM GpppBODIPY ([enzyme] = 2.4 nM) in Figs. 2C and 3C shows that
GpppBODIPY is within 4-fold as good a substrate as ApppBODIPY
(kcat/Km = 5.8 × 105 s Nucleotides and Nucleotide Analogs as Competitive Inhibitors of
Fhit-ApppBODIPY and GpppBODIPY Kinetics--
The readout of
first-order ApppBODIPY assays,
kcat/Km times enzyme
concentration, is well suited for assays of competitive inhibitors.
Competitive inhibitors rob from the pool of available enzyme,
decreasing
kcat/Km (apparent).
The decrease in
kcat/Km
(apparent) is a function of the equilibrium binding constant and
the concentration of the competitor. When the competing ligand is not a
substrate, the equilibrium binding constant represents
KI. When the competing ligand is itself a Fhit
substrate, the equilibrium binding constant is Km, the apparent dissociation constant for all bound forms with enzyme.
As shown in Fig. 4 and summarized in
Table I, ApnA compounds, purine mononucleotides,
inorganic pyrophosphate, and monophosphate were titrated into
ApppBODIPY assays as competitive inhibitors. ApppA and AppppA displayed
the lowest Km values. The Km for
ApppA measured as a competing substrate was 2.0 ± 0.2 µM, consistent with the Km value
measured for ApppA by 3H product formation, 1.9 ± 0.2 µM (12). The additional phosphate group and two phosphate
groups in AppppA and ApppppA increased Km by 30%
and 600%, respectively. The next best competitor was inorganic
pyrophosphate with a KI of 19.9 ± 3.8 µM. ATP and GTP, probably the most abundant cellular
mononucleotides (26), were difficult to fit to Equation 1 (see
"Experimental Procedures"), potentially because of formation of
pyrophosphate. To estimate the Km values of ATP and
GTP, the slowly hydrolyzed
To prove that the compounds inhibit competitively, rather than by a
noncompetitive or uncompetitive mechanism, compounds were titrated into
fluorogenic GpppBODIPY initial-rate assays over a range of substrate
and inhibitor concentrations. As shown in Fig.
5, ApppA, pyrophosphate, and AMP all
increase the apparent Km of GpppBODIPY without
affecting the kcat value, displaying the
classical signature of competitive inhibitors in Eadie-Hofstee plots.
These experiments also demonstrated that, much as the BODIPY for
adenosine substitution was responsible for a 10-fold decrease in
kcat with minimal effect on
Km, the guanine for adenine substitution is
responsible for a 10-fold decrease in kcat with minimal effect on Km.
The new compounds described herein can be considered analogs
of ATP and GTP as well as ApnA and have
potential uses with a wide variety of enzymes including ATPases and
GTPases. The compounds have been used to purify and characterize
the Fhit active site of
NitFhit,3 the Fhit ortholog
in Caenorhabditis elegans that is fused to Nit (27), a
tetrameric protein that binds two Fhit dimers and confers a novel
protein-association activity to the complex.3
In addition to basic science applications, by combining the fluorogenic
Fhit substrate with newly developed Fhit-specific inhibitors (28), a
Fhit diagnostic kit can be developed for use in clinical laboratories.
The GpppBODIPY assay for Fhit, as a 96-well fluorogenic assay, is also
suitable for a high throughput screen for inhibitors. Among Fhit
inhibitors, uncompetitive compounds (those that bind and retard the
enzyme-substrate complex) might include compounds that are competitive
with a Fhit effector (12, 13).
The present study provides valuable information about properties of
substrates and related compounds that determine binding to Fhit.
Fhit-ApnA complexes may be required for
signaling (12), and formation of these complexes would have to occur in the face of competition with mononucleotides, monophosphate,
pyrophosphate, and other compounds. The finding that reversible binding
constants for ApnA, pyrophosphate, and purine
mononucleotides are 2 E The data presented herein illustrate a surprising degree of
kcat discrimination among chemically similar
substrates. Although the kinetics of Fhit-dependent
cleavage of ApppA are robust, the function of Fhit appears to depend
not on cleavage but binding ApnA substrates (5,
6, 12). We have argued that important Fhit substrates are those with
low Km values but not necessarily the highest
kcat values. Less optimal substrates, such as
AppppA, may be more important than ApppA if they are more abundant and
if their residence time on Fhit is longer than that of ApppA (12). In
the cell, the lifetime of Fhit-substrate complexes may be stabilized by
effector interactions. The observation that substrates with
fundamentally unaltered chemical lability such as ApppBODIPY and
GpppBODIPY are cleaved with reduced kcat
values suggests that Fhit has binding modes that are at least 100-fold stabilized with respect to optimized in vitro kinetics.
The stereochemical course of the Fhit reaction (11) dictates that ADP
(in case of ApppA), ATP (in case of AppppA), or ppBODIPY (in case of
fluorescent substrates) must leave before the hydrolytic water can be
bound by the enzyme. Thus, any Fhit or Fhit-effector conformation that
prevents leaving-group exit or blocks water entry would be expected to
retard substrate hydrolysis. The 20 µM
pyrophosphate-binding site that is competitive with substrate is a
likely facilitator of leaving group-reattack. A Fhit effector may
stabilize Fhit-ApnA by pinning the leaving group down on this site.
Many intracellular and extracellular receptors are enzymatically inert,
while others, such as GTPases, are slow enzymes with intrinsically
long-lived enzyme-substrate complexes. Fhit appears to be a receptor
for ApnA with rapid kinetics but with features
that allow it to be stabilized in vivo. The kinetics and
structural biology of Fhit-associated proteins (15, 27) are expected to
shed more light on this matter.
We thank Kay Huebner, Mike Blackburn, and
Perry Frey for helpful discussions, and Dieter Klaubert of Molecular
Probes for suggesting synthesis of GpppBODIPY. Synthesis was performed
at Molecular Probes.
*
This work was supported by National Institutes of Health NCI
Research Grant CA75954 (to C. B.), a National Institutes of Health NCI institutional training grant (to A. D.), and new investigator awards from the March of Dimes Birth Defects Foundation, the Burroughs Wellcome Fund, and the Arnold and Mabel Beckman Foundation (to C. B.).The costs of publication of this
article were defrayed in part by the
payment of page charges. The article
must therefore be hereby marked
"advertisement" in
accordance with 18 U.S.C. Section
1734 solely to indicate this fact.
§
Present address: Unilever Research, Edgewater, NJ 07020.
2
Fong, L. Y. Y., Fidanza, V., Zanesi, N., Lock,
L. F., Siracusa, L. D., Mancini, R., Siprashvili, Z., Ottey, M.,
Martin, S. E., Dolsky, R., Druck, T., McCue, P. A., Croce, C. M., and
Huebner, K. (2000) Proc. Natl. Acad. Sci. U. S. A. 97, in press.
3
H. C. Pace, S. C. Hodawadekar, A. Draganescu, J. Huang, P. Bieganowski, Y. Pekarsky, C. M. Croce, and C. Brenner, manuscript in preparation.
The abbreviations used are:
ApppA, diadenosine
triphosphate;
HIT, histidine triad;
GalT, galactose-1-phosphate
uridylyltransferase;
ApnA, diadenosine
polyphosphate;
AMC, 7-diethylamino-4-methylcoumarin;
BODIPY FL, 4-4-difluoro-5,7-dimethyl-4-bora-3a,4a-diaza-s-indacine-3-yl;
ATP
Fhit-nucleotide Specificity Probed with Novel Fluorescent and
Fluorogenic Substrates*
§,,
Kimmel Cancer Center, Thomas Jefferson
University, Philadelphia, Pennsylvania 19107, and ¶ Molecular
Probes, Eugene, Oregon 97402
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
INTRODUCTION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
Asn allele of Fhit, which is more than a millionfold
reduced in kcat and intermediate formation (12),
is nonetheless functional in tumor suppression (6). Because this mutant
protein retains ApppA binding in the low micromolar range, it was
hypothesized that the tumor-suppressing function of Fhit consists of
the ability to form complexes with substrates rather than cleavage of
diadenosine polyphosphates (ApnA) (12). Much as
G-proteins are receptors for regulated GTP binding and hydrolysis that
transmit a signal as enzyme-substrate complexes, Fhit protein has been
hypothesized to signal for apoptosis as an enzyme-substrate complex
(13, 14). An alternative but not exclusive model suggests that the
tumor-suppressing function of Fhit may depend on promoting microtubule
assembly (15).
S and GTPS. We characterized the resulting ApppAMC,
ApppBODIPY, and GpppBODIPY compounds biochemically and found them to be
sensitive probes of Fhit activity. Despite a lack of any fluorescence
acceptor function on guanine, GpppBODIPY had fluorescence that was more
than 5-fold quenched relative to parental BODIPY compounds and with
respect to the ppBODIPY enzymatic product. Proton NMR measurements
reported herein provide evidence for the proximity of the guanine to
BODIPY, suggesting that BODIPY fluorescence is quenched by a stacked or
collisional mechanism (21).
S, and GTPS, and the KI of
Fhit for AMP, inorganic pyrophosphate, and monophosphate. Surprisingly,
pyrophosphate competes 10-fold better for the Fhit active site than do
purine mononucleotides. The results indicate that the ability of Fhit to function as an ApnA-dependent
signaling protein in epithelial tumor suppression may depend on a
hierarchy of competing compounds: ApnA competing
out pyrophosphate, and pyrophosphate competing out purine mononucleotides.
EXPERIMENTAL PROCEDURES
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
S or
GTPS tetralithium salts (25 mg, Sigma 85% pure, 0.05 mmol) were
dissolved in 3 ml of water, buffered to pH 9.0 with sodium bicarbonate.
Equimolar amounts of thiol-reactive fluorescent dyes
(7-diethylamino-3-(4'-maleimidylphenyl)-4-methylcoumarin (22) or
N-(4,4-difluoro-5,7-dimethyl-4-bora-3a,4a-diaza-s-indacine-3-yl)methyl)iodoacetamide (23), Molecular Probes) were added in 3.0 ml of dioxane. Reactions were
stirred and monitored by silica gel TLC, using
dioxane:2-propanol:water:ammonium hydroxide (40:20:35:35) as the mobile
phase. ATPS, GTPS, and the unreacted dyes migrated with
RF values of 0.25, 0.20, and 0.95, respectively,
while fluorescent adenosine nucleotide products had an
RF of 0.7 and GpppBODIPY had an
RF of 0.65. When, after several hours, reactions
were judged complete by TLC, the resulting solutions were concentrated
via rotary evaporation to 2 ml. Crude products were applied to an
aqueous 2 × 30-cm column of Sephadex LH-20 (Amersham Pharmacia
Biotech). Pooling and lyophilization of pure product fractions afforded
nucleotide-dye conjugates as their sodium salts with 76-86% yield.
For ApppAMC, 1H NMR (D2O) peaks were 8.51 (s,
1H, adenosine H2); 8.10 (s, 1H, adenosine H8); 7.55 (m, 2H, dye CH-3
and CH-5); 7.38 (m, 4H, dye phenyl); 6.81 (m, 1H, dye CH-6); 6.59 (d,
1H, dye CH-8); 6.10 (d, 1H, C1); 4.6 (m, 1H, -C(O)CHS-); 4.3 (m, 3H,
C2,C3,C4); 3.50 (m, 6H, C5 + NCH2CH3); 2.17 (s, 2H,
C(O)-CH2-CH); 1.22 (t, 6H, NCH2CH3); and 31P (D2O)
peaks were 6.5 ppm (d, 1P); -9.3 (m, 1P); -21.4 (m, 1P). For
ApppBODIPY, the proton peaks were 8.31 (s, 1H, adenosine H2); 8.03 (s,
1H, adenosine H8); 7.29 (s, 1H, dye CH); 6.83 (d, 1H, dye CH); 6.40 (d,
1H, dye CH); 6.29 (s, 1H, dye CH); 5.98 (d, 1H, C1); 4.59 (s, 2H,
-C(O)CH2S-); 4.51 (d, 2H, C5); 4.3 (m, 3H, C2,C3,C4); 3.75 (d, 2H, dye CH2NH-); 2.47 (s, 3H, dye CH3);
2.28 (s, 3H, dye CH3); and phosphorous peaks were 8.6 ppm
(d, 1P); -9.4 (d, 1P); -21.45 (dd, 1P). For GpppBODIPY, the proton
peaks were 7.90 (s, 1H, guanosine C8); 7.83 (br s, 1H, NH); 7.77 (br m,
4H, NH2 and OH); 7.29 (s, 1H, dye CH); 6.92 (s, 1H, dye
CH); 6.39 (s, 1H, dye CH); 6.25 (s, 1H, dye CH); 5.73 (m, 1H, C1); 4.57 (s, 2H, SCH2); 4.49 (t, 1H, C3); 4.41 (br s, 1H, C2); 4.28 (br s, 1H,
C4); 4.21 (dd, 2H, C5); 3.79 (dq, 2H, NCH2); 2.43 (s, 3H, dye CH3); and
2.25 (s, 3H, dye CH3). The covalent structures of ApppA, ApppAMC,
ApppBODIPY, and GpppBODIPY are represented in Fig. 1.
5 µl) were spotted on silica TLC
plates (E. Merck) at 60-120-s intervals. Plates were air-dried and
developed in 2-propanol:NH4OH:1,4-dioxane:H2O (50:35:8:7 for ApppAMC and ApppBODIPY; 50:33:6:11 for GpppBODIPY). Developed plates were imaged by epi-UV illumination and quantitated on
a Bio-Rad Fluor-S instrument using Multi-Analyst 1.0.2 software. Three
types of thin layer assays were performed. First-order decay assays,
reactions in which time courses of complete consumption of low
concentrations of fluorescent substrate were measured, were used to
determine the specificity constant,
kcat/Km. Initial rate assays,
reactions that measured the rates of appearance of the first few
percent of products formed as a function of substrate concentration,
were used to determine kcat and
Km. Competitive inhibition assays, first-order
assays with titration of nonlabeled competitive inhibitors, were used
to determine binding constants of competitors from their ability to
reduce
kcat/Km (apparent). For
first-order decay assays, substrate fluorescence minus background fluorescence was obtained in arbitrary units. Plots of log[remaining substrate] against time yielded experimental slopes, having units of
s
1, which were multiplied by 
1/[enzyme], to obtain
values of kcat/Km or
kcat/Km (apparent).
For initial rate assays, ppBODIPY fluorescence was converted to
picomoles with a standard product curve and kcat
and Km values were derived from Lineweaver-Burk
plots (24). For calculation of KI (or
Km) in competitive inhibition assays,
kcat/Km apparent values were
plotted against [I] and values of
kcat/Km and
KI (or Km) were determined
using Equation 1.
In these experiments, the value for
kcat/Km, although treated as
an independent variable, was always within 15% of the experimentally
determined value.
![<FR><NU>k<SUB><UP>cat</UP></SUB></NU><DE>K<SUB>m</SUB></DE></FR> (<UP>apparent</UP>)=<FR><NU>k<SUB><UP>cat</UP></SUB></NU><DE>K<SUB>m</SUB></DE></FR>−<FR><NU>[<UP>I</UP>]<FENCE><FR><NU>k<SUB><UP>cat</UP></SUB></NU><DE>K<SUB>M</SUB></DE></FR></FENCE></NU><DE>[<UP>I</UP>]+K<SUB>I</SUB></DE></FR>](/content/vol275/issue7/fulltext/4555/img001.gif)
(Eq. 1)
RESULTS
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
sheet that forms two
identical purine nucleotide-binding sites (9, 12, 25). In Hint dimers,
the two nucleotide-binding sites accommodate two equivalents of AMP or
GMP with the phosphates proximal to the catalytic histidines (9).
In Fhit dimers bound to ApnA, one pair of AMP
moieties are buried proximal to the catalytic histidines with
polyphosphate chains extending from the tightly bound AMP groups to
expose the second pair of adenosines in a solvent-accessible site near
Thr-79 (12). Because Fhit tolerates substitutions of the second
adenosine (3, 11), we expected that Fhit would hydrolyze ApppX-type
substrates to produce AMP plus ppX. Thiol-reactive fluorescent dyes,
7-diethylamino-3-(4'-maleimidylphenyl)-4-methylcoumarin (22) and BODIPY
FL C1-iodoacetamide (23), which were initially synthesized
to label protein thiols, were reacted with ATPS to generate first
generation fluorescent compounds, ApppAMC and ApppBODIPY. The second
generation substrate, GpppBODIPY, was made by conjugating BODIPY FL
C1-iodoacetamide to GTPS. Fluorescent substrates are depicted in Fig. 1.
View larger version (20K):
[in a new window]
Fig. 1.
Covalent structures of ApppA, ApppAMC,
ApppBODIPY, and GpppBODIPY. Fluorescent ApppA analogs were
synthesized from ATP S, GTPS, and thiol-reactive fluorescent dyes
as described under "Experimental Procedures."
View larger version (65K):
[in a new window]
Fig. 2.
Time courses of cleavage of fluorescent
substrates under
kcat/Km
conditions. Digital fluorescent images of ApppAMC (A),
ApppBODIPY (B), and GpppBODIPY (C) reactions
separated by TLC.
1
M1 and 2.3 × 106
s1 M1, respectively.
View larger version (17K):
[in a new window]
Fig. 3.
kcat/Km
determination of fluorescent substrates. Plots of log remaining
substrate fluorescence against time: ApppAMC (A),
ApppBODIPY (B), and GpppBODIPY (C).
Kinetic parameters with Fhit
1
M1 versus 3.8 × 107 s1 M1 for ApppA
(12)). Initial rates as a function of ApppBODIPY concentration were
measured and revealed that the basis for the catalytic disadvantage is
in the kcat term. While the
Km for ApppBODIPY, 3.0 µM, is less
than 60% higher than that for ApppA, the kcat
for ApppBODIPY, 7.3 s1, is 10-fold lower than that for
ApppA (Table I). Considering that ApppBODIPY is an ApppX-type compound,
containing an unaltered adenylating functionality (11), it is
interesting to consider why the BODIPY substitution affects
kcat rather than Km. Retention of a low Km at the expense of reduced
kcat could indicate that ApppBODIPY has multiple
binding modes, only some of which are productive, or that ppBODIPY is
not as good a leaving group as ADP. Thus, the 10-fold reduction in
kcat might correspond to the reciprocal fraction
of time ApppBODIPY is in a productive, ApppA-type conformation or a
tendency of the ppBODIPY product to re-attack His-96-AMP rather than
exiting the active site.
1 M1
versus 2.3 × 106 s1
M1) and that cleavage to ppBODIPY produces a
5.4-fold increase in fluorescence. The fluorogenic nature of GpppBODIPY
allowed us to measure hydrolysis continuously or as stopped end points
in a multiwell fluorescent plate reader. As shown in Table I,
substitution of guanine for adenine reduces kcat
10-fold while reducing Km 2-fold. In the crystal
structure of Hint-GMP, the carbonyl oxygen of His-42 makes a buried
hydrogen bond to the N-2 nitrogen of GMP (9). A similar interaction in
Fhit could be positioning the GMP moiety of GpppBODIPY nonoptimally for
catalysis and/or changing the rate-limiting step of the reaction.
S forms of these nucleotides (11) were
examined. All purine mononucleotides tested had
KI and Km values
approximately 10-fold higher than that of pyrophosphate. Monophosphate,
on the other hand, inhibited with a KI of
2.9 ± 0.4 mM.
View larger version (15K):
[in a new window]
Fig. 4.
Titration of ApppA as an inhibitor of
ApppBODIPY. Increasing concentrations of ligands reduce
kcat/Km
(apparent) and allow determination of K values
(Table I) using Equation 1.
View larger version (22K):
[in a new window]
Fig. 5.
Nucleotides and related compounds are
competitive with substrate. Increasing amounts of ApppA
(A), pyrophosphate (B), and AMP (C)
were titrated into initial rate assays of GpppBODIPY. For each
concentration of substrate and inhibitor, rates were plotted by the
method of Eadie and Hofstee.
DISCUSSION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
6, 2 E5, and 2 E4 M,
respectively, suggests that Fhit may have evolved a hierarchical system
to avail itself of ApnA in the presence of
competing compounds. Prior to our measurements of pyrophosphate and
purine mononucleotides as competitive inhibitors of Fhit, one might
have expected that the ground state of Fhit would be ATP-bound. Indeed,
if purine mononucleotides are at low millimolar levels (26), 10 times
their equilibrium-binding constants, ~90% of Fhit would be occupied
by mononucleotides in the absence of other competitors. The reported
amount of inorganic pyrophosphate (1.33 × 1016 mol,
Ref. 29) per lymphocyte (volume = 1.37 × 1013
liters, Ref. 30) suggests that the concentration of pyrophosphate (~1
mM) exceeds the KI for pyrophosphate
by 50-fold. Thus, Fhit may be primarily bound to pyrophosphate rather
than ATP under low ApnA conditions. From the
competition binding data presented in Table I, we calculate that a
spike of ~100 µM ApnA would
convert half the Fhit-pyrophosphate to
Fhit-ApnA. Conditions that lead to dramatic
increases in ApnA levels include interferon (31)
and etoposide (32) treatment of promyelocytes, and administration of
glucose to pancreatic cells (33).
ACKNOWLEDGEMENTS
FOOTNOTES
To whom correspondence should be addressed: Kimmel Cancer
Center, Thomas Jefferson University, 233 S. Tenth St., Rm. 826, Philadelphia, PA 19107. Tel.: 215-503-4573; Fax: 215-923-1696; E-mail:
brenner@dada.jci.tju.edu.
ABBREVIATIONS
S, adenosine 5'-O-(3-thiotriphosphate);
GTPS, guanosine
5'-O-(3-thiotriphosphate);
TLC, thin layer chromatography;
ATPS, adenosine 5'-O-(1-thiotriphosphate);
GTPS, guanosine 5'-O-(1-thiotriphosphate).
REFERENCES
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
1.
Ohta, M.,
Inoue, H.,
Cotticelli, M. G.,
Kastury, K.,
Baffa, R.,
Palazzo, J.,
Siprashvili, Z.,
Mori, M.,
McCue, P.,
Druck, T.,
Croce, C. M.,
and Huebner, K.
(1996)
Cell
84,
587-597[CrossRef][Medline]
[Order article via Infotrieve]
2.
Huebner, K.,
Garrison, P. N.,
Barnes, L. D.,
and Croce, C. M.
(1998)
Annu. Rev. Genet.
32,
7-31[CrossRef][Medline]
[Order article via Infotrieve]
3.
Barnes, L. D.,
Garrison, P. N.,
Siprashvili, Z.,
Guranowski, A.,
Robinson, A. K.,
Ingram, S. W.,
Croce, C. M.,
Ohta, M.,
and Huebner, K.
(1996)
Biochemistry
35,
11529-11535[CrossRef][Medline]
[Order article via Infotrieve]
4.
Sozzi, G.,
Pastorino, U.,
Moiraghi, L.,
Tagliabue, E.,
Pezzella, F.,
Ghirelli, C.,
Tornielli, S.,
Sard, L.,
Huebner, K.,
Pierotti, M. A.,
Croce, C. M.,
and Pilotti, S.
(1998)
Cancer Res.
58,
5032-5037 5.
Huebner, K.,
Sozzi, G.,
Brenner, C.,
Pierotti, M. A.,
and Croce, C. M.
(1999)
Adv. Oncol.
15,
3-10
6.
Siprashvili, Z.,
Sozzi, G.,
Barnes, L. D.,
McCue, P.,
Robinson, A. K.,
Eryomin, V.,
Sard, L.,
Tagliabue, E.,
Greco, A.,
Fusetti, L.,
Schwartz, G.,
Pierotti, M. A.,
Croce, C. M.,
and Huebner, K.
(1997)
Proc. Natl. Acad. Sci. U. S. A.
94,
13771-13776 7.
Ji, L.,
Fang, B.,
Yeh, N.,
Fong, K.,
Minna, J. D.,
and Roth, J. A.
(1999)
Cancer Res.
59,
3333-3339 8.
Sard, L.,
Accornero, P.,
Tornielli, S.,
Delia, D.,
Bunone, G.,
Campiglio, M.,
Colombo, M. P.,
Gramegna, M.,
Croce, C. M.,
Pierotti, M. A.,
and Sozzi, G.
(1999)
Proc. Natl. Acad. Sci. U. S. A.
96,
8489-8492 9.
Brenner, C.,
Garrison, P.,
Gilmour, J.,
Peisach, D.,
Ringe, D.,
Petsko, G. A.,
and Lowenstein, J. M.
(1997)
Nat. Struct. Biol.
4,
231-238[CrossRef][Medline]
[Order article via Infotrieve]
10.
Geeganage, S.,
and Frey, P. A.
(1998)
Biochemistry
37,
14500-14507[CrossRef][Medline]
[Order article via Infotrieve]
11.
Abend, A.,
Garrison, P. N.,
Barnes, L. D.,
and Frey, P. A.
(1999)
Biochemistry
38,
3668-3676[CrossRef][Medline]
[Order article via Infotrieve]
12.
Pace, H. C.,
Garrison, P. N.,
Robinson, A. K.,
Barnes, L. D.,
Draganescu, A.,
Rosler, A.,
Blackburn, G. M.,
Siprashvili, Z.,
Croce, C. M.,
Huebner, K.,
and Brenner, C.
(1998)
Proc. Natl. Acad. Sci. U. S. A.
95,
5484-5489 13.
Brenner, C.
(1999)
Phosphorus Sulfur Silicon
144,
745-748
14.
Brenner, C.,
Bieganowski, P.,
Pace, H. C.,
and Huebner, K.
(1999)
J. Cell. Physiol.
181,
179-187[CrossRef][Medline]
[Order article via Infotrieve]
15.
Chaudhuri, A. R.,
Khan, I. A.,
Prasad, V.,
Robinson, A. K.,
Luduena, R. F.,
and Barnes, L. D.
(1999)
J. Biol. Chem.
274,
24378-24382 16.
Brenner, C.,
Pace, H. C.,
Garrison, P. N.,
Robinson, A. K.,
Rosler, A.,
Liu, X. H.,
Blackburn, G. M.,
Croce, C. M.,
Huebner, K.,
and Barnes, L. D.
(1997)
Protein Eng.
10,
1461-1463 17.
Blackburn, G. M.,
Liu, X. H.,
Rosler, A.,
and Brenner, C.
(1998)
Nucleosides Nucleotides
17,
301-308[Medline]
[Order article via Infotrieve]
18.
Barnes, L. D.,
Robinson, A. K.,
Mumford, C. H.,
and Garrison, P. N.
(1985)
Anal. Biochem.
144,
296-304[CrossRef][Medline]
[Order article via Infotrieve]
19.
Ji, L.,
Fang, B.,
and Roth, J. A.
(1999)
Anal. Biochem.
271,
114-116[CrossRef][Medline]
[Order article via Infotrieve]
20.
Asensio, A. C.,
Oaknin, S.,
and Rotllan, P.
(1999)
Biochim. Biophys. Acta
1432,
396-400[CrossRef][Medline]
[Order article via Infotrieve]
21.
Dhar, G.,
and Bhaduri, A.
(1999)
J. Biol. Chem.
274,
14568-14572 22.
Khalfan, H.,
Abuknesha, R.,
Rand-Weaver, M.,
Price, R. G.,
and Robinson, D.
(1986)
Histochem. J.
18,
497-499[CrossRef][Medline]
[Order article via Infotrieve]
23.
Karolin, J.,
Johansson, L. B.-A.,
Strandberg, L.,
and Ny, T.
(1994)
J. Am. Chem. Soc.
116,
7801-7806[CrossRef]
24.
Jencks, W. P.
(1987)
Catalysis in Chemistry and Enzymology
, Dover Publications, New York
25.
Lima, C. D.,
Damico, K. L.,
Naday, I.,
Rosenbaum, G.,
Westbrook, E. M.,
and Hendrickson, W. A.
(1997)
Structure
5,
763-774[Medline]
[Order article via Infotrieve]
26.
Kornberg, A.,
and Baker, T. A.
(1992)
DNA Replication
, 2nd Ed.
, p. 54, W. H. Freeman and Company, New York
27.
Pekarsky, Y.,
Campiglio, M.,
Siprashvili, Z.,
Druck, T.,
Sedkov, Y.,
Tillib, S.,
Draganescu, A.,
Wermuth, P.,
Rothman, J. H.,
Huebner, K.,
Buchberg, A. M.,
Mazo, A.,
Brenner, C.,
and Croce, C. M.
(1998)
Proc. Natl. Acad. Sci. U. S. A.
95,
8744-8749 28.
Liu, X.,
Brenner, C.,
Guranowski, A.,
Starzynska, E.,
and Blackburn, G. M.
(1999)
Angew. Chem. Int. Ed.
38,
1245-1247
29.
Barshop, B. A.,
Adamson, D. T.,
Vellom, D. C.,
Rosen, F.,
Epstein, B. L.,
and Seegmiller, J. E.
(1991)
Anal. Biochem.
197,
266-272[CrossRef][Medline]
[Order article via Infotrieve]
30.
Thompson, C. B.,
Scher, I.,
Schaefer, M. E.,
Lindsten, T.,
Finkelman, F. D.,
and Mond, J. J.
(1984)
J. Immunol.
133,
2333-2342[Abstract]
31.
Vartanian, A.,
Narovlyansky, A.,
Amchenkova, A.,
Turpaev, K.,
and Kisselev, L.
(1996)
FEBS Lett.
381,
32-34[CrossRef][Medline]
[Order article via Infotrieve]
32.
Vartanian, A.,
Prudovsky, I.,
Suzuki, H.,
Dal Pra, I.,
and Kisselev, L.
(1997)
FEBS Lett.
415,
160-162[CrossRef][Medline]
[Order article via Infotrieve]
33.
Ripoll, C.,
Martin, F.,
Manuel Rovira, J.,
Pintor, J.,
Miras-Portugal, M. T.,
and Soria, B.
(1996)
Diabetes
45,
1431-1434[Abstract]
Copyright © 2000 by The American Society for Biochemistry and Molecular Biology, Inc.
CiteULike 
Complore 
Connotea 
Del.icio.us 
Digg 
Reddit 
Technorati What's this?
This article has been cited by other articles:
|
|
 |
|
  T. Takahashi, M. Tada, S. Igarashi, A. Koyama, H. Date, A. Yokoseki, A. Shiga, Y. Yoshida, S. Tsuji, M. Nishizawa, et al. Aprataxin, causative gene product for EAOH/AOA1, repairs DNA single-strand breaks with damaged 3'-phosphate and 3'-phosphoglycolate ends Nucleic Acids Res., June 28, 2007; 35(11): 3797 - 3809. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 A. W. Kijas, J. L. Harris, J. M. Harris, and M. F. Lavin Aprataxin Forms a Discrete Branch in the HIT (Histidine Triad) Superfamily of Proteins with Both DNA/RNA Binding and Nucleotide Hydrolase Activities J. Biol. Chem., May 19, 2006; 281(20): 13939 - 13948. [Abstract] [Full Text] [PDF]
|
|
|
|
|
|
H. F. Seidle, P. Bieganowski, and C. Brenner Disease-associated Mutations Inactivate AMP-Lysine Hydrolase Activity of Aprataxin J. Biol. Chem., June 3, 2005; 280(22): 20927 - 20931. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 H. Murakoshi, R. Iino, T. Kobayashi, T. Fujiwara, C. Ohshima, A. Yoshimura, and A. Kusumi Single-molecule imaging analysis of Ras activation in living cells PNAS, May 11, 2004; 101(19): 7317 - 7322. [Abstract] [Full Text] [PDF]
|
|
|
|
|
|
A. Krakowiak, H. C. Pace, G. M. Blackburn, M. Adams, A. Mekhalfia, R. Kaczmarek, J. Baraniak, W. J. Stec, and C. Brenner Biochemical, Crystallographic, and Mutagenic Characterization of Hint, the AMP-Lysine Hydrolase, with Novel Substrates and Inhibitors J. Biol. Chem., April 30, 2004; 279(18): 18711 - 18716. [Abstract] [Full Text] [PDF]
|
|
|
|
|
|
J. Korlach, D. W. Baird, A. A. Heikal, K. R. Gee, G. R. Hoffman, and W. W. Webb Spontaneous nucleotide exchange in low molecular weight GTPases by fluorescently labeled {gamma}-phosphate-linked GTP analogs PNAS, March 2, 2004; 101(9): 2800 - 2805. [Abstract] [Full Text] [PDF]
|
|
|
|
|
|
D. A. Kwasnicka, A. Krakowiak, C. Thacker, C. Brenner, and S. R. Vincent Coordinate Expression of NADPH-dependent Flavin Reductase, Fre-1, and Hint-related 7meGMP-directed Hydrolase, DCS-1 J. Biol. Chem., October 3, 2003; 278(40): 39051 - 39058. [Abstract] [Full Text] [PDF]
|
|
|
|
|
|
F. Trapasso, A. Krakowiak, R. Cesari, J. Arkles, S. Yendamuri, H. Ishii, A. Vecchione, T. Kuroki, P. Bieganowski, H. C. Pace, et al. Designed FHIT alleles establish that Fhit-induced apoptosis in cancer cells is limited by substrate binding PNAS, February 18, 2003; 100(4): 1592 - 1597. [Abstract] [Full Text] [PDF]
|
|
|
|
|
|
P. Bieganowski, P. N. Garrison, S. C. Hodawadekar, G. Faye, L. D. Barnes, and C. Brenner Adenosine Monophosphoramidase Activity of Hint and Hnt1 Supports Function of Kin28, Ccl1, and Tfb3 J. Biol. Chem., March 22, 2002; 277(13): 10852 - 10860. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 M. Yoshida, T. Sawada, H. Ishii, R. E. Gerszten, A. Rosenzweig, M. A. Gimbrone Jr, Y. Yasukochi, and F. Numano HMG-CoA Reductase Inhibitor Modulates Monocyte-Endothelial Cell Interaction Under Physiological Flow Conditions In Vitro : Involvement of Rho GTPase-Dependent Mechanism Arterioscler. Thromb. Vasc. Biol., July 1, 2001; 21(7): 1165 - 1171. [Abstract] [Full Text] [PDF]
|
|
|
|
|
|
T. A. Bennett, T. A. Key, V. V. Gurevich, R. Neubig, E. R. Prossnitz, and L. A. Sklar Real-time Analysis of G Protein-coupled Receptor Reconstitution in a Solubilized System J. Biol. Chem., June 15, 2001; 276(25): 22453 - 22460. [Abstract] [Full Text] [PDF]
|
|
| ||||||||||||||||||||||||||||||||||||||||||||||||||
