By
From the Department of Cancer Immunology and AIDS, Dana-Farber Cancer Institute, Boston, Massachusetts 02115
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Abstract |
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MHC class II molecules and invariant chain assemble at a neutral pH in the endoplasmic reticulum and are transported to a low pH compartment where the invariant chain is trimmed to the class II-associated invariant chain peptide (CLIP). For many major histocompatibility complex class II molecules, DM is required for rapid removal of CLIP, which allows binding of antigenic peptides. Since I-Ag7 confers susceptibility to type I diabetes in NOD mice, the biochemical requirements for peptide loading were examined using soluble I-Ag7 expressed in insect cells. I-Ag7 formed long-lived complexes with naturally processed peptides from transferrin and albumin, whereas several peptides that represent T cell epitopes of islet autoantigens were poor binders. I-Ag7-peptide complexes were not sodium dodecyl sulfate (SDS) resistant, indicating that SDS sensitivity may be an intrinsic property of I-Ag7. Complexes of I-Ag7 and CLIP formed at a neutral pH, but rapidly dissociated at pH 5. This rapid dissociation was due to a poor fit of M98 of CLIP in the P9 pocket of I-Ag7, since substitution of M98 by a negatively charged residue greatly enhanced the stability of the complex. These biochemical properties of I-Ag7 result in the rapid generation of empty molecules at an endosomal pH and have a global effect on peptide binding by I-Ag7.
Key words: major histocompatibility complex; autoimmunity; antigen presentation; I-Ag7; type I diabetes ![]() |
Introduction |
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Genome-wide analyses in families with type I diabetes
and in nonobese diabetic (NOD)1 mice demonstrated
that multiple genes contribute to susceptibility and that the
MHC is an important susceptibility locus (1). In humans,
susceptibility is associated with the MHC class II region, in
particular with the DR4/DQ8 and DR3/DQ2 haplotypes. The risk for the development of type I diabetes is particularly high in subjects who carry both the DR4/DQ8 and
DR3/DQ2 haplotype or who are homozygous for either
haplotype (1, 6). It is generally thought that the DQ molecules (DQ8 and DQ2) are involved in the disease process,
but particular DR4 alleles also contribute to susceptibility
(for review see reference 7). Both DQ8 and DQ2 are characterized by the absence of aspartic acid at 57 (alanine in
both alleles). The DR2/DQ6 haplotype (DQB1*0602)
confers dominant protection from the disease.
Two features characterize the MHC class II region of
NOD mice. NOD mice express only I-Ag7 but not I-E
molecules, due to a deletion in the E promoter. This lack
of I-E expression is important since transgenic expression of I-E or other I-A molecules protects from spontaneous
disease (5, 8). The I-A molecule of NOD mice, I-Ag7,
has the same
chain as I-Ad but a unique
chain sequence.
The most striking characteristic of the I-Ag7
chain is the
presence of histidine and serine at
56 and
57, instead of
proline and aspartic acid as in other murine I-A alleles (12).
Crystallographic studies of human and murine MHC class II molecules demonstrated that
57 is located in the P9
pocket of the peptide binding site. In most MHC class II
molecules,
57 forms a salt bridge with
76, which is missing in I-Ag7 (13).
It has recently been proposed that I-Ag7 molecules are poor peptide binders. This hypothesis is based on the observation that only a small fraction of immunoprecipitated I-Ag7 molecules are SDS resistant. Also, binding experiments with affinity-purified, detergent-solubilized I-Ag7 molecules demonstrated little or no binding of peptides in that study (17). To examine the biochemical properties of I-Ag7 in the absence of detergent, we expressed I-Ag7 as a soluble protein in Drosophila Schneider cells. I-Ag7 formed long-lived complexes with naturally processed peptides from transferrin and serum albumin, while several peptides that represent T cell epitopes of islet antigens were poor binders. I-Ag7 formed a complex with the class II-associated invariant chain peptide (CLIP) at a neutral pH, but these complexes rapidly dissociated at pH 5. These biochemical properties of I-Ag7 result in the rapid generation of empty molecules at the pH of the peptide loading compartment and have a global effect on peptide binding by this MHC class II molecule.
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Materials and Methods |
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Synthetic Peptides.
Peptides were synthesized by Quality Controlled Biochemicals, Inc. and subjected to quality control by reverse-phase HPLC and mass spectrometry.cDNA Constructs.
cDNA constructs were made by reverse transcriptase PCR using RNA from NOD spleens. Fos and Jun dimerization domains were attached to the 3' end of the I-Ag7Transfection of Drosophila Schneider Cells.
Drosophila melanogaster S2 cells (4 × 106) were transfected with 20 µg of each plasmid, 0.5 µg of hygromycin selection vector pUC-hygMT, and 20 µl of liposomes (Invitrogen) in 1 ml medium without FCS for 4 h. After transfection, cells were grown in Schneider medium (Sigma Chemical Co.) supplemented with 10% of FCS. Selection was performed by addition of hygromycin to a final concentration of 0.1 mg/ml. Approximately 2 wk after transfection, cells were cloned by limiting dilution in 96-well plates. Clones were expanded and tested for secretion of I-Ag7 by Western blot analysis after induction of expression with copper sulfate (1 mM). The clone with the highest expression level was scaled up in roller bottles using Schneider medium supplemented with 5% FCS and 0.1 mg/ml of hygromycin. The supernatant was harvested 4 d after induction of protein expression with copper sulfate at 1 mM (Sigma Chemical Co.).Purification of I-Ag7.
Supernatants were concentrated by ultrafiltration using a YM30 spiral membrane cartridge (Amicon). The I-A-specific 10-2.16 mAb (20; hybridoma from the American Type Culture Collection) was coupled to cyanogen bromide-activated Sepharose 4B beads (Pharmacia Biotech). The concentrated supernatant was passed through a Sepharose 4B precolumn and the 10-2.16 column at a flow rate of 9 ml/h. The column was then washed with 100 mM phosphate buffer, pH 8.0, and the protein was eluted with 2 bed volumes of 50 mM glycine, pH 11.5. Fractions were immediately neutralized by addition of 2 M Tris, pH 8.8, and dialyzed against PBS. Protein concentration was determined with the Coomassie Plus protein assay (Pierce).Western Blot Analysis and HPLC Gel Filtration.
Antisera specific for the Fos and Jun dimerization domains were generated by immunizing Lewis rats with synthetic peptides (provided by Dr. P. Kim, Whitehead Institute, Cambridge, MA). Fos peptide sequence, Ac-CGGTDTLQAETDQLEDEKYALQTEIANLLKEKEKL-CONH2; Jun peptide sequence, Ac-CGGIARLEEKVKTLKAQNYELASTANMLREQVAQL-CONH2. For Western blot analysis, proteins were separated under reducing conditions by SDS-PAGE (12%) and transferred to a polyvinylidene difluoride membrane (Millipore Corp.). Membranes were blocked overnight in 3% non-fat dry milk in TBST-buffer (50 mM Tris, pH 8.0, 150 mM NaCl, 0.2% Tween 20). Membranes were probed with Fos antiserum (1:1,000) and/or Jun antiserum (1:500). Bound Fos and Jun antibodies were detected by incubating the membranes with horseradish peroxidase-conjugated anti-rat IgG (1:3,000). The blots were developed by ECL (Amersham). HPLC gel filtration analysis of I-Ag7 was performed using a Bio-Gel SEC 30-XL column (300 × 7.8 mm; Bio-Rad) with phosphate buffered saline, pH 7.8, at a flow rate of 0.8 ml/min. The following proteins were used as molecular mass standards: thyroglobulin (669 kD), aldolase (158 kD), BSA (67 kD), ovalbumin (43 kD), and chymotrypsinogen A (25 kD).Peptide Binding Assays.
Purified I-Ag7 (0.6 µg) was incubated with biotinylated test peptide at 37°C for 18 h in a final volume of 50 µl. Buffers were either 20 mM sodium acetate/100 mM NaCl, pH 5.0, or PBS, pH 7.4, both containing 1 mM PMSF and 1 mM EDTA. In parallel, a 96-well plate (Fluoronunc; Nunc) was coated overnight at 4°C with 50 µl of 10 µg/ml of the I-A-specific antibody 10-2.16 in sodium bicarbonate buffer, pH 9.6. Nonspecific binding sites were blocked with 10% FCS in PBS/0.05% Tween 20 (PBS-Tween) for 2 h at room temperature. Wells were washed three times with PBS-Tween and I-Ag7-peptide samples were added to the wells. After a 1-h incubation, wells were washed four times with PBS-Tween and europium-labeled streptavidin (Wallac Oy, Finland) was added (1:2,000 in PBS/0.5% BSA, 100 µl/well) for detection of I-Ag7-bound biotinylated peptide. After a 1-h incubation at room temperature, wells were washed six times with PBS-Tween and Delfia enhancement solution (Wallac Oy) was added. Fluorescence was quantitated after 30 min in a fluorescence plate reader (Delfia 1234; Wallac Oy). For competition assays, 0.6 µg of soluble I-Ag7 was incubated with biotinylated transferrin peptide (1 µM) at pH 5.0 in the presence of nonbiotinylated competitor peptide (8 nM-25 µM). I-Ag7-bound biotinylated transferrin peptide was quantitated as described above.Peptide Dissociation Experiments.
For CLIP and CLIP 98D dissociation assays, soluble I-Ag7 was loaded with biotinylated CLIP or CLIP 98D (1 µM) at 37°C for 18 h at pH 7.4. An equal volume of 20 mM sodium acetate, pH 4.5, or PBS, pH 7.4, was added in the presence of nonlabeled mouse serum albumin peptide (100 µM). The final pH was either 5.0 or 7.4. At different time points (5-120 min), the reaction was stopped by freezing the samples atHerpes Simplex Virus 2 VP16-specific T Cell Line and T Cell Proliferation Assay.
7-wk-old female NOD mice were immunized subcutaneously with 100 µg of Herpes simplex virus (HSV)-2 VP16 peptide in CFA. Draining lymph nodes were removed 10 d after immunization and lymph node cells were seeded at 5 × 105 per well in 96-well U-bottomed plates in serum-free media (AIM-V; GIBCO BRL) containing 5.5 × 10 ![]() |
Results |
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Soluble I-Ag7
was expressed in Drosophila Schneider cells by replacing the
transmembrane and cytoplasmic segments of I-A and I-A
with leucine zipper dimerization domains from the
transcription factors Fos and Jun, respectively. A short,
flexible linker [Val-Asp-(Gly)5] that encoded a SalI restriction site was placed between the extracellular domains of
I-A
and I-A
and the Fos/Jun segments (Fig. 1). Leucine zipper dimerization domains were previously shown to
promote the assembly of HLA-DR2 and I-Ad (19, 21).
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The I-A-Fos and I-A
-Jun constructs were separately
cloned into the pRmHa-3 vector under the control of the
copper-inducible metallothionein promoter (18). These
constructs were cotransfected with a hygromycin selection
plasmid into S2 cells and transfectants were cloned by limiting dilution after initial selection with hygromycin. Expression was induced by addition of copper sulfate to the
growth medium and the protein was purified from concentrated supernatants by affinity chromatography using mAb
10-2.16. The yield was ~0.7-1.6 mg/liter of culture.
SDS-PAGE of the purified protein demonstrated two
bands with an apparent molecular mass of 43.3 and 33 kD
(Fig. 2 A). The identity of these bands as I-A-Fos and
I-A
-Jun, respectively, was confirmed by Western blot
analysis using antisera specific for the Fos and Jun leucine
zippers (Fig. 2 B). The migration of the two chains was
similar to that observed for
and
chains of HLA-DR2
expressed with Fos/Jun dimerization domains (19). Purified I-Ag7 eluted from a HPLC gel filtration column with a
molecular mass appropriate for soluble I-Ag7 (Fig. 2 C).
Importantly, the protein did not form high molecular mass
aggregates, indicating that it was indeed soluble in the absence of detergent.
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Soluble I-Ag7 was used to examine the binding of naturally processed I-Ag7 peptides as well as peptides from islet autoantigens under detergent-free conditions (Fig. 3, Table I). This is important because detergents can have a major effect on peptide binding by MHC class II molecules. For example, detergents with unbranched intermediate length hydrocarbon chains were found to promote dissociation of CLIP from HLA-DR (22). Two different binding assays were performed. In the direct binding assay, biotinylated peptides were incubated with soluble I-Ag7 and bound biotinylated peptides were quantitated with europium-labeled streptavidin after capture of complexes with an I-A-specific antibody. In the competition assay, unlabeled peptides were used at different concentrations to compete for binding of a biotinylated transferrin peptide to I-Ag7.
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A naturally processed peptide from mouse albumin (residues 560-574) was the best binder in both assays (reference 23, Fig. 3). This peptide competed for binding of the biotinylated transferrin peptide at very low peptide concentrations and also gave very high counts in the direct binding assay, even when the concentration of the biotinylated albumin peptide was <100 nM. Strong binding could also be demonstrated for another naturally processed peptide from transferrin (res. 55-68), as well as for a peptide from HSP60 (res. 441-460) (Fig. 3). The murine CLIP peptide showed little or no binding at this pH (pH 5). Several peptides that were identified as T cell epitopes of islet antigens competed for binding to I-Ag7 only at relatively high peptide concentrations, indicating that they were relatively poor binders. This included all three peptides from GAD 65 (res. 247- 266, 509-528, and 524-543) as well as HSP60 (169-180) and insulin (9-23). The HSP60 (169-180), insulin (9-23), and GAD65 (249-263) peptides were also synthesized with an NH2-terminal biotin group and tested in the direct binding assay. These peptides gave only low counts that were close to background (data not shown). It is important to note that the majority of the peptides that have been described as T cell epitopes actually represent the human rather than the murine sequences. Since there are sequence differences in the sequences of some of these peptides, it is possible that some of the murine peptides are stronger binders. The immunodominant myelin basic protein peptide (MBP, Ac1-11) that induces experimental autoimmune encephalomyelitis in mice with the H-2u haplotype is also a low affinity binder, whereas the immunodominant T cell epitope of MBP in mice with the H-2s haplotype (res. 87- 99) is a high affinity binder (24).
Rapid Dissociation of CLIP from I-Ag7 at an Endosomal pH.The transferrin peptide bound to I-Ag7 at both an acidic and a neutral pH (Fig. 4 B). The binding kinetics were characteristic for an "empty" MHC class II molecule and similar to those previously observed for soluble HLA-DR2 (Fig. 4 C; reference 19). In contrast, CLIP bound to I-Ag7 at a neutral pH; at an acidic pH little or no binding was detected (Fig. 4 A). Analysis of human and murine CLIP peptides has demonstrated a binding mode in which two methionine residues of CLIP occupy the P1 and P9 pockets of the MHC class II peptide binding site. These residues correspond to positions 90 and 98 of mouse as well as residues 91 and 99 of human invariant chain, respectively (25). Since the transferrin peptide carried a negative charge at the P9 position, the corresponding residue of CLIP (methionine 98) was substituted by aspartic acid (CLIP 98D). This single amino acid substitution resulted in strong binding both at a neutral and at an acidic pH (Figs. 4 and 5). These results demonstrated that the binding characteristics of CLIP to I-Ag7 were due to the interaction of methionine 98 with the P9 pocket of I-Ag7.
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MHC class II molecules assemble with invariant chain at a neutral pH in the endoplasmic reticulum and are then transported through the Golgi complex to an endosomal compartment that has a low pH. In this compartment, the invariant chain is proteolytically cleaved, leaving the CLIP peptide in the binding site. The removal of CLIP is catalyzed by H-2M, which allows binding of antigenic peptides (28). Therefore, it was important to examine the stability of complexes that were assembled at a neutral pH and then shifted to an acidic pH. For that purpose, I-Ag7 was incubated with biotinylated CLIP at a neutral pH at 37°C. An unlabeled competitor peptide was then added in order to prevent rebinding of biotinylated CLIP and the pH was changed for different periods of time (5-120 min) (Table II). After this incubation period, the sample was neutralized and the amount of bound biotinylated peptide was quantitated. This experimental design in which complexes were formed at a neutral pH and neutralized again after incubation at pH 5 for different periods of time allowed the kinetics of CLIP dissociation to be analyzed.
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These experiments demonstrated that even a brief incubation (5 min) at pH 5.0 before neutralization resulted in complete dissociation of CLIP from I-Ag7 (Table II). Even with shorter incubation times at pH 5 (<2 min), no bound CLIP was detected (data not shown). When the complex was kept at pH 7.4, dissociation was considerably slower and bound CLIP was still detected after 120 min. The rapid, pH-dependent dissociation of CLIP was due to methionine 98 of CLIP, which occupies the P9 pocket of MHC class II molecules (25). Substitution by aspartic acid (CLIP 98D) greatly increased the stability of the complex (Table II). These results indicated that the stability of I-Ag7-CLIP complexes was pH dependent, and that the P9 pocket of I-Ag7 was critical in determining this property.
A possible explanation for the pH-dependent dissociation of CLIP was that the interaction of peptide side chains with the P9 pocket was pH dependent. Therefore, a panel of CLIP analogue peptides in which methionine 98 was substituted by all naturally occurring amino acids was examined in the competition assay (Table III). These experiments demonstrated three important properties of I-Ag7: (i) At both an acidic and a neutral pH, I-Ag7 has a strong preference for a negatively charged residue at P9. (ii) The interaction of I-Ag7 and CLIP is relatively weak at a neutral pH, and there is little or no interaction at an acidic pH. (iii) The interaction of some peptide side chains with the P9 pocket is pH dependent. Particularly striking is the observation that a CLIP analogue with histidine at P9 competes well at pH 7.4 (IC50 of 4 µM), but not at pH 5.0 (IC50 of >125 µM).
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Since it has been hypothesized that the interaction of peptides with I-Ag7 is short lived (17), we determined the dissociation rates of several peptides, which included the naturally processed transferrin and serum albumin peptides, the CLIP 98D analogue, and peptides that have been identified as T cell epitopes in NOD mice (Fig. 6, Table IV). Purified I-Ag7 was first incubated with one of the biotinylated peptides (1 µM), then the pH was adjusted to pH 7.4 or maintained at pH 5.0 and mouse serum albumin peptide was added to a final concentration of 100 µM to prevent rebinding of dissociated biotinylated peptide. The GAD 65 peptide dissociated very rapidly and a t1/2 value could not be estimated. In contrast, complexes of I-Ag7 and several other peptides were long lived, particularly at a neutral pH. The estimated t1/2 value for the serum albumin peptide was >72 h and for the transferrin peptide ~45 h at pH 5.0 and >72 h at a neutral pH. The dissociation of the CLIP 98D analogue was faster, with a t1/2 value of ~23 h at pH 5.0 and ~70 h at pH 7.4 (Fig. 6). These results demonstrated that I-Ag7 forms long-lived complexes with naturally processed peptides and that the dissociation rate of peptides was affected by pH.
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Nevertheless, I-Ag7-peptide complexes were not resistant to SDS (Fig. 7). I-Ag7 (0.6 µg) was loaded at pH 5.0 with four different peptides (transferrin, serum albumin, CLIP, or CLIP 98D analogue) by overnight incubation at 37°C. Fractions of I-Ag7-peptide complexes (0.1 µg) were examined for the formation of SDS-resistant dimers by Western blot analysis using polyclonal antisera specific for the Fos and Jun segments. An SDS-resistant dimer could not be detected with any of the peptides tested. Therefore, the SDS assay does not determine whether peptides were bound to I-Ag7 before addition of detergent. Soluble HLA-DR1 expressed in insect cells forms SDS-stable dimers with the influenza hemagglutinin (307-319) peptide (33). This indicates that SDS-sensitivity is not a general property of soluble MHC class II molecules expressed in insect cells.
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Since several of the peptides that were identified as T cell epitopes of islet autoantigens were poor binders, we examined if peptides with such binding properties could induce a T cell response. We chose the peptide from HSV-2 VP16, which has been reported to bind to HLA-DQ8 (34), since it represented a foreign antigen. This peptide showed little binding in the direct binding assay, but competed for binding of the biotinylated transferrin peptide at high peptide concentrations (data not shown). NOD mice were primed with this peptide in CFA and a T cell line specific for the HSV-2 peptide could be established from draining lymph nodes by restimulation with the HSV-2 peptide (Fig. 8 A). This T cell line was I-Ag7 restricted since the response could be completely blocked by mAb 10-2.16, but not by a control antibody (Y3-P) (Fig. 8 B). Stimulation of this T cell line required the continuous presence of the peptide in the culture. Even a single wash of the APCs after overnight incubation with the peptide completely eliminated the T cell response (Fig. 8 C, lane 2). These results demonstrate that T cells from NOD mice can be primed even by a peptide that is a poor binder for I-Ag7.
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Discussion |
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Soluble I-Ag7 was used to define the biochemical requirements for peptide loading by this MHC class II molecule, which confers susceptibility to type I diabetes in NOD mice. Several peptides, including two naturally processed peptides from exogenous antigens, bound to I-Ag7. The interaction with the invariant chain-derived CLIP peptide was relatively weak and pH dependent. CLIP bound to I-Ag7 at a neutral pH, but rapidly dissociated at an endosomal pH. This property of CLIP was due to methionine 98, which occupies the P9 pocket of the MHC class II peptide binding site (25). Substitution of this residue of CLIP greatly increased the stability of the complex, both at an acidic and neutral pH. These characteristics of I-Ag7 result in the rapid generation of empty molecules at an endosomal pH.
Several mutant cell lines have been described that are
defective in antigen presentation due to a lack of DM
expression. In these cell lines, MHC class II-CLIP complexes accumulate because DM does not catalyze the removal of CLIP (32). For several human and murine MHC
class II molecules, CLIP peptides are abundant among naturally processed peptides in normal cell lines, reflecting a
relatively stable interaction (35, 36). For example, CLIP peptides have been eluted from purified I-Ab and I-Ad.
CLIP was found to bind with a relatively high affinity to
I-Ad (IC50 of 14 nM) and was one of the best binders identified for this class II molecule (36). These results are important, since I-Ag7 and I-Ad share the same I-A chain
(12). Thus, the binding properties of CLIP to I-Ag7 appear
to be due to the unique I-Ag7
chain.
The requirement for DM in the presentation of antigens by I-Ag7 has been analyzed using T cell hybridomas specific for chicken ovalbumin (37). For all T cell hybridomas, the antigen was presented by transfectants that expressed only I-Ag7 and invariant chain, but not H-2M, indicating that the murine DM homologue is not essential for antigen presentation by I-Ag7. For two out of four hybridomas with a distinct epitope specificity, presentation was enhanced by coexpression of H2-M. These results indicate that presentation of certain epitopes by I-Ag7 can be enhanced by H-2M. This may be due to "editing" of peptide content as well as stabilization of empty I-Ag7 molecules by H-2M, as described for human MHC class II molecules (30, 31, 38).
The recently solved crystal structure of I-Ad demonstrates several features of I-A-peptide interactions that are
important in this context (16). Detailed analysis of the I-Ad
peptide binding motif demonstrated that only two peptide
residues in a 6-amino acid core were important for binding
(39). These residues are located in the P4 and P9 pockets of
the I-Ad crystal structure. I-Ad and I-Ag7 have the same chain sequence, but differ at 17 positions of the
chain.
An important difference is the presence of an interchain salt
bridge between
57 Asp and
76 Arg in I-Ad, which is
absent in I-Ag7 (
57 Ser). In I-Ag7-peptide complexes, a
salt bridge may instead be formed by P9 Asp or P9 Glu of
bound peptides and
76 Arg. This would explain the
strong preference for negatively charged residues at the P9 position, which was first noted among naturally processed
peptides eluted from I-Ag7 (23). In contrast, I-Ad has a preference for alanine or serine at the P9 position. An I-Ag7
peptide binding motif has been proposed, in which a preference for aliphatic residues was noted at P6 and for hydrophobic residues at P9 (40). Also, at P11 binding was enhanced by the presence of aspartic acid. It appears that these
data are in general agreement with other data on I-Ag7-
peptide interactions, provided that the relative positions are reassigned such that these data reflect the preferences of the P4, P7, and P9 pockets of I-Ag7.
Are I-Ag7 molecules poor peptide binders or are only some of the peptides that have been identified thus far poor ligands? This may be a separate issue from the lack of SDS resistance. The analysis of soluble I-Ag7 clearly demonstrates that this MHC class II molecule binds peptides. Two naturally processed peptides from extracellular antigens, mouse albumin and transferrin, are strong binders, indicating that I-Ag7 does not have a global defect in presentation of exogenous antigens. Peptide binding by purified I-Ag7 has only been reported in two studies that used detergent-solubilized molecules. In one of these studies, little or no specific peptide binding could be demonstrated (17). In the other study, high detergent concentrations (2% NP-40) were used in the peptide binding assay (40). Binding was demonstrated for a hen egg lysozyme peptide (res. 9-27), but not for the mouse albumin peptide that had been eluted from purified I-Ag7 and that represents the best binder for soluble I-Ag7 (23). It is possible that these difficulties in examining peptide binding by I-Ag7 are related to the isolation method, in particular to the use of certain detergents. The naturally processed transferrin and serum albumin peptides formed long-lived complexes with I-Ag7, in particular at a neutral pH. However, several peptides that have been identified as T cell epitopes of islet antigens were found to be poor binders. A similar observation has been made in the experimental autoimmune encephalomyelitis model, since the immunodominant MBP peptide (Ac1-11) in mice with the H-2u haplotype is a very weak binder (24). Taken together, our data indicate that some peptides form long-lived complexes with I-Ag7. However, it is possible that a smaller fraction of I-Ag7 molecules represent long-lived class II-peptide complexes and/or that the average affinity of I-Ag7 bound peptides is lower than that of peptides bound to other I-A molecules.
I-Ag7 immunoprecipitated from splenocytes of NOD
mice does not form SDS-resistant dimers (17). This property was also observed for soluble I-Ag7, even when the
molecules were loaded with peptides. Therefore, it appears
that SDS-sensitivity of the dimer is an intrinsic property of
I-Ag7 and does not directly reflect peptide content. SDS
sensitivity of the I-Ag7 dimer could be due to polymorphic
residues at the dimerization interface of I-A and I-A
.
Mutational analysis of I-Ag7 indicated that
56 and
57 do
not determine SDS-sensitivity (17). The absence of the salt
bridge between
57 and
76 is therefore not responsible
for the lack of SDS resistance. It is also important to keep in
mind that instability of the dimer in SDS does not indicate
that the dimer is also unstable under native conditions. In
fact, analysis of I-Ag7 purified from B cells did not indicate
that the dimer was unstable in the absence of SDS (17).
The pH-dependent interaction of I-Ag7 results in the rapid generation of empty molecules at an endosomal pH. These results demonstrate a novel mechanism by which the presentation of antigenic peptides can be affected by a disease-associated MHC class II molecule.
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Footnotes |
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Address correspondence to Kai W. Wucherpfennig, Department of Cancer Immunology and AIDS, Dana-Farber Cancer Institute, 44 Binney St., Boston MA 02115. Phone: 617-632-3086; Fax: 617-632-2662; E-mail: wucherpf{at}mbcrr.harvard.edu
Received for publication 12 January 1999 and in revised form 19 March 1999.
D.H.F. Hausmann's present address is Universität Rostock, Klinik fur Innere Medizin, Abteilung f ür Gastroenterologie, Ernst-Heydemann Str. 6, 18055 Rostock, Germany, and S. Hausmann's present address is Universität Rostock, Institut für Medizinische Biochemie, Schillingallee 70, 18057 Rostock, Germany.We wish to thank Dr. P. Kim for the generous gift of the Fos and Jun leucine zipper peptides and Dr. M. Lipes (Joslin Diabetes Center, Boston, MA) for generously providing RNA from NOD spleens.
This work was supported by a Career Development Award from the American Diabetes Association and by a grant from the National Institutes of Health (AI39619) to K.W. Wucherpfennig. D.H.F. Hausmann and S. Hausmann are recipients of postdoctoral fellowships from the Deutsche Forschungsgemeinschaft (DFG Ha2556/1-1) and the Deutscher Akademischer Austauschdienst, respectively.
Abbreviations used in this paper CLIP, class II-associated invariant chain peptide; HSV, Herpes simplex virus; MBP, myelin basic protein; NOD, nonobese diabetic.
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References |
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