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Journal of Bacteriology, May 2001, p. 2874-2880, Vol. 183, No. 9
0021-9193/01/$04.00+0 DOI: 10.1128/JB.183.9.2874-2880.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
-Agglutinin and a-Agglutinin,
Saccharomyces cerevisiae Sexual Cell Adhesion
Molecules
Department of Biological Sciences and the Institute for Biomolecular Structure and Function, Hunter College of the City University of New York, New York, New York 10021,1 and Department of Biochemistry and Microbiology, Cook College, Rutgers University, New Brunswick, New Jersey 089012
Received 6 November 2000/Accepted 7 February 2001
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ABSTRACT |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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-Agglutinin and a-agglutinin are complementary cell adhesion
glycoproteins active during mating in the yeast Saccharomyces cerevisiae. They bind with high affinity and high specificity: cells of opposite mating types are irreversibly bound by a few pairs of
agglutinins. Equilibrium and surface plasmon resonance kinetic analyses
showed that the purified binding region of -agglutinin interacted
similarly with purified a-agglutinin and with a-agglutinin expressed on
cell surfaces. At 20°C, the KD for the
interaction was 2 × 10
9 to 5 × 109 M. This high affinity was a result of a very low
dissociation rate (
2.6 × 104 s1)
coupled with a low association rate (= 5 × 104
M1 s1). Circular-dichroism spectroscopy
showed that binding of the proteins was accompanied by measurable
changes in secondary structure. Furthermore, when binding was assessed
at 10°C, the association kinetics were sigmoidal, with a very low
initial rate. An induced-fit model of binding with substantial
apposition of hydrophobic surfaces on the two ligands can explain the
observed affinity, kinetics, and specificity and the conformational
effects of the binding reaction.
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INTRODUCTION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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There has been little work on the
binding characteristics of microbial cell adhesion proteins, which can
function under a variety of conditions not encountered in cell adhesion
systems of multicellular organisms (28). Sexual cell
adhesion in the yeast Saccharomyces cerevisiae is mediated
through two interacting cell wall glycoproteins,
a-agglutinin and -agglutinin, which are expressed on
haploid a and cells, respectively (29, 41).
These proteins are expressed at low levels constitutively, and gene
expression and cell surface concentration are upregulated in response
to a sex pheromone produced by the opposite mating type. The pheromones
do not change the binding affinity (40).
a-Agglutinin consists of two subunits. The binding subunit
Aga2p is a glycopeptide containing 69 amino acid residues and about 20 O-linked oligomannosyl chains (3). Aga2p carries the
adhesive domain, and its C-terminal 10 amino acids (sequence GSPINTQYVF ) can act as a ligand for -agglutinin
(2). A pair of disulfide bonds links Aga2p to the
anchorage subunit of a-agglutinin Aga1p (2,
35). Aga1p itself is a highly O-glycosylated protein of 725 amino acid residues including an N-terminal secretion signal and a
C-terminal signal for addition of a glycosyl phosphatidylinositol anchor (GPI). Aga1p anchors Aga2p onto the cell surface but has no
direct role in binding (35, 35a).
-Agglutinin, the other cell adhesion molecule responsible for
agglutination, is the product of the AG1
(SAG1) gene. The N-terminal half of -agglutinin is
homologous to the immunoglobulin superfamily and contains the binding
site for a-agglutinin (4, 16, 42). This region
is 
-sheet rich and shows a high degree of conformational flexibility
(45, 46). Residues near His292 and
Lys154 have been implicated in binding (2, 4, 6,
45). The C-terminal half of -agglutinin anchors the protein
and consists of a highly glycosylated "stalk" of about 300 amino
acids. This is followed by a modified GPI anchor that covalently
attaches the molecule to 1,6-glucan, a cell wall polysaccharide
(31, 32, 42). These features of the -agglutinin
sequence are similar to those of several Candida albicans
cell adhesion proteins that mediate host-pathogen interactions
(11-13, 17, 18).
The agglutinins bind tightly to each other at low to moderate ionic
strengths and with a pH optimum of 5.5. Binding of
125I--agglutinin fragments to cell-bound
a-agglutinin showed a specific and complex interaction
consistent with at least two states, weak and tight. Weakly bound
125I--agglutinin was removed from the a cells
by washing. The tight state had a KD of about
109 M and was essentially irreversible, implying a low
rate of dissociation (30). Formation of this state was
cold sensitive.
We now describe a study of the binding interaction based on highly purified recombinant agglutinins. A surface plasmon resonance (SPR) analysis confirmed the original estimates of KD and together with circular dichroism (CD) showed a conformational basis for complex binding kinetics. The binding kinetics demonstrated a basis for the cold sensitivity of sexual agglutination.
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MATERIALS AND METHODS |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Materials.
The following reagents were obtained from Sigma
Chemical Company, St. Louis, Mo: cycloheximide,
p-chloromercuribenzoic acid (PCMB), -methylmannoside, and
bovine serum albumin (BSA). Protein standards, Bio-Gel P-60, and
Bio-Gel P-100 were purchased from Bio-Rad (Richmond, Calif.).
Restriction enzymes were from New England Biolabs. Endoglycosidase H
was from Boehringer Mannheim. Plasmon resonance experiments were
performed on BIACORE X, which together with C1 sensor
chips, N-hydroxysuccinimide (NHS),
N-ethyl-N'-(3-dimethylaminopropyl)-carbodiimide hydrochloride, and 1 M ethanolamine (pH 8.5) were obtained from Pharmacia Biosensor AB (Uppsala, Sweden). Polyacrylamide gel
electrophoresis (PAGE) reagents and standards were from Bio-Rad.
Purification of Aga2p.
W303 diploid cells containing plasmid
YEpPGK-AGA2 constitutively expresses Aga2p under the control
of the PGK promoter. Cells were grown in synthetic medium
without uracil to 4 × 107/ml and harvested. Cell
culture supernatants were then collected and concentrated 10-fold
through a Millipore filter with a 10-kDa molecular-mass cutoff.
Concentrated supernatant was further dialyzed against 20 mM sodium
acetate (pH 5.5)-1 mM EDTA, lyophilized, and resuspended in the same
buffer with 10% (vol/vol) glycerol. Aga2p was purified using a Bio-Gel
P-60 size exclusion column equilibrated in 20 mM sodium acetate, pH
5.5. Because of its extensive glycosylation, Aga2p has an apparent
molecular mass of 33 kDa on sodium dodecyl sulfate (SDS)-polyacrylamide
gels stained with Coomassie blue (Fig.
1).
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Purification of -agglutinin.
-Agglutinin containing
residues 20 to 351 (-agglutinin20-351) was purified
from the cell culture supernatant (4 liters) of yeast strain L21
(MAT ade2-1 his3-11,15 leu2-3,112 trpl-1 ura3-1 can1-100 ag1-3) containing
pPGK-AGl351. A DEAE-Sephadex A-25 column and
a Bio-Gel P-60 size exclusion column were used for the purification
(4). Partially deglycosylated -agglutinin20-351 had an apparent molecular mass of 45 kDa on Coomassie blue-stained SDS-polyacrylamide gel and was of 99%
purity by scanning densitometry (Molecular Dynamics) (Fig. 1).
PAGE. The protein samples were electrophoresed in SDS- or non-SDS-polyacrylamide gels with 10% running gels and 4% stacking gels (26).
Anti--agglutinin antibody preparation.
Anti--agglutinin antibody was produced by injecting purified protein
(100 µg, twice) in Hunter's Titermax into rabbits. The sera were
then collected 10 to 25 weeks after the initial injection and were
absorbed twice against washed, heat-killed a cells.
Separation of -agglutinin aggregates and immunodetection.
A sample of purified -agglutinin was thawed and filtered through a
Bio-Gel P-100 column in 100 mM sodium acetate, pH 5.5. The samples
collected from the column were electrophoresed in non-SDS- and
SDS-10% polyacrylamide gels and then transferred to a nitrocellulose
membrane by electrophoresis. The blot was first incubated in 10 mM
Tris-140 mM NaCl (pH 7.4; buffer B), with 3% gelatin for 30 min and
then in anti--agglutinin antibody (diluted 1:500) for 1 h.
Afterwards, the blot was washed and incubated in anti-rabbit
immunoglobulin G peroxidase conjugate (diluted 1:1,000) in buffer B
with 1% gelatin for 1 h. The blot was then washed and visualized
with 4-chloro-1-naphthol in 10 ml of cold methanol and 3% hydrogen
peroxide in 50 ml of buffer B. The fractions containing no aggregates
were used for BIACORE experiments.
SPR. The detection of binding or dissociation in SPR is based on the change in the refractive index due to association of a soluble analyte to an immobilized ligand. The resulting signal is proportional to the amount of protein bound, and 1,000 resonance units correspond to 1 ng/mm2 (20). The flat carboxymethylated surface of a C1 sensor chip was first cleaned with 10 µl of 0.1 M glycine-NaOH and then activated by 35 µl of a solution containing 0.2 M N-ethyl-N'-3-aminopropyl carbodiimide and 0.05 M NHS at a flow rate of 5 µl/min. Then, two 25-µl aliquots of purified Aga2p (5 µg/ml) in 100 mM phosphate buffer were injected over the surface at a flow rate of 5 µl/min. The remaining unreacted NHS-ester groups were deactivated by injection of 25 µl of 1 M ethanolamine-HCl, pH 8.5, and the surface was further blocked by injecting if twice with 25 µl of 100-µg/ml BSA in HBS buffer (10 mM HEPES and 150 mM NaCl, pH 7.4). The flow rate was 5 µl/min.
The buffer was then switched to MES buffer (10 mM MES [morpholineethanesulfonic acid] and 150 mM NaCl, pH 5.9), and the chip was blocked twice more by injection of BSA. MES buffer was used as the association and dissociation buffer for the interaction of a-agglutinin and-agglutinin. Association and subsequent dissociation were measured by the injection of 100 µl of an
-agglutinin solution at a flow rate of 20 µl/min, using several
concentrations of -agglutinin The sensor surface was regenerated by
injection of 100 µl of 4 M MgCl2.
The association rate constant (Kon) and the
dissociation rate constant (koff) were obtained
from curve fitting by nonlinear least-squares regression. The
equilibrium dissociation constant was calculated from the following
equation: KD = koff/kon. Data analysis
was performed using the BIA Evaluation 3.0 software package (Pharmacia
Biosensor AB) (21), which calculates nonlinear regressions according to the Langmuir isotherm theory. Curves from 20°C isotherms were fitted over 200-s intervals, with mean residuals of 2%. The sigmoidal associations at 10°C were fitted in two independent regions
of the binding curve, an early region (110 to 180 s) and a later
one (200 to 330s). For the early regions, the mean residual was <3%,
and for the late regions, it was <2%. Estimates of
koff were obtained from 30-min dissociation
curves to compensate for the low rate and the apparent linearity at
shorter times. The values were also checked by hand on semilogarithmic plots.
Isotopic labeling of -agglutinin with 125I-Bolton
Hunter reagent.
Purified -agglutinin (0.1 mg/ml) was dialyzed
against 200 mM sodium phosphate buffer, pH 8.5, overmight. The protein
(20 µg) was reacted with 250 µCi of 125I-Bolton Hunter
reagent (New England Nuclear Corp.) for 3 h at 0°C. The reaction
mixture was diluted 20-fold in the reaction buffer (100 mM sodium
acetate [pH 5.5], 1 µM CaCl2, and 1 µM
MnSO4). The diluted sample was applied to a 1-ml prepacked
lentil lectin-agarose column, which was preequilibrated with reaction
buffer. The protein was eluted with 1 M -methylmannoside and 500 mM
sodium chloride in 100 mM sodium acetate, pH 5.5. The labeled
-agglutinin was stored at 4°C in the eluting buffer supplemented
with 10% glycerol and 1 mg of BSA per ml.
Binding of 125I--agglutinin to yeast cells.
Various concentrations of 125I--agglutinin were
incubated with 2 × 106 X2180-1A
(MATaSUC2 mal mel gal2
CUP1) or X2180-1B (MAT SUC2 mal mel
gal2 CUP1) cells in a total volume of 250 µl on a rotary
shaker at 200 rpm at 25 or 0°C for 90 min, the time required to reach
equilibrium. The buffer used for this study was 100 mM sodium acetate,
pH 5.5, supplemented with 1 mg of BSA per ml, 1µg of cycloheximide
per ml, 1 µM p-chloromercuribenzoic acid (39). After the incubation, cells with bound
-agglutinin were centrifuged, the supernatants were aspirated, and
the cells were then washed three times. The bound
125I--agglutinin was counted in a Compugamma 1282 (LKB
Wallac Inc.), and specific binding was determined as the difference in
the levels of binding between MATa and
MAT cells under identical conditions. The nonspecific
binding to MAT cells was not saturable and was similar to
noncompetable binding to MATa cells, as
previously reported. (39). Equilibrium constants were
determined from Scatchard analysis of the binding.
Concentration determination of
125I--agglutinin.
Samples of
125I--agglutinin (10 µl) were incubated with 2 × 106 a or cells in a 200-µl total volume to
obtain the maximum specific binding capacity of a cells.
Specific binding was then determined in a competition assay between
125I--agglutinin (5 µl) and different concentrations
of unlabeled -agglutinin of known concentration. After incubation,
the cells with bound 125I--agglutinin were washed and
counted. The concentration of 125I--agglutinin was
calculated to be 0.105 µM in the stock solution, based on the
concentration of unlabeled -agglutinin giving 50% inhibition of
binding (1).
Peptide synthesis. A peptide containing the C-terminal 10 residues of Aga2p was synthesized by the solid-phase method using fluorenylmethoxycarbonyl chemistry on an Applied Biosystems automated model 432A peptide. The peptide resins were treated with 80% trifluoroacetic acid (TFA)-5% water-5% ethanedithiol-10% thioanisole at room temperature for 2 h to cleave and deprotect the peptides, which were then precipitated and washed in cold methyl t-butyl ether and collected by centrifugation at 25°C.
Purification of the peptides was achieved by reverse-phase high-performance liquid chromatography on a C18 column (21.4 by 250 mm) using 0.1% TFA as buffer A and 70% acetonitrile in 0.1% TFA as buffer B. A linear gradient between 0 and 100% buffer B in buffer A was used at a flow rate of 5 ml/min over a period of 60 min. The elution profile was monitored at 215 nm. The purified peptides were lyophilized and redissolved in deionized water at 25°C and stored at 4°C.Agglutination assay.
S. cerevisiae wild-type
haploid strains X2180-1A (MATa SUC2 mal mel
gal2 CUP1) and X2180-1B (MAT SUC2 mal mel
gal2 CUP1) were used for bioassays. a cells and cells were grown separately in minimal medium to 2 × 107 cells per ml, and a cells were treated with
the sex pheromone -factor as described previously (41).
These cells were harvested and washed in 100 mM sodium acetate, pH 5.5, at 25°C. -Agglutinin was incubated with a cells on a
rotary shaker at 25°C for 90 min, and cells were then added. The
activity of -agglutinin was determined by its ability to inhibit the
agglutination of a cells (41), with 1 U being
the amount of protein needed to inhibit agglutination by 10%.
CD spectroscopy. Far-UV CD spectra were recorded on a Jasco J-710 spectropolarimeter equipped with a thermo-regulated cell holder with a 0.05-cm path length (HELLMA). Each spectrum represents the average of 10 spectra taken at 0.5-nm intervals from 250 to 200 nm. The spectra were corrected by subtraction of the appropriate buffer baseline spectra and smoothed by Jasco Series 700 software. Each experiment was repeated three times. CD data presented here were analyzed by the self-consistent method (SELCON) (36, 37).
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RESULTS |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Binding of 125I--agglutinin to intact cells.
As
indicated in Fig. 2, the binding of
125I--agglutinin to a cells at 25 and 0°C
showed only slight differences in affinity or site numbers. There was
little nonspecific binding to cells of mating type . When the
protein concentration was 5 nM or higher, the binding approached
saturation. The inset of Fig. 2 shows Scatchard plots of the binding,
with cells displaying a KD of 6.34 × 1010 M at 0°C and 8.6 × 1010 M at
25°C, values similar to that previously reported (30). There were about 7.5 × 104 -agglutinin molecules
bound per a cell at saturation. For samples incubated at
either temperature, washing the cells before counting did not reduce
the specific binding significantly. Therefore, no weak interactions
were observed at either temperature. We speculate that the weak and
cold-sensitive binding seen in a previous study might have been due to
low-affinity binding of partially active fragments of -agglutinin
(30).
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SPR analysis of binding kinetics.
In equilibrium binding
experiments with radioactively labeled -agglutinin, low temperature
had little effect on the binding isotherm. However, previous studies
showed that low temperature does reduce cellular agglutinability both
in vivo and in vitro (41, 43). SPR was used to obtain the
koff and the kon and to
detect the effect of low temperature on the interaction of the
agglutinins in real time.
-agglutinin was adjusted so that the
response amplitude of the binding would be in the desired range
(22, 33). "Sensorgrams" for the interaction of various
concentrations of -agglutinin with the immobilized a-agglutinin at 20 and 10°C are shown in Fig.
3. At 20°C there was a very low
koff of (7.0 ± 1.4) × 105 s1 and a single
kon of (4.61 ± 0.03) × 104 M1 s1. These values give a
KD of (1.55 ± 0.31) × 109.
At 10°C, the koff was (5.4 ± 0.5) × 105 s1 (Fig. 3), slightly lower than
that at 20°C. A sigmoid association curve was observed with an
initial very low kon of (0.13 ± 0.07) M1 s1 and a later higher
kon of (5.59 ± 0.4) × 104 M1 s1, similar to the
single kon at 20°C. Therefore, at 10°C there were two apparent dissociation constants, (6.18 ± 3.49) × 104 M and (9.8 ± 1.0) × 1010 M.
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Effects of protein aggregates.
Protein aggregates may
sometimes bind with high affinity, and dissociation rates decrease in
geometric proportion to the number of the binding sites in the
aggregates (24, 44). To correct the estimate of
koff for the presence of aggregates,
gel-filtered -agglutinin was prepared and injected into the BIACORE
instrument. This material had a kon of (5.6 ± 2.2) × 104 M1, similar to that of
the experiment shown in Fig. 3, and a higher koff of (2.6 ± 0.6) × 104 s1, corresponding to a
KD of (5.5 ± 2.6) × 109 M.
Conformational changes of the agglutinins induced by
a-agglutinin peptide binding.
Sigmoidal association kinetics
and low kon and koff are
characteristics of binding dependent on conformational change in the ligands (induced-fit models [25]). A CD analysis of
binding of -agglutinin binding to an a-agglutinin peptide
tested for conformational changes on binding.
-agglutinin and competes with Aga2p
(2). We synthesized this peptide and found its specific
activity to be 2.6 × 1010 U/mol, similar to that
previously determined (3) and corresponding to an affinity
250-fold less than that of native of a-agglutinin). We have
also found that site-specific mutations in the C-terminal residues of
Aga2p inactivate it. No other region of the protein was required for
activity (35a).
We then determined far-UV CD spectra of 5 × 106 M
-agglutinin and the 1 × 105 M Aga2p C-terminal
decapeptide. A spectrum of a complex of these components was acquired
after coincubation in 10 mM sodium acetate, pH 5.5, at 25°C for 30 min. Under these conditions, at least 96% of the -agglutinin would
have ligand bound. The CD spectrum of the a-agglutinin
peptide in the same buffer was then subtracted from that of the
complex. The difference spectrum (Fig. 4)
showed that the complex still contained a principal negative magnitude band at 217 nm, which was narrower than that of -agglutinin alone. The positive peak below 207 nm was strongly intensified, and there was
an extra positive shoulder at 225 to 234 nm. All these changes came
either from conformational changes of -agglutinin upon binding or a
combination of secondary-structure changes of both -agglutinin and
the a-agglutinin peptide. Secondary-structure analysis was
consistent with a slight increase in each of the periodic structural
components and a decrease in aperiodic structure from 38.6 to 31.6%
(36). These changes are greater than the measured experimental errors, so some unstructured regions of a- and
-agglutinin became more structured upon ligand binding
(15). An increase in structure for 7% of the residues
would correspond to about 24 amino acid residues.
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Effect of reduced temperature on the conformation of
-agglutinin.
To determine if cold temperature affected the
secondary structure of -agglutinin, far-UV CD spectra of
-agglutinin were measured and compared at 25 and 0°C. As shown in
Fig. 5, CD spectra at both temperatures
showed a major band at 217 nm, a contribution of peptide chromophores
in -conformation. However, at 0°C, the magnitude of the negative
band at 217 nm was intensified and broadened at lower wavelengths,
indicating a possible increase of -sheet structure. In addition, at
0°C, the spectrum was less negative between 227 and 237 nm. The
protein appeared to be more structured at low temperature than at room
temperature: the total -sheet content increased from 47.8 to 54.4%,
and the random structure dropped from 36.5 to 26.1%. Such a change
corresponds to an addition of about 24 to 34 residues to regions with
periodic secondary structures (-helix or -sheet).
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Complexity of binding.
Kinetics and secondary-structure
analysis of interacting yeast sexual agglutinins showed complexity and
the characteristics of an induced-fit interaction (25).
The binding parameters obtained in various experiments yield
KDs of 1 × 109 to 5 × 109 M, corresponding to a binding energy of 
11 to 12
kcal/mol. The uncertainty in KD results from the
uncertainty in the koff, which is close to the
limit of reliability of SPR, and indeed equilibrium binding gives a
KD corresponding to the tighter binding value.
-agglutinin and also the ligand
a-agglutinin. All of these observations are compatible with
a model in which initial interaction of the agglutinins triggers a
conformational shift that greatly increases the contact area between
the glycoproteins, resulting in tight binding and a very low
dissociation rate, as observed.
Effect of low temperature on protein flexibility.
Incubation
at 0 to 10°C results in poor agglutination of intact cells (41,
43). In SPR experiments (Fig. 3), there was also a marked
decrease in the initial association rate of the agglutinins at low
temperatures. This result can be interpreted as reduced flexibility in
one or both of the components. There is direct evidence for such
reduced flexibility in -agglutinin at reduced temperatures. This
protein showed a 7 to 10% increase in the fraction of the periodic
secondary structure (-helix and -sheet) and a concomitant
decrease in the fraction of the aperiodic secondary structure. The
increase in the fraction of the periodic secondary structure
encompasses 24 to 34 residues, far greater than the standard deviation
for secondary-structure assignments (about 1.3% or 4 residues). This
change represents a decrease in the inherent flexibility of
-agglutinin (45, 46), because the conformations of
residues in sheets and helices are stabilized by backbone hydrogen
bonding, as well as by side chain interactions. However, the binding
characteristics implied that, at low temperatures, the rate-limiting
step was a conformational change in the ligand a-agglutinin.
Conformational changes on binding.
The conformational change
observed on binding includes removal of about 24 amino acids from less
structured aperiodic conformations to helix or sheet. There are 10 residues in the a-agglutinin peptide used as the ligand, so
there is an approximate minimum of 14 residues of -agglutinin whose
secondary-structural state is altered by binding. There is a precedent
for this type of interaction: PDZ domains bind the C-terminal regions
of their ligands, with the ligand forming an extra -strand in a
sheet. Like the agglutinin system, the ligand-receptor complex is more
structured than the sum of the individual components. Also, like in the
agglutinin system, binding is tight and dissociation is extremely slow
(5, 7).
A model of the interaction of the agglutinins at different
temperatures.
A model of the interaction between the agglutinins
based on binding data and secondary-structure analysis is shown
below: inhibited at low temperature +[] [a'] 
[a] [a·]
-Agglutinin binds to state [a] with
high affinity in a multistep reaction at room temperature.
-Agglutinin binds to state [a'] poorly, if it binds at
all. The result is a sigmoidal kinetic association curve at low
temperature. As the -agglutinin binds to the small amount of
agglutinin available in the [a] state, the resulting depletion of agglutinin in the [a] state promotes the slow formation of more agglutinin in the [a] state from that in
the [a'] inactive state. At low temperatures the apparent initial kon is 5 × 105-fold lower than at 25°C; this difference is enough to
delay bond formation measurably in agglutination assays
(41) as well as in the SPR association experiment (Fig.
3B). There is no significant effect on binding in extended incubations
with 125I--agglutinin (Fig. 2), because the
a-agglutinin is present in great excess in those
experiments, and there is sufficient material in the [a]
state to bind the available -agglutinin.
Similar binding systems.
The above model of binding-induced
conformational changes of the agglutinins is similar to the induced-fit
model of interaction of substrate and enzyme, where the active site of
the enzyme assumes a shape complementary to that of the substrate after
it is bound (25). Well-characterized examples include
interactions of antigens with antibodies. For example, a structural
rearrangement next to the helical binding site of a tobacco mosaic
virus protein occurs during the high-affinity interaction between the
protein and its antibody (9, 34). Slow conformational
changes of human immunodeficiency virus core protein p24 are involved
in the high-affinity interaction of the protein to its own monoclonal antibody (14). Conformational changes of the integrin
IIb3 (platelet GPIIb-IIIa) triggered by
binding of Arg-Gly-Asp sequences in fibrinogen generate a high-affinity
binding state of integrin (8). Using SPR, Huber also
studied the interaction of IIb3 with
fibrinogen and found an initial low-affinity interaction leading to a
higher-affinity state (19). Conformational changes of the
cell adhesion protein thrombrospondin are induced by binding to the
receptor CD36 (GPIIIb or GPIV) (27).
Biological consequences of binding.
In the yeast sexual
agglutination system, the situation in vivo is that cellular
aggregation is irreversible. Cell surface concentrations of the
agglutinins are about 103 M after their expression has
been upregulated by sex pheromones (35a). At this
concentration, strong adhesive bonds between agglutinating cells would
form within a few seconds, as has been observed previously (38). A dissociation rate of 104
s1 would mean that two singly tethered cells likely
dissociate in several hours, about the time two cells take to fuse. The
koff values for bivalent systems are the
products of the univalent rates. So, if two cells were attached through
two adhesive bonds, the dissociation of most pairs would take
108 s (more than a year). Thus, in contrast to the
transient interactions that characterize cell interactions in the
immune system, yeast sexual agglutination makes adhesive bonds that are
irreversible within biologically relevant times.
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ACKNOWLEDGMENTS |
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We thank Dixie Goss, in the Department of Chemistry at Hunter College, for use of the CD spectrophotometer.
This work was supported by grants from the National Institute of General Medical Science (1R01-GM47176) to Janet Kurjan, University of Vermont; the Research Center in Minority Institutions Program of the NIH (RR-03037); and the New Jersey Agriculture Experiment Station (paper D-01405-1-01).
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FOOTNOTES |
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* Corresponding author. Mailing address: Department of Biological Sciences, Hunter College, 695 Park Ave., New York, NY 10021. Phone: (212) 772-5235. Fax: (212) 772-5227. E-mail: lipke{at}genectr.hunter.cuny.edu.
Present address: Brigham and Women's Hospital, Harvard Medical
School, Boston, MA 02115.
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REFERENCES |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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| 1. | Berson, S. A., and R. S. Yalow. 1967. Radioimmunoassays of peptide hormones in plasma. N. Engl. J. Med. 277:640-647. |
| 2. | Cappellaro, C., C. Baldermann, R. Rachel, and W. Tanner. 1994. Mating type-specific cell-cell recognition of Saccharomyces cerevisiae: cell wall attachment and active sites of a- and alpha-agglutinin. EMBO. J. 13:4737-4744[Medline]. |
| 3. | Cappellaro, C., K. Hauser, V. Mrsa, M. Watzele, G. Watzele, C. Gruber, and W. Tanner. 1991. Saccharomyces cerevisiae a- and alpha-agglutinin: characterization of their molecular interaction. EMBO J. 10:4081-4088[Medline]. |
| 4. |
Chen, M. H.,
Z. M. Shen,
S. Bobin,
P. C. Kahn, and P. N. Lipke.
1995.
Structure of Saccharomyces cerevisiae alpha-agglutinin. Evidence for a yeast cell wall protein with multiple immunoglobulin-like domains with atypical disulfides.
J. Biol. Chem.
270:26168-26177 |
| 5. | Daniels, D. L., A. R. Cohen, J. M. Anderson, and A. T. Brunger. 1998. Crystal structure of the hCASK PDZ domain reveals the structural basis of class II PDZ domain target recognition. Nat. Struct. Biol. 5:317-325[CrossRef][Medline]. |
| 6. | de Nobel, H., P. N. Lipke, and J. Kurjan. 1996. Identification of a ligand-binding site in an immunoglobulin fold domain of the Saccharomyces cerevisiae adhesion protein alpha-agglutinin. Mol. Biol. Cell 7:143-153[Abstract]. |
| 7. | Doyle, D. A., A. Lee, J. Lewis, E. Kim, M. Sheng, and R. MacKinnon. 1996. Crystal structures of a complexed and peptide-free membrane protein-binding domain: molecular basis of peptide recognition by PDZ. Cell 85:1067-1076[CrossRef][Medline]. |
| 8. | Du, X. P., E. F. Plow, A. L. Frelinger, T. E. O'Toole, J. C. Loftus, and M. H. Ginsberg. 1991. Ligands "activate" integrin alpha IIb beta 3 (platelet GPIIb-IIIa). Cell 65:409-416[CrossRef][Medline]. |
| 9. | Dubs, M. C., D. Altschuh, and M. H. Van Regenmortel. 1992. Interaction between viruses and monoclonal antibodies studied by surface plasmon resonance. Immunol. Lett. 31:59-64[CrossRef][Medline]. |
| 10. | Friguet, B., L. Djavadi-Ohaniance, and M. E. Goldberg. 1989. Polypeptide-antibody binding mechanism: conformational adaptation investigated by equilibrium and kinetic analysis. Res. Immunol. 140:355-376[CrossRef][Medline]. |
| 11. |
Fu, Y.,
G. Rieg,
W. A. Fonzi,
P. H. Belanger,
J. E. Edwards, Jr., and S. G. Filler.
1998.
Expression of the Candida albicans gene ALS1 in Saccharomyces cerevisiae induces adherence to endothelial and epithelial cells.
Infect. Immun.
66:1783-1786 |
| 12. | Gaur, N. K., and S. A. Klotz. 1997. Expression, cloning, and characterization of a Candida albicans gene, ALA1, that confers adherence properties upon Saccharomyces cerevisiae for extracellular matrix proteins. Infect. Immun. 65:5289-5294[Abstract]. |
| 13. |
Gaur, N. K.,
S. A. Klotz, and R. L. Henderson.
1999.
Overexpression of the Candida albicans ALA1 gene in Saccharomyces cerevisiae results in aggregation following attachment of yeast cells to extracellular matrix proteins, adherence properties similar to those of Candida albicans.
Infect. Immun.
67:6040-6047 |
| 14. | Glaser, R. W., and G. Hausdorf. 1996. Binding kinetics of an antibody against HIV p24 core protein measured with real-time biomolecular interaction analysis suggest a slow conformational change in antigen p24. J. Immunol. Methods 189:1-14[CrossRef][Medline]. |
| 15. | Greenfield, N. J. 1996. Methods to estimate the conformation of proteins and polypeptides from circular dichroism data. Anal. Biochem. 235:1-10[CrossRef][Medline]. |
| 16. | Grigorescu, A., M.-H. Chen, H. Zhao, P. C. Kahn, and P. N. Lipke. 2000. A CD2-based model of yeast alpha-agglutinin elucidates solution properties and binding characteristics. IUBMB Life 50:105-113[CrossRef][Medline]. |
| 17. | Hoyer, L. L., and J. E. Hecht. 2000. The ALS6 and ALS7 genes of Candida albicans. Yeast 16:847-855[CrossRef][Medline]. |
| 18. | Hoyer, L. L., T. L. Payne, M. Bell, A. M. Myers, and S. Scherer. 1998. Candida albicans ALS3 and insights into the nature of the ALS gene family. Curr. Genet. 33:451-459[CrossRef][Medline]. |
| 19. | Huber, W., J. Hurst, D. Schlatter, R. Barner, J. Hubscher, W. C. Kouns, and B. Steiner. 1995. Determination of kinetic constants for the interaction between the platelet glycoprotein IIb-IIIa and fibrinogen by means of surface plasmon resonance. Eur. J. Biochem. 227:647-656[Medline]. |
| 20. | Johnsson, B., S. Lofas, and G. Lindquist. 1991. Immobilization of proteins to a carboxymethyldextran-modified gold surface for biospecific interaction analysis in surface plasmon resonance sensors. Anal. Biochem. 198:268-277[CrossRef][Medline]. |
| 21. | Jonsson, U., L. Fagerstam, B. Ivarsson, B. Johnsson, R. Karlsson, K. Lundh, S. Lofas, B. Persson, H. Roos, I. Ronnberg, et al. 1991. Real-time biospecific interaction analysis using surface plasmon resonance and a sensor chip technology. BioTechniques 11:620-627[Medline]. |
| 22. | Karlsson, R. 1994. Real-time competitive kinetic analysis of interactions between low-molecular-weight ligands in solution and surface-immobilized receptors. Anal. Biochem. 221:142-151[CrossRef][Medline]. |
| 23. | Karlsson, R., A. Michaelsson, and L. Mattsson. 1991. Kinetic analysis of monoclonal antibody-antigen interactions with a new biosensor based analytical system. J. Immunol. Methods 145:229-240[CrossRef][Medline]. |
| 24. | Kishore, U., L. E. A. Leigh, P. Eggleton, P. Strong, M. V. Perdikoulis, A. C. Willis, and K. B. Reid. 1998. Functional characterization of a recombinant form of the C-terminal, globular head region of the B-chain of human serum complement protein, C1q. Biochem. J. 333:27-32. |
| 25. | Koshland, D. E., Jr., and K. E. Neet. 1968. The catalytic and regulatory properties of enzymes. Annu. Rev. Biochem. 37:359-410[CrossRef][Medline]. |
| 26. | Laemmli, U. K. 1970. Cleavage of structural proteins during the assembly of the head of bacteriophage T4. Nature 227:680-685[CrossRef][Medline]. |
| 27. |
Leung, L. L.,
W. X. Li,
J. L. McGregor,
G. Albrecht, and R. J. Howard.
1992.
CD36 peptides enhance or inhibit CD36-thrombospondin binding. A two-step process of ligandreceptor interaction.
J. Biol. Chem.
267:18244-18250 |
| 28. | Lipke, P. N. 1996. Cell adhesion proteins in the nonvertebrate eukaryotes. Prog. Mol. Subcell. Biol. 17:119-157[Medline]. |
| 29. |
Lipke, P. N., and J. Kurjan.
1992.
Sexual agglutination in budding yeasts: structure, function, and regulation of adhesion glycoproteins.
Microbiol. Rev.
56:180-194 |
| 30. |
Lipke, P. N.,
K. Terrance, and Y. S. Wu.
1987.
Interaction of -agglutinin with Saccharomyces cerevisiae a cells.
J. Bacteriol.
169:483-488 |
| 31. |
Lu, C. F.,
J. Kurjan, and P. N. Lipke.
1994.
A pathway for cell wall anchorage of Saccharomyces cerevisiae -agglutinin.
Mol. Cell. Biol.
14:4825-4833 |
| 32. |
Lu, C. F.,
R. C. Montijn,
J. L. Brown,
F. Klis,
J. Kurjan,
H. Bussey, and P. N. Lipke.
1995.
Glycosyl phosphatidylinositol-dependent cross-linking of alpha-agglutinin and beta 1,6-glucan in the Saccharomyces cerevisiae cell wall.
J. Cell Biol.
128:333-340 |
| 33. | Malmqvist, M., and R. Karlsson. 1997. Biomolecular interaction analysis: affinity biosensor technologies for functional analysis of proteins. Curr. Opin. Chem. Biol. 1:378-383[CrossRef][Medline]. |
| 34. |
Rini, J. M.,
U. Schulze-Gahmen, and I. A. Wilson.
1992.
Structural evidence for induced fit as a mechanism for antibody-antigen recognition.
Science
255:959-965 |
| 35. |
Roy, A.,
C. F. Lu,
D. L. Marykwas,
P. N. Lipke, and J. Kurjan.
1991.
The AGA1 product is involved in cell surface attachment of the Saccharomyces cerevisiae cell adhesion glycoprotein a-agglutinin.
Mol. Cell. Biol.
11:4196-4206 |
| 35a. | Shen, Z. M., L. Wang, H. Zhao, J. Kurjan, J. Pike, and P. N. Lipke. Delineation of functional regions within the subunits of the Saccharomyces cerevisiae cell adhesion molecule a-agglutinin. J. Biol. Chem., in press. |
| 36. | Sreerama, N., and R. W. Woody. 1994. Protein secondary structure from circular dichroism spectroscopy. Combining variable selection principle and cluster analysis with neural network, ridge regression and self-consistent methods. J. Mol. Biol. 242:497-507[Medline]. |
| 37. | Sreerama, N., and R. W. Woody. 1993. A self-consistent method for the analysis of protein secondary structure from circular dichroism. Anal. Biochem. 209:32-44[CrossRef][Medline]. |
| 38. | Terrance, K. 1983. Ph.D. dissertation. City University of New York, New York, N.Y. |
| 39. |
Terrance, K.,
P. Heller,
Y. S. Wu, and P. N. Lipke.
1987.
Identification of glycoprotein components of -agglutinin, a cell adhesion protein from Saccharomyces cerevisiae.
J. Bacteriol.
169:475-482 |
| 40. |
Terrance, K., and P. N. Lipke.
1987.
Pheromone induction of agglutination in Saccharomyces cerevisiae a cells.
J. Bacteriol.
169:4811-4815 |
| 41. |
Terrance, K., and P. N. Lipke.
1981.
Sexual agglutination in Saccharomyces cerevisiae.
J. Bacteriol.
148:889-896 |
| 42. |
Wojciechowicz, D.,
C. F. Lu,
J. Kurjan, and P. N. Lipke.
1993.
Cell surface anchorage and ligand-binding domains of the Saccharomyces cerevisiae cell adhesion protein -agglutinin, a member of the immunoglobulin superfamily.
Mol. Cell. Biol.
13:2554-2563 |
| 43. | Yamaguchi, M., K. Yoshida, and N. Yanagishima. 1982. Isolation and partial characterization of cytoplasmic alpha agglutination substance in the yeast Saccharomyces cerevisiae. FEBS Lett. 139:125-129[CrossRef][Medline]. |
| 44. |
Yurchenco, P. D., and Y. S. Cheng.
1993.
Self-assembly and calcium-binding sites in laminin. A three-arm interaction model.
J. Biol. Chem.
268:17286-17299 |
| 45. | Zhao, H. 1999. Ph.D. dissertation. City University of New York, New York, N.Y. |
| 46. | Zhao, H., M. H. Chen, Z.-M. Shen, P. C. Kahn, and P. N. Lipke. Environmentally-induced conformational switching in the
yeast cell adhesion protein, -agglutinin. Protein Sci., in press.
|
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