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Restricted IgA Repertoire in Both B-1 and B-2 Cell-Derived Gut Plasmablasts¹

Maaike Stoel^*,, Han-Qing Jiang, Cleo C. van Diemen^*, Judy C. A. M. Bun^*, Peter M. Dammers^*, M. Christine Thurnheer, Frans G. M. Kroese^*, John J. Cebra and Nicolaas A. Bos^2,*

^* Department of Cell Biology, Section Histology and Immunology, University of Groningen, Faculty Medical Sciences, Groningen, The Netherlands; and Department of Biology, University of Pennsylvania, Philadelphia, PA 19104

	Abstract

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Mucosal IgA is the most abundantly produced Ig upon colonization of the intestinal tract with commensal organisms in the majority of mammals. The repertoire of these IgA molecules is still largely unknown; a large amount of the mucosal IgA cannot be shown to react with the inducing microorganisms. Analysis of the repertoire of used H chain Ig (V_H) genes by H-CDR3 spectrotyping, cloning, and sequencing of V_H genes from murine intestinal IgA-producing plasma cells reveals a very restricted usage of V_H genes and multiple clonally related sequences. The restricted usage of V_H genes is a very consistent observation, and is observed for IgA plasma cells derived from B-1 or conventional B-2 cells from different mouse strains. Clonal patterns from all analyzed V_H gene sequences show mainly independently acquired somatic mutations in contrast to the clonal evolution patterns often observed as a consequence of affinity maturation in germinal center reactions in peripheral lymphoid organs and Peyer’s patches. Our data suggest a model of clonal expansion in which many mucosal IgA-producing B cells develop in the absence of affinity maturation. The affinity of most produced IgA might not be the most critical factor for its possible function to control the commensal organisms, but simply the abundance of large amounts of IgA that can bind with relatively unselected affinity to redundant epitopes on such organisms.

	Introduction

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The lamina propria (LP)³ of the intestinal tract of most mammalian species contains the largest number of plasma cells in the whole body. Most of these plasma cells produce IgA. This IgA is actively transported through the intestinal epithelium into the gut as secretory IgA (sIgA). The function of sIgA within the gut lumen is largely unknown. One favored mode of action of sIgA is to prevent adhesion of microorganisms to the gut epithelium and thus promote exclusion from the gut (immune exclusion) (1, 2). Both in humans and in experimental animals nearly all of the commensal gut organisms are coated with sIgA (3, 4). Despite this IgA coating, a relatively stable commensal ecosystem can survive in the gut and is considered to be beneficial for the host.

The presence of commensal microorganisms is important for the induction of IgA production, because germfree animals that do not contain microorganisms lack intestinal IgA (5). Introduction of commensal microorganisms into formerly germfree animals leads to the rapid onset of IgA production (6, 7). Recently, Macpherson et al. (8) showed that even in mice lacking T cells, some IgA can be specifically induced by introducing new microorganisms into the intestinal tract. However, not all of the IgA that is induced by particular microorganisms reacts with those microbes. This bystander or natural IgA can account for >90% of all the gut IgA, even in animals monoassociated with one single species of commensal microorganisms (7). The ratio of Ag-specific vs natural IgA depends on the inducing microorganisms (9). The specificity repertoire of this natural IgA is largely unknown.

One pathway for B cells to become IgA plasma cells is by induction of germinal center (GC) reactions in the Peyer’s patches (PP) and isolated lymphoid follicles (ILF) that are present along the small intestinal tract. At these sites, B cells are activated and induced to switch to IgA. Activated B cells leave the PP to migrate via mesenteric lymph nodes and the thoracic duct to the LP of the small intestine to become IgA plasma cells. Class switching possibly also takes place outside of the PPs in the LP (10). IgA⁺ plasma cells located in the LP express both activation-induced cytidine deaminase and transcripts from circular DNA that has been looped out during class switch recombination, making it very likely they had just completed class switch recombination. However, the presence of ILF within the LP as inductive sites cannot be excluded. In addition, lymphotoxin--deficient mice (which lack organized lymphoid structures such as PP and mesenteric lymph nodes) reconstituted with bone marrow from normal mice reveal normal amounts of intestinal IgA (11). This indicates that the presence of lymphoid structures such as mesenteric lymph nodes and PP is not necessary for the generation of IgA⁺ B cells.

In mice, B-1 cells also contribute to IgA production in the gut (12). B-1 cells differ in phenotype and function from conventional (CNV) B-2 cells. The IgM Abs produced by B-1 cells are often encoded by unmutated Ig V_H genes (13) and are frequently reactive with autoantigens and carbohydrate (thymus-independent type 2) Ags of microorganisms (8, 14). The physiological contribution of B-1 and B-2 cells to the intestinal IgA is still largely unknown. Different experimental models showed a B-1 cell contribution varying from 1% (15) to >50% (12).

B-1 cells are not present in PP. Peritoneal B-1 cells may switch in situ, because germline I-C transcripts were detected in peritoneal B-1 cells (16). The exact anatomical site and the factors required for B-1 cells to switch to IgA are still open for discussion. Macpherson et al. (8) have proposed that B-1 cells can contribute to IgA production even in TCR , knockout mice, but transfer of purified B-1 cells without T cells into SCID mice does not lead to significant IgA production (17). The chemokines CCL25 and CCL28 can act as attractants for both B-1 and B-2 IgA Ab-secreting cells (18, 19). IL-5, IL-6, IL-10, and IL-15 stimulate plasma cell differentiation and expression of IgA (20, 21).

Although sIgA specific for mucosal pathogens such as Vibrio cholerae (22), Salmonella typhimurium (23), and rotavirus (24) can protect in vivo against such infections, the exact role of sIgA in protection against mucosal pathogens has recently been challenged. Mice deficient in sIgA (IgA^–/–, J chain^–/–, poly-IgR^–/–) showed efficient vaccine-induced protection against some respiratory viral mucosal pathogens (22, 25, 26, 27).

Because of the great diversity of microorganisms present in the gut, the repertoire of IgA Abs is expected to be very diverse. The repertoire of IgA V_H genes in adult humans suggests a wide dissemination of clonally expanded B cells, usually with high numbers of somatic mutations (28, 29). To evaluate the IgA repertoire in the mouse, an IgA RT-PCR was developed to analyze the variation in H chain CDR3 (H-CDR3) lengths among IgA-producing intestinal B cells. The IgA repertoire expressed by intestinal IgA-producing plasmablasts was analyzed in several strains of mice, of which some had genetic defects resulting in either predominantly B-1 or B-2 cells.

	Materials and Methods

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Mice

BALB/c and C57BL/6 mice were obtained from The Jackson Laboratory. CBA/N and CBA/Ca mice were obtained from Harlan Nederland, and the A/J and A/WySnJ mice were kindly provided by M. Cancro, University of Pennsylvania. BALB/c, C57BL/6, CBA/N, CBA/Ca, A/J, and A/WySnJ mice were used to obtain small intestine and spleen samples. Mice were kept under CNV conditions. PP were surgically removed from the small intestine and analyzed separately. Approximately 1-cm-long parts of the ileum and one-third of the spleen were embedded into TissueTek OCT medium (Sakura Finetek) and snap frozen (–80°C) for cryostat sectioning, and the remainder of the duodenum and ileum was used for bulk RNA isolation.

RT-PCR

RNA was isolated by the TRIzol method (Invitrogen Life Technologies), according to the manufacturer’s instructions, from PP, the small intestine cleared of PP (hereafter called LP), sorted splenic B cells (IgD^highIgM^low), and from different numbers (1, 2, 3, 4, 5, 6, 7) of 7-µm LP cryostat sections. cDNA was produced by using random hexamer primers (Amersham Biosciences), and integrity of the cDNA was controlled by -actin PCR, using an upstream (5'-CCTAAGGCCAACCGTGAAAAG-3') primer and a downstream (5'-TCTTCATGGTGCTAGGAGCCA-3') primer. Spectrotype V_H gene PCR were done with an upstream IGHV5 (PC7183) V_H gene family-specific framework region 3 (FR3) primer (5'-ACAGTCTGAGGTCTGAGGACAC-3') or an IGHV1 (J558) V_H gene family-specific FR3 primer (5'-GCCTGACATCTGAGGACTCT-3') in combination with a downstream 5'FAM-labeled IgA C region primer (5'-CTCAGGCCATTCAGAGTACA-3'). The downstream primer was labeled with the fluorescent label FAM for the purpose of detecting the different PCR fragments during gel electrophoresis. For cloning, a universal V_H gene primer (5'-AGGTSMARCTGCAGSAGTCWGG-3') (30) was used in combination with the previously mentioned IgA C region primer. A total of 1 or 2 µl of cDNA was amplified by PCR in a 25 µl reaction mixture containing 0.6 µM upstream primer, 0.6 µM IgA C region primer, 20 mM Tris-HCl (pH 8.4), 50 mM KCL, 1.5 mM MgCl₂, 2.5 U TaqDNA polymerase (Invitrogen Life Technologies), and 0.2 mM each of dGTP, dATP, dTTP, and dCTP. The PCR amplification program consisted of 30 cycles of 30 s at 94°C (2 min in first cycle), 1 min at 58°C, and 1 min at 72°C. The program was followed by 10 min at 72°C to allow extension of all products. IgM V_H genes were amplified from FACS-sorted (IgD^high, IgM^low) recirculating follicular (RF) B cells (from spleen of the same BALB/c mice) using a downstream FAM-labeled common IgM C region primer (5'-CCCTGGATGACTTCAGTGTTG-3'). For spectrotype analysis, PCR products were analyzed by gel electrophoresis on a Megabase-1000 system (Amersham Biosciences).

Cloning

IgA V_H genes were cloned and sequenced from PCR products derived from LP of CNV C57BL/6, BALB/c, CBA/N, CBA/Ca, A/J, and A/WySnJ mice. PCR products were cloned directly into pCR4 TOPO vector (Invitrogen Life Technologies) and sequenced using an automated sequencing device, as described (31). Before cloning, the PCR fragment of interest was cut out of the agarose gel and purified using the agarose gel extraction kit (Qiagen), according to the manufacturers’ instructions.

Immunohistochemistry

Cryostat sections adjacent to the sections used for RNA analysis were stained with a peroxidase (PO)-labeled goat anti-mouse IgA Ab. PO activity was revealed by 3-amino-9-ethylcarbazole containing 0.01% H₂O₂. For orientation, nuclei were counterstained with hematoxylin.

V_H gene analysis

V_H sequences were compared with each other and with germline sequences in the European Molecular Biology Laboratory database (www.ebi.ac.uk, pp. 8, 12, 29), the International Immunogenetics information system (IMGT) database (http://imgt.cines.fr/, pp. 8, 12, 29), and published IGHV1 (J558) V_H genes (32). Replacement over silent (R/S) ratios for FR and CDR were determined, as described (33). The Taq-polymerase error rate was calculated to be 1:1014 (22 errors in 22,309 nt) on the basis of all sequenced IgA C regions. Clonal relationship among sequences derived from the same mouse was defined as having identical V-D-J junctions.

	Results

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IgA-producing cells in PP and LP show a restricted CDR3 repertoire

CDR3 length spectrotyping is a method that is based on the length variability of the CDR3 due to the use of different D and J genes and to insertion or deletion of nucleotides during the V(D)J rearrangement process. If a PCR is performed using primers for FR3 and a C region on a polyclonal B cell population, a Gaussian distribution of different fragment sizes is expected, which can be visualized by automated fragment length analysis (34, 35). This method has been used to determine the average H-CDR3 length among polyclonal IgM-producing B cell populations in the rat (33). We confirmed such random distribution among IgM⁺ RF-B cells in the mouse. Fig. 1 shows polyclonal patterns of H-CDR3 lengths among the IgM molecules. Subsequently, the distribution and average of the H-CDR3 lengths of IgA V_H-D-J_H rearrangements from Ab-producing cells in the LP of the small intestine and from the PP of conventionally reared C57BL/6 and BALB/c mice were analyzed. V_H gene primers for both the IGHV5 (PC7183) and the IGHV1 (J558) V_H gene FR3 family were used. Because it has been calculated that in conventionally reared mice 10⁸ IgA-producing plasmablasts are present within the LP of the small intestine (36), a similar polyclonal distribution among these IgA-producing plasmablasts was expected. To our surprise, H-CDR3 spectrotypes from PP and LP from both mouse strains reveal a distribution of the peak intensities of H-CDR3 lengths that differs from a Gaussian distribution in all IgA samples analyzed (Fig. 2), in contrast to the H-CDR3 spectrotypes of IgM⁺ splenic RF-B cells from the same BALB/c and C57BL/6 mice. This non-Gaussian distribution will be referred to as restricted repertoire in the remainder of this work. The restricted repertoire in the LP samples in both the IGHV5 (PC7183) and the largest mouse V_H gene family IGHV1 (J558), which contains at least 50% of the V_H genes, was very unexpected, because our samples contain many IgA plasma cells (36).

View larger version (21K): [in this window] [in a new window]   FIGURE 1. Spectrotype analysis of IgM VH genes. IgM VH from the PC7183 and J558 VH family were amplified from splenic RF-B cells originating from BALB/c and C57BL/6 mice. Two mice of each strain were analyzed, of which one is shown.

View larger version (12K): [in this window] [in a new window]   FIGURE 2. Spectrotype analysis of IgA VH genes. IgA VH genes from the PC7183 VH family were amplified from two BALB/c and C57BL/6 mice from different samples: RNA from Peyer’s patches (upper row), from four cryostat sections of the LP (middle row), and from whole small intestinal LP of the same mice (bottom row).

To further extend these observations and to eliminate possible contributions of ILF to the spectrotype analysis from LP samples, we analyzed cDNA samples that were directly obtained from cryostat sections of the small intestine from the same mice used for the original RNA isolations. The same pattern as obtained from PP and LP from the same mouse was found. The similar patterns between the spectrotypes derived from cryostat sections and from the total LP when derived from the same mouse show that the amount of IgA cDNA is not the limiting factor in the spectrotype analysis of total LP. In parallel, adjacent sections were stained with anti-IgA, and they show the abundance of IgA plasma cells in those sections, and the absence of ILFs (Fig. 3).

View larger version (81K): [in this window] [in a new window]   FIGURE 3. Total IgA stains of small intestine. Cryostat sections are from BALB/c (A) and C57BL/6 (B). IgA plasma cells were stained (brown) by goat anti-mouse IgA PO, followed by 3-amino-9-ethylcarbazole substrate, and nuclei were counterstained (blue) by hematoxylin.

To analyze whether the observed restriction in H-CDR3 spectrotypes is found in both B-1 and B-2 cell-derived IgA plasma cells, H-CDR3 spectrotype analysis was performed on cDNA samples that were obtained from the LP of conventionally reared CBA/N, CBA/Ca, A/J, and A/WySnJ mice. CBA/N mice carry a mutation (xid) in the Btk gene, leading to a lack of B-1 cells, while CBA/Ca mice are their normal controls (37). The A/WySnJ mice carry a 4.7-kb gene insertion that disrupts the 3' end of the BR3 gene (Bcmd mutation) (38, 39), resulting in a peripheral B cell deficiency. Moreover, this Bcmd mutation reduces the life span and pool size of peripheral B-2 cells, but has no effect on peripheral B-1 cells. The A/J mice are their normal controls. Similar to the control mice, both B-1 and B-2 cell-enriched mice (A/WySnJ and CBA/N, respectively) show a restricted H-CDR3 spectrotype pattern of IgA (Fig. 4). The A/WySnJ and A/J mice show more diversity in H-CDR3 length than the CBA mice and the previously mentioned BALB/c and C57BL/6 mice. Despite this higher diversity in the A/J and A/WySnJ strains, all analyses show no normal (Gaussian) distribution of H-CDR3 lengths in their spectrotypes. Furthermore, each spectrotype appears to be unique for each mouse separately.

View larger version (26K): [in this window] [in a new window]   FIGURE 4. Spectrotype analysis of IgA VH genes. Top, The analysis of whole LP samples of A/WySnJ (left) and A/J (right) mice. Bottom, Analysis of eight cryostat sections of the LP from CBA/N (left) and CBA/ca (right) mice. Analysis was performed for both the J558 and PC7183 VH gene family for three separate mice in each group.

To confirm and extend these observations, V_H-D-J_H rearrangements from LP samples of the conventionally reared BALB/c, C57BL/6, A/WySnJ, A/J, CBA/N, and CBA/Ca mice were amplified by RT-PCR, cloned, and sequenced. A universal V_H gene primer combined with a C exon1 primer was used for this cloning experiment to amplify all possible V_H gene families (30). From each sample, 9–13 V_H genes were analyzed, resulting in analysis of a total of 61 V_H genes. In each sample, except for the A/WySnJ and A/J mice, we observe multiple V_H sequences that have identical V_H-D-J_H joining sequences and thus represent clonally related sequences. This confirms the restricted repertoire as revealed by H-CDR3 length spectrotyping. The number of clonally related sequences varies from two to three clonally related members (Table I). Among these clonally related sequences, differences (greater than Taq error) are found within the V_H genes. The seven clones represent 26% of the total amount of sequences.

V_H gene sequences were compared with each other and with germline sequences in the European Molecular Biology Laboratory database (www.ebi.ac.uk, pp. 8, 12, 29), the IMGT database (http://imgt.cines.fr/, pp. 8, 12, 29), and published IGHV1 (J558) V_H genes (32). Among the sequences, the mutation frequency varied between 0 and 13% (0–28 mutations), and there were 12 germline-encoded sequences.

Among clonally related sequences, the pattern of somatic mutations was analyzed by comparison with known germline V_H sequences and analysis of shared somatic mutations. In the clonally related sequences, a pattern of somatic evolution is found that was different than observed during affinity maturation in GC. In GC, B cells are selected that accumulate mutations that favor binding to the selecting Ag, resulting in B cells that have Abs with higher affinity for the selecting Ag (40). In our clonal trees, however, the majority of somatic mutations are not shared among clonally related sequences (Fig. 5). R/S ratios for FR and CDR were determined, as described (33), and most sequences (41 of 61) show no significant differences in their CDR and FR from what would have been expected from random distributed mutations (Table II). Of the sequences that do show a significant deviation from the expected ratio, 12 deviations are in the FR and 13 in the CDR (41).

View larger version (39K): [in this window] [in a new window]   FIGURE 5. Alignment of clonally related IgA VHDJH sequence-derived VH genes from C57BL/6 and CBA/N mice and genealogical trees deduced from the mutations observed in the VH genes of these clones. Sequences of the germline gene are shown on top. Dashes indicate identical nucleotides, and gaps resulting from IMGT subdivision are marked by dots. Replacement mutations are shown in bold/underscored characters.

	Discussion

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Although it is likely that gut IgA plasmablasts producing the highest levels of mRNA may swamp out the contributions of IgA⁺ B cells to the pool of amplified cloned V_H genes that are expressed, our findings do suggest oligoclonality among these activated productive cells. This finding then still poses the problem of their selective activation. The fact that we find several clonally related sequences in such a small sample supports our findings with the spectrotype analysis in that there is a restricted usage of specific V_H genes. Cloning and sequencing experiments on splenicIgM-producing cells did not reveal clonally related sequences at all (data not shown). The mutation pattern of the clonally related IgA V_H genes suggests that selection of the cells expressing these genes is probably not driven by selection for the highest affinity, as seen in a typical GC reaction involving B-2 cells. In GC, B cells are positively selected and accumulate mutations that favor binding to the selecting Ag, resulting in B cells that have Abs with high affinity for the selecting Ag (40). However, in our clonal schemes, the majority of the somatic mutations are not shared among clonally related sequences (Fig. 5). Although the observed sequences were derived from the same cloning experiments, the level of somatic mutations within the V_H region among sequences that had identical V-D-J rearrangements was clearly higher than expected from our calculated Taq polymerase error of 1:1014. This provides evidence that the cDNA was derived from independent (clonally related) plasmablasts. The observation that most of these somatic mutations were not shared among clonally related sequences strengthened this notion. It is important, however, to keep in mind that the recovered sequences represent only part of the actual clone. Some mutations were shared in the clones derived from the CBA/N mice. A possible explanation may be that the germline gene in this strain has a different sequence than the closest known germline sequence. Alternatively, it is possible that some clonal selection is occurring in the CBA/N mice. Furthermore, most R/S mutation ratios among FR and CDR suggest no significant deviation from the expected ratio by random mutations (41). Similar conclusions about antigenic selection were drawn in a study by Sehgal et al. (42). Together, these findings imply that selection among IgA V_H genes is probably not driven by selection for the highest affinity in a typical GC reaction.

There are at least two, not mutually exclusive, explanations for these findings. First, the clones of IgA-producing cells found in the gut develop and expand from a limited number of precursor B cells outside of GC of gut lymphoid tissue; the high number of divisions lead to random, nonshared mutations without induction of the somatic hypermutation process. The restricted nature of the selection is not compatible with polyclonal B cell stimulators such as LPS as a driving force for this expansion, unless other B cell-specific superantigens such as Staphylococcus aureus protein A could selectively expand particular B cells (43).

The second explanation for these findings could be that the IgA B-2 cell precursors are selected within the GC of PP or ILF, but on the basis of other criteria than currently accepted. Normally, Ag selection is driven by competition for a limiting amount of Ag (44, 45). In the case of the continuous presence of Ags derived from gut commensal bacteria in the GC, survival of many B-2 cells without affinity maturation may occur because of the lack of competition. In addition, presentation of arrays of repetitive microbial determinants on the surface of follicular dendritic cells could even lead to T cell-independent selection of these B cells. This could explain why even in TCR , knockout mice an IgA response induced by gut microorganisms could be observed (8). Non-T cell-derived cytokines in these GC could favor the isotype switch to IgA (46). Because B-1 cells are not found in GC of PP and presumably not in those of ILF, these cells must undergo their Ag selection and expansion at other sites. In SCID mice reconstituted with B-1 cells in combination with T cells, we observed large numbers of dividing IgA⁺ cells in the mesenteric lymph nodes, suggesting that this could be an alternative site for Ag stimulation in these mice (47).

In one of our clones, we observed a very high number of somatic mutations (25 mutations) compared with the original germline V_H sequence (Fig. 5). This is in line with the high number of somatic mutations in human gut IgA V_H genes (28). This could be explained by chronic stimulation by commensal organisms, which is in accordance with the age-dependent accumulation of somatic mutations in human V_H genes (48). Alternatively, we cannot exclude the possibility of V_H gene replacement, because the observed highly mutated V_H gene shows more similarity to other V_H genes than to the original germline V_H gene. A third possibility is that this sequence, although it has the same V-D-J joining region, is not part of the same clone and uses a different germline V_H gene.

In conclusion, the IgA repertoire that is induced by commensal gut organisms is very restricted. This is true both for B-1 and B-2 cells and may be an inherent property of the mucosal immune system. The affinity of most produced IgA might not be the most critical factor for its function, but simply the abundance of large amounts of IgA that can bind with relatively unselected affinity to redundant epitopes on gut organisms and control these populations. Superimposed on this primary pathway, the B-2 cells have the property to undergo high affinity selection for particular epitopes of virulence factors of pathogenic organisms that are present in limiting amount in the microenvironment of the GC of the PP. This dual model for IgA repertoire selection may explain the peaceful coexistence of commensal organisms that do induce large amounts of natural IgA, while at the same time specific mucosal IgA responses can completely protect against pathogenic microorganisms.

	Footnotes

 
The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore be hereby marked advertisement in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

¹ This work was supported by National Institutes of Health Grant AI37108 (to J.J.C.). M.C.T. was supported by a fellowship from the Swiss National Science Foundation.

² Address correspondence and reprint requests to Dr. Nicolaas A. Bos, Department of Cell Biology, Section Histology and Immunology, University of Groningen, Faculty Medical Sciences, A. Deusinglaan 1, 9713 AV Groningen, The Netherlands. E-mail address: n.a.bos{at}med.rug.nl

³ Abbreviations used in this paper: LP, lamina propria; CNV, conventional; FR, framework region; GC, germinal center; H-CDR3, H chain CDR3; ILF, isolated lymphoid follicle; IMGT, International Immunogenetics information system; PO, peroxidase; PP, Peyer’s patch; RF, recirculating follicular; R/S, replacement over silent; sIgA, secretory IgA.

Received for publication October 17, 2003. Accepted for publication November 5, 2004.

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