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J. Biol. Chem., Vol. 277, Issue 1, 155-160, January 4, 2002
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From the Department of Biochemistry, Tulane University Health
Sciences Center, New Orleans, Louisiana 70112-2699
Received for publication, August 9, 2001, and in revised form, October 9, 2001
Antigen three-dimensional structure potentially
limits antigen processing and presentation to helper T-cell epitopes.
The association of helper T-cell epitopes with the mobile loop in Hsp10s from mycobacteria and bacteriophage T4 suggests that the mobile
loop facilitates proteolytic processing and presentation of adjacent
sequences. Sites of initial proteolytic cleavage were mapped in
divergent Hsp10s after treatment with a variety of proteases including
cathepsin S. Each protease preferentially cleaved the Hsp10s in the
mobile loop. Flexibility in the 22-residue mobile loop most probably
allows it to conform to protease active sites. Three variants of the
bacteriophage T4 Hsp10 were constructed with deletions in the mobile
loop to test the hypothesis that shorter loops would be less sensitive
to proteolysis. The two largest deletions effectively inhibited
proteolysis by several proteases. Circular dichroism spectra and
chemical cross-linking of the deletion variants indicate that the
secondary and quaternary structures of the variants are native-like,
and all three variants were more thermostable than the wild-type Hsp10.
Local structural flexibility appears to be a general requirement for
proteolytic sensitivity, and thus, it could be an important factor in
antigen processing and helper T-cell epitope immunogenicity.
Numerous studies indicate that the context of a T-helper epitope
influences its immunogenicity (1-6). Cryptic epitopes can be shielded
from presentation by various mechanisms that ultimately interfere with
binding of peptides to the class II
MHC1 protein (7) or transport
of the complex to the cell surface (8). Antigen processing contributes
directly to these mechanisms by removing or failing to remove antigen
sequences that influence presentation of the epitope. Studies testing
the role of proteases in knock-out mice have been complicated by the
requirement for proteolytic maturation of the class II MHC protein.
Nevertheless, antigen presentation is altered when cathepsin S or
cathepsin L deficiency is combined with invariant chain deficiency (9). Thus, the pathway of proteolytic degradation can influence antigen presentation.
Early studies suggested that antigen primary sequence affected antigen
processing at the level of recognition and binding by a protease (1,
10). More recently, the effect of cleavage site primary sequence on
immunogenicity was demonstrated. The creation of a dibasic cleavage
site for a prohormone processing enzyme enhanced the presentation of a
flanking epitope in hen egg lysozyme (11), and disruption of a cleavage
site for asparaginyl endopeptidase interfered with presentation of the
tetanus toxoid antigen (12).
However, other reports have suggested that three-dimensional structure
modulates antigen processing. Stabilization by intramolecular cross-links inhibited presentation of an epitope of hen egg lysozyme (13). An acid-induced structural change enhanced presentation of an
epitope of influenza hemagglutinin (3). Unfolding prior to processing
disrupted presentation of an immunodominant epitope of mouse
immunoglobulin (2).
The distribution of local disorder in the antigen could modulate
antigen processing. It is well established that proteases tend to
cleave between domains in multi-domain proteins and at other
locally disordered sites. Even in a single-domain protein, proteolytically sensitive sites tend to occur in segments characterized by high crystallographic B-factors (14). The conformation of the
polypeptide around the incipient cleavage site must be easily distorted
to accommodate binding to the protease (15, 16). To our knowledge, no
ATP-dependent protein unfolding activity (other than
acidification) has been described for the lysosome. The pH of the
antigen-processing compartment probably depends on the cell type and
degree of activation (17). Nevertheless, most proteins retain
native-like three-dimensional structure in acidic environments as low
as pH 2 in many cases (18).
Analyses of published structural data and epitope maps for several
model antigens have suggested that local structural disorder increases
immunogenicity in the adjacent sequences (19, 20). Here, we have
tested this hypothesis by analyzing the structure and immunology
of bacteriophage T4 Hsp10 (T4Hsp10). As in all Hsp10s, T4Hsp10 has a
flexibly disordered Hsp60-binding mobile loop (21) that we suspected
would favor presentation of flanking sequences to helper T-cells.
T4Hsp10 is homologous to bacterial and mammalian Hsp10s by comparison
of the respective three-dimensional structures, although it exhibits
less than 20% sequence identity with any of these Hsp10s (22). The
mobile loops of Escherichia coli Hsp10 (GroES) and T4Hsp10
contain preferred sites for cleavage by trypsin and protease K,
respectively (20, 23). Earlier studies have mapped helper T-cell
epitopes to sequences flanking the mobile loop of Mycobacterium
leprae Hsp10 in infected humans and immunized mice (24-26). In a
companion paper (27), we confirm the presence of an
immunodominant epitope adjacent to the mobile loop in T4Hsp10.
Here, we examined the potential for three-dimensional structure to
influence processing and presentation by analyzing the proteolytic
sensitivity of the mobile loop in Hsp10s. We find that treatment of
diverse Hsp10s with a variety of proteases consistently yields products
of initial cleavage in the mobile loop, suggesting that antigen
processing by lysosomal proteases would initiate with cleavage in the
mobile loop. Variants of T4Hsp10 containing deletions in the
mobile loop were constructed in order to probe the changes in protease
sensitivity and immune responses. Our results suggest that loop
deletion can reduce proteolytic sensitivity without gross disruption of
antigen three-dimensional structure. In a companion paper (27) we show
that reduced proteolytic sensitivity correlates with reduced helper
T-cell and antibody epitope immunodominance.
Proteins and Peptides--
Deletions in the T4Hsp10 coding
sequence of plasmid pAlex (a kind gift of A. Richardson, University of
Geneva, Switzerland) were introduced using the Stratagene
site-directed mutagenesis kit. DNA sequencing confirmed the native
sequence of each construct, with the exception of the intended
mutation. Protein purification was executed as previously described for
T4Hsp10 (28), except that the Superdex-200 gel-filtration step was
substituted with hydroxyapatite chromatography employing a 20-300
mM gradient of sodium phosphate, pH 6.8.
Limited Proteolysis--
All reactions were carried out in a
total volume of 50 µl and contained 100 µM T4Hsp10,
T4Hsp10dLIG, T4Hsp10d8, or T4Hsp10d8C (subunits) except where otherwise
noted. All enzymes were from Sigma and of the highest grade available.
Reactions with trypsin containing 10 mM Tris-HCl, pH 7.5, and 5 µg/ml protease proceeded for 30 min on ice and then were
terminated by the addition of phenylmethylsulfonyl fluoride to
20 µM. Reactions with protease V8 containing 50 mM sodium phosphate, pH 7.5, 1 µM
dithiothreitol, and 25 µg/ml protease proceeded for 30 min at room
temperature and then were terminated by the addition of Nonidet P-40 to
1.5%. Reactions with cathepsin S (kind gift of M. McGrath, Axys
Pharmaceuticals, Inc.) in a total volume of 65 µl containing 50 mM Tris-HCL, pH 7.5, 192 mM KCl, 1 µM dithiothreitol, and 0.8 µg/ml protease proceeded for
30 min at room temperature and then were terminated by the addition of
E-64 (Sigma) to 10 µM. Reactions with protease K
containing 50 µM target protein, 40 mM
Tris-HCl, pH 7.5, 192 mM KCl, 1 µM dithiothreitol, and 25 µg/ml protease proceeded for 15 min on ice and
then were terminated by the addition of phenylmethylsulfonyl fluoride
to 20 µM. Reactions with papain containing 10 mM MES-KOH (pH 5.7), 4 mM Mass Spectrometry--
For mapping cleavage sites in E. coli and human Hsp10s, 0.5 µl of the reaction was analyzed using
a Thermofinnigan Lasermat matrix-assisted laser desorption
time-of-flight (MALDI-TOF) mass spectrometer (Tulane Coordinated
Instrumentation Facility) and Circular Dichroism Spectroscopy--
Far-UV circular dichroism
(CD) spectra were recorded on an OLIS spectropolarimeter using a cell
with path length 1 mm. Samples contained 25 µM protein
(subunits) in 10 mM sodium phosphate, pH 6.8, at 25 °C.
The wavelength was scanned in triplicate between 300 and 188.2 nm using
110 points, and the spectra were averaged. A similarly recorded
background spectrum was subtracted from the sample spectrum to obtain
the protein spectrum. Melting curves monitored by CD were obtained by
recording the CD at 205 and 206 nm at 2° intervals over the range of
22 to 84 °C and then averaging the values at the two wavelengths for
each temperature (reported as Glutaraldehyde Cross-linking--
Reactions were initiated by
addition of 25% glutaraldehyde to achieve a final concentration of 2%
(w/v) in 100 µl of 5 mM sodium phosphate buffer, pH 6.8, and 100 µM T4Hsp10, T4Hsp10dLIG, T4Hsp10d8, or
T4Hsp10d8C. After 2, 10, or 20 min at room temperature, reactions were
quenched by the addition of sodium borohydride to a final concentration
of 400 mM. After 20 min, proteins were precipitated at room
temperature with 10% trichloroacetic acid in the presence of 100 mM NaCl, collected by centrifugation at 15,000 × g, combined with NuPAGE LDS sample buffer
(Invitrogen), run on a NuPAGE bis-Tris 4-20% polyacrylamide gel with
NuPAGE MES buffer (Invitrogen), and stained with Coomassie Blue.
Preferred Cleavage Sites in the Mobile Loop
The proteolytic sensitivity of diverse Hsp10 proteins was probed
with several serine and cysteine proteases including cathepsin S. Cysteine proteases constitute the bulk of the lysosomal proteases, and
cathepsin S has been implicated in antigen processing (9). A strong
preference for cleavage in the mobile loop should dominate the cleavage
site selectivity regardless of Hsp10 sequence or protease specificity.
Such a highly preferred site most likely would be the site of first
cleavage by the mixture of proteases in the lysosome. For each
combination of Hsp10 and protease, experimental conditions were
optimized for the accumulation of products resulting from an initial
endoproteolytic cleavage, as judged by the resolution of one or more
large fragments in SDS-PAGE.
For each protease and Hsp10, one or more abundant fragments were
observed at ~3000 and 7000 Da by mass spectrometry (Table I). Cleavage sites (Fig.
1) were identified by the presence of both N- and C-terminal fragments corresponding to the masses predicted from the Hsp10 sequence (±21 Da). There were several examples of
alternative cleavage sites in human Hsp10 for a single protease. A
secondary site was evident as a less abundant pair of large and small
fragments. It was clear that each fragment was derived from cleavage of
the full-length protein for the following two reasons. First, the
difference in mass between large fragments was equal to the difference
in mass between small fragments; and second, the difference was equal
to the mass of residues between the alternative sites, e.g.
Gly28-Met31 in the cathepsin S
digestion of human Hsp10. Initial cleavage sites in T4Hsp10 could not
be determined from the mass spectrometry data. Although fragments
clustered near 3000 and 7000, the sum of the masses for predominant
fragments was less than the total mass of T4Hsp10. Presumably, the
initial cleavage products were rapidly converted to smaller
fragments.
Deletions in the Mobile Loop Stabilize T4Hsp10 and Inhibit
Proteolysis
Deletion Design--
Deletion variants of T4Hsp10 were constructed
to test the relationship of mobile loop size and flexibility to
proteolytic sensitivity (Fig. 2). We
reasoned that a shorter loop would have less flexibility to adopt the
conformation necessary for binding to a protease. The 3-residue
deletion in T4Hsp10dLIG was designed to shorten the loop and stabilize
a nascent hairpin turn in the center of the loop (21) by removing a
glycine and by placing an isoleucine opposite threonine 31 on
the other Purification and Secondary Structure--
The biophysical
properties of the deletion variants were similar to those of wild-type
T4Hsp10. Each variant accumulated in the soluble phase of E. coli cells at high levels and was purified using the protocol
developed for T4Hsp10. T4Hsp10 and the three variants eluted from
Q-Sepharose at the same position in the gradient, but the variants
eluted from hydroxyapatite at elevated sodium phosphate concentrations.
Whereas T4Hsp10 eluted at 65 mM, T4Hsp10dLIG eluted at 70 mM, T4Hsp10d8 at 120 mM, and T4Hsp10d8C at 150 mM. The far-UV CD spectra of T4Hsp10 and the deletion
variants were similar, as expected for retention of the native, mostly
Thermal Stability--
The thermal stability of T4Hsp10 and the
deletion variants was evaluated by monitoring the CD at 205.5 nm over
the temperature range of 22 to 84 °C. Thermal denaturation of all
four proteins was evident as a cooperative transition in the CD
intensity (Fig. 3B). Spectra recorded after the transition
exhibited strong minima near 200 nm (data not shown), which is expected
if a substantial portion of the denatured proteins behaves as a random
coil (32). The deletion variants melted at temperatures ranging from 3 to 7 °C higher than T4Hsp10.
Cross-linking with Glutaraldehyde--
The quaternary structures
of T4Hsp10 and the deletion variants were analyzed by chemical
cross-linking. Treatment of T4Hsp10 with glutaraldehyde generated a
ladder of six polypeptides with slower electrophoretic mobility in
SDS-PAGE (Fig. 4). Because T4Hsp10 is
known to form a heptamer (22), we assigned the six bands to dimer
through heptamer. The bands were less intense with increasing molecular
weights up to hexamer and heptamer, which were more intense than
pentamer. A longer incubation with the cross-linker increased
the intensity of the hexamer and heptamer at the expense of lower
molecular weight bands, but no discrete bands above heptamer were
formed. Thus, we concluded that the cross-linking reaction with T4Hsp10
is essentially complete upon formation of the heptamer.
Each deletion variant formed a ladder of cross-linked polypeptides that
was similar to that formed by T4Hsp10. As for T4Hsp10, a longer
incubation with the cross-linker increased the amount of heptamer but
not higher order multimers. The cross-linked samples of T4Hsp10d8 also
produced a diffuse band near and above the molecular weight of
heptamer. This material probably is the result of multiple intersubunit
and/or intrasubunit cross-links (33, 34), which are somehow more likely
in the modified mobile loop. Nevertheless, among the discrete
cross-linked species after the 10-min incubation, the heptamer was the
most abundant. The heptamer species of T4Hsp10d8C was poorly
represented among the cross-linked species. This variant may have been
resistant to cross-linking because the mobile loop was less flexible.
At longer incubation times, more of the T4Hsp10d8C accumulated in the
tetramer and pentamer forms, suggesting that an oligomer of that size
or larger predominated. Because the cross-linked species discontinued
above the level of heptamer, we concluded that T4Hsp10d8C also existed
predominantly as the heptamer.
Limited Proteolysis--
Differences between T4Hsp10 and the
deletion variants in proteolytic sensitivity were largely independent
of the choice of protease (Fig. 5).
Sensitivity of T4Hsp10dLIG was similar to that of T4Hsp10 except for
slight decreases in sensitivity to trypsin (30%) and protease V8
(20%). T4Hsp10d8 was much less sensitive than T4Hsp10 to trypsin
(6-fold) and cathepsin S (6-fold) but only slightly less sensitive to
protease K (10%) and protease V8 (20%). T4Hsp10d8C was much less
sensitive than T4Hsp10 to all four proteases (protease K, 4-fold;
trypsin, 5-fold; protease V8, 36-fold; and cathepsin S, 14-fold).
Earlier work comparing helper T-cell epitope maps to structural
data indicated that helper T-cell epitopes were frequently associated
with adjacent unstable loops. We hypothesized that unstable loops
promote presentation of adjacent sequences by virtue of their
sensitivity to endoproteolytic processing in antigen presenting cells.
For the present work, Hsp10 was selected for an examination of the
relationship of structure and proteolytic sensitivity because helper
T-cell epitopes have been found adjacent to the mobile loop (24-27),
and the mobile loop provides a natural target for initial
endoproteolytic cleavage during antigen processing.
Results from mapping the sites of initial cleavage in E. coli and human Hsp10s demonstrate the exceptional proteolytic
sensitivity of the mobile loop. When combined with the earlier studies
on E. coli and bacteriophage T4 Hsp10s, we find that four
proteases cleave three divergent Hsp10s within a 12-residue segment of
the 22-residue mobile loop. The shared preference of the proteases for
this segment cannot be attributed to a coincidence of required primary
sequences. The proteases exhibit little sequence specificity (35).
Trypsin requires a positively charged residue (Lys/Arg) in P1,
but the 13 Lys/Arg in E. coli Hsp10 and the 15 Lys/Arg in
human Hsp10 are evenly distributed in the sequences. The other proteases are less specific. Proteinase K prefers aromatic and hydrophobic residues in P1. Papain prefers bulky hydrophobic residues in P2 and slightly prefers Lys/Arg in P1. Cathepsin S prefers branched
hydrophobic residues in P2. Local structural disorder in the mobile
loop probably is the most important factor determining the initial
cleavage site. Local disorder is typical of protein segments that are
easily distorted into a conformation suitable for binding to the
protease active site (15).
Preferential cleavage in the mobile loop can be explained by the loop
being larger and more flexible than other potentially protease-sensitive sites in the Hsp10s (Fig.
6). The roof
Proteolytic Sensitivity and Helper T-cell Epitope Immunodominance
Associated with the Mobile Loop in Hsp10s*
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
INTRODUCTION
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
MATERIALS AND METHODS
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
-mercaptoethanol,
and 20 µg/ml protease proceeded for 60 min at room temperature and
then were terminated by the addition of E-64 to 5 µM. An
aliquot of each reaction was mixed with SDS-containing sample buffer,
resolved by SDS-PAGE using the Tris/Tricine buffer system (29), and
stained with Coomassie Blue. Quantification of the remaining intact
protein was by integration of the band in the image of the stained gel
captured by an AlphaImager 2200 (Alpha Innotech).
-cyano-3-hydroxycinnamic acid as the
matrix. Mass determinations were calibrated with substance P
((M + H)+, 1349 Da), which was co-deposited on the target
prior to analysis. Fragment mass predictions were generated with
PeptideMass2 using Swiss-Prot
sequence entries CH10ECOLI or CH10HUMAN.
205.5). The data for each
protein were fit by nonlinear regression (GraphPad Prism) to the
equation
![y={(y<SUB><UP>f</UP></SUB>+m<SUB><UP>f</UP></SUB> · [T])+(y<SUB><UP>u</UP></SUB>+m<SUB><UP>u</UP></SUB> · [T])·<UP>exp</UP>[(&Dgr;H<SUB><UP>m</UP></SUB>/RT)](/content/vol277/issue1/fulltext/155/img001.gif)
![·((T−T<SUB><UP>m</UP></SUB>)/T<SUB><UP>m</UP></SUB>)]}/(1+<UP>exp</UP>[(&Dgr;H<SUB><UP>m</UP></SUB>/RT)](/content/vol277/issue1/fulltext/155/img002.gif)
(Eq. 1)
where y represents the observed CD signal,
yf and yu are the
intercepts, and mf and mu
the slopes of the pre- and posttransition base lines, T is
the temperature, Tm is the midpoint of the
thermal unfolding curve, and
![·((T−T<SUB><UP>m</UP></SUB>)/T<SUB><UP>m</UP></SUB>)])](/content/vol277/issue1/fulltext/155/img003.gif)
Hm is the
enthalpy change for unfolding at Tm (30).
Thermal unfolding was found not to be reversible, and thus
Hm cannot be taken as the enthalpy for
equilibrium unfolding of the protein. Nevertheless,
Tm gives an indication of protein stability
against thermal denaturation.
RESULTS
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
Products of Hsp10 limited proteolysis assigned by mass spectrometry
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Fig. 1.
Alignment of Hsp10 sequences indicating
structural features and preferred sites for endoproteolytic cleavage
(T, trypsin; P, papain;
CS, cathepsin S; PK, protease
K). The immunodominant helper T-cell epitopes of M. leprae Hsp10 in humans and of T4Hsp10 in mice are from Refs. 24
and 27, respectively. Locations of -strands
(arrows) and or 310 helices (coils) are
indicated below the sequence of T4Hsp10. Nascent elements of
secondary structure are indicated with dashed lines.
Residues deleted in the T4Hsp10 variants are indicated with
"X". Data for trypsin cleavage of E. coli
Hsp10 and protease K digestion of T4 Hsp10 were from Refs. 23 and 21,
respectively.
-strand (31). The 8-residue deletion in T4Hsp10d8
symmetrically removed from T4Hsp10dLIG four residues in each strand of
the nascent hairpin. The 8-residue deletion in T4Hsp10d8C removed from
T4Hsp10dLIG a segment that forms an helix in the T4Hsp10 crystal
lattice but that is essentially disordered in solution (21). The
deletions affect sequences only within the mobile loop and thus were
not expected to disturb the ordered part of the native structure.
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Fig. 2.
Ribbon diagrams of a single subunit of
T4Hsp10 indicating residues deleted in the mobile loop deletion
variants. The mobile loop
(Gln24-Val45) plus two residues on each
flank are indicated in single-letter code. In the construction of
T4Hsp10dLIG, the removal of Leu35 and Ile36
(circled) repositions Ile37 opposite
Thr31 in the nascent hairpin, which can provide a
stabilizing interaction (31); and removal of Gly38
(circled) reduces flexibility. In the construction of
T4Hsp10d8, four residues (circled) are deleted from each
flank of the nascent hairpin in T4Hsp10dLIG. In the construction of
T4Hsp10d8C, eight residues (broken circle) are
deleted from the C-terminal flank of the nascent hairpin in
T4Hsp10dLIG. T4Hsp10d8C lacks the entire segment comprising a small
helix that was stabilized by the crystal lattice (22).
-sheet secondary structure (Fig.
3A). However, in the spectrum
of T4Hsp10d8C, the intensity of the band at 198 nm was more positive,
which is consistent with a larger fraction of -sheet (32).
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Fig. 3.
CD spectra (A) and thermal
denaturation curves (B) for T4Hsp10 and mobile loop
deletion variants. The similar spectra indicate similar secondary
structure content in the four proteins, although the more positive band
at 198 nm reports a slightly larger -sheet content for T4Hsp10d8C.
For all four proteins, heat denaturation monitored by CD at 205.5 nm
exhibits a cooperative transition. All three variants are more
thermostable than T4Hsp10. The Tm values were as
follows (in °C): T4Hsp10, 56.0; T4Hsp10dLIG, 59.5; T4Hsp10d8, 58.5;
and T4Hsp10d8C, 63.3.
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Fig. 4.
Oligomeric structure of T4Hsp10 and mobile
loop deletion variants. Treatment of T4Hsp10 with
glutaraldehyde produced a ladder of six cross-linked species
corresponding to dimer through heptamer (identified by
arrows labeled 2-7). Increasing the time of
incubation with cross-linker increased the amount of heptamer and
decreased the amount of smaller species but did not result in the
formation of discrete species larger than a heptamer.
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Fig. 5.
Proteolytic sensitivity of T4Hsp10 and mobile
loop deletion variants. A, reaction conditions
with T4Hsp10 were optimized for accumulation of large fragments
(Large frags.) detected by SDS-PAGE, and then the
same conditions were employed with the deletion variants. B,
quantification of intact protein following limited proteolysis.
Proteases designations are the same as in the legend for Fig. 1;
V8, protease V8. T4Hsp10 variants are designated by the
suffix identifying the deletion (dLIG for T4Hsp10dLIG,
etc.). Proteolytic sensitivity was defined in terms of the fraction
degraded in the illustrated reactions. The fraction degraded was taken
as the fraction intact subtracted from unity. The intact fraction was
measured as the integrated intensity of the intact band in the treated
lane divided by the integrated intensity of the intact band in the
mock-treated control lane. T4Hsp10dLIG was only slightly less sensitive
than T4Hsp10 to trypsin and protease V8. In contrast, T4Hsp10d8 was six
times less sensitive to trypsin, and cathepsin S. T4Hsp10d8C was at
least four times less sensitive to any of the four proteases.
DISCUSSION
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
-hairpin of E. coli Hsp10 was predicted to be metastable on the basis of its high
B-factors and minimal tertiary structural contacts (36). Likewise, the
roof -hairpin of human Hsp10 has enough segmental disorder to give
resolvable NMR resonances, and the roof -hairpin was not
observed in the crystal structure (37). Although highly flexible, the
roof -hairpin may be too small to accommodate the deformation
required for binding to a protease. A segment of only seven residues in
E. coli Hsp10 has B-factors that exceed the average value,
and only four residues of human Hsp10 were observed by NMR. Hubbard and
Thornton propose that 12 residues are necessary for efficient cleavage
by trypsin (16). The peripheral loop of T4Hsp10 has 12 residues with
above average B-factors, but resonances for the peripheral loop were
not observed in our previous NMR study, indicating that it is not as
flexible as the mobile loop. Thus, the peripheral loop is eight
residues shorter than the mobile loop and much less flexible, which
explains the preferential cleavage in the mobile loop.
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Fig. 6.
Ribbon diagram of T4Hsp10
(A) and plot of crystallographic B-factors for
backbone amide nitrogen atoms in a single subunit of T4Hsp10
(B). Preferred sites of proteolytic cleavage by
protease K are illustrated. Crystallographic data were from Protein
Data Bank code 1G31, and the ribbon diagram was prepared using
Molscript (39). Ribbon segments corresponding to the immunodominant
T-helper sequence (27) are filled in black. In
panel B, the horizontal dashed line indicates the
average B-factor value (55 Å), and the horizontal bar
indicates the extent of the mobile loop defined by NMR (21). The
C-terminal portion of the mobile loop, including a short helix,
mediates crystal lattice contacts with another molecule of T4Hsp10
(22); and thus B-factors do not reflect the full extent and flexibility
of the mobile loop in solution. The mobile loop and two additional
loops have higher than average B-factors, but only the mobile loop
contains preferred cleavage sites for a variety of proteases in diverse
Hsp10s. The roof -hairpin and peripheral loop may not contain
preferred cleavage sites because they are smaller and less
flexible.
The structure of an Hsp10 in the antigen-processing compartment should be similar to the structures previously described by x-ray crystallography and NMR. Antigen processing is believed to occur in acidic conditions in or near the lysosome. Much of the structural information about E. coli and human Hsp10s was gathered in acidic conditions, and the structure is essentially unchanged over a wide range of pH. Crystals of E. coli Hsp10 were grown at pH 5.5 (36), and NMR studies on mobile loop conformation and dynamics were carried out at pH levels ranging from 4.0 to 7.0 (23, 38). Likewise, crystals of human Hsp10 were grown at pH 3.5,3 and NMR studies were performed from pH 3.5 to 6.8 (37). In all cases, the extent and behavior of the flexible segments were essentially identical. Thus, a highly protease-sensitive region created by local disorder in the Hsp10 structure should be the target of initial endoproteolytic cleavage in vitro and in vivo.
Three mobile loop deletion variants of T4Hsp10 were constructed to test
the hypothesis that reductions in loop size and flexibility inhibit
proteolytic cleavage. Low-resolution structural analysis suggests that
the consequences of the deletions were restricted to the mobile loop.
The behavior of the variants during purification was similar to that of
T4Hsp10. The circular dichroism spectra of the variants suggest that
their secondary structure content is similar to that of T4Hsp10.
T4Hsp10d8C had a slightly larger -sheet content, but this
could be confined to the mobile loop. Thermal denaturation curves for
the variants exhibited highly cooperative transitions, indicating that
the proteins have well organized, probably native-like structure. The
transition midpoints for all three variants were at elevated
temperatures relative to T4Hsp10, as predicted for stabilized structure
in the mobile loop. Finally, the results from chemical cross-linking
suggest that the variants assume the native heptameric quaternary structure.
The mobile loop deletions reduced proteolytic sensitivity according to
expected changes in loop structure and flexibility. The deletions were
designed to shrink the loop and simultaneously stabilize a nascent
-hairpin conformation. The added conformational restraints should
increase the energetic cost of substrate binding to the protease. The
three-residue deletion was designed to stabilize the nascent hairpin
without substantially shortening the loop. Hubbard et al.
(16) found that trypsin requires the deformation of at least 10 residues of the substrate around the cleavage site, and the deformation
is much easier in a loop of 12 residues or more. Because the mobile
loop of T4Hsp10 spans the 22-residue sequence from Gln24 to
Val45, removal of three residues should not severely affect
the ability of the loop to be deformed. In T4Hsp10dLIG, sensitivity to
protease K and cathepsin S is unaffected, and sensitivity to trypsin
and protease V8 is only slightly reduced. In contrast, removal
of 11 residues from the loop shrinks it to a borderline size for the
deformation required by trypsin. Accordingly, T4Hsp10d8 and T4Hsp10d8C
become much more resistant to trypsin and cathepsin S by comparison to
T4Hsp10 and T4Hsp10dLIG.
The structure of the remaining loop segment also may influence
proteolytic sensitivity. The deletion in T4Hsp10d8 leaves a segment of
nascent helix intact, whereas the deletion in T4Hsp10d8C completely
removes the helix. The tendency for the loop in T4Hsp10d8 (as well as
T4Hsp10 and T4Hsp10dLIG) to explore alternative structures may make it
more probable that the loop will adopt a conformation acceptable to the
protease. In contrast, exclusive formation of -sheet in the loop of
T4Hsp10d8C would strongly disfavor proteolysis. Thus, differences in
loop structure could account for the greater sensitivity of
T4Hsp10d8 than T4Hsp10d8C to cleavage by proteinase K and protease V8.
The results presented here establish the broad sensitivity to
proteolysis of Hsp10 mobile loops, and they support the theory that
local disorder promotes presentation to helper T cells of the adjacent
sequence by providing sites for proteolytic cleavage. Mobile loop
deletions reduce proteolytic sensitivity to varying degrees, and the
structural changes appear to be localized to the mobile loop. Thus,
loop deletion provides a simple strategy for modifying epitope immunodominance.
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ACKNOWLEDGEMENTS |
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We are grateful to P. Wittung-Stafshede and J. Guidry for access to the CD spectropolarimeter and assistance with glutaraldehyde cross-linking and to the New Orleans Protein Folding Intergroup for critical discussion.
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FOOTNOTES |
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* This work was supported by National Institutes of Health Grant R01-AI42350.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.
To whom correspondence should be addressed: Dept. of Biochemistry,
Tulane University Health Sciences Center, 1430 Tulane Ave., New
Orleans, LA 70112-2699. Tel.: 504-586-3990; Fax: 504-584-2739; E-mail: landry@tulane.edu.
Published, JBC Papers in Press, October 22, 2001, DOI 10.1074/jbc.M107624200
2 Found on the Internet at www.expasy.ch.
3 J. F. Hunt, B. J. Scott, L. Henry, J. Guidry, S. J. Landry, and J. Deisenhofer, unpublished results.
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ABBREVIATIONS |
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The abbreviations used are: MHC, major histocompatibility complex; Hsp, heat shock protein; T4Hsp10, bacteriophage T4 Hsp10; MES, 4-morpholineethanesulfonic acid; E-64, trans-epoxysuccinyl-L-leucylamido-(4-guanidino)butane.
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REFERENCES |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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