B Lymphocytes Induce the Formation of Follicular Dendritic Cell Clusters in a Lymphotoxin alpha -dependent Fashion

By Yang-Xin Fu,* Guangming Huang,§ Yang Wang,Dagger and David D. ChaplinDagger §

From the * Department of Laboratory Medicine/Pathology, the Dagger  Department of Internal Medicine, and the § Howard Hughes Medical Institute and Center for Immunology, Washington University School of Medicine, St. Louis, Missouri 63110

    Abstract
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Abstract
Introduction
Materials & Methods
Results & Discussion
References

Lymphotoxin (LT)alpha is expressed by activated T cells, especially CD4+ T helper type 1 cells, and by activated B and natural killer cells, but the functions of this molecule in vivo are incompletely defined. We have previously shown that follicular dendritic cell (FDC) clusters and germinal centers (GCs) are absent from the peripheral lymphoid tissues of LTalpha -deficient (LTalpha -/-) mice. LTalpha -/- mice produce high levels of antigen-specific immunoglobulin (Ig)M, but very low levels of IgG after immunization with sheep red blood cells. We show here that LTalpha -expressing B cells are essential for the recovery of primary, secondary, and memory humoral immune responses in LTalpha -/- mice. It is not necessary for T cells to express LTalpha to support these immune functions. Importantly, LTalpha -expressing B cells alone are essential and sufficient for the formation of FDC clusters. Once these clusters are formed by LTalpha -expressing B cells, then LTalpha -deficient T cells can interact with B cells to generate GCs and productive class-switched antibody responses. Thus, B cells themselves provide an essential signal that induces and maintains the lymphoid microenvironment essential for GC formation and class-switched Ig responses.

    Introduction
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Abstract
Introduction
Materials & Methods
Results & Discussion
References

Lymphotoxin (LT)1alpha exists in two molecular forms, a soluble homotrimer that is structurally related to soluble TNF and that can bind and activate the two recognized TNF receptors TNFR-I and TNFR-II (1, 2), and a membrane-bound heterotrimer in association with the structurally related LTbeta chain with stoichiometry LTalpha 1LTbeta 2 (3, 4). This ligand interacts with the TNFR-related protein (TNFR-rp, also known as the LTbeta receptor; references 4, 5), a receptor that is expressed widely on nonlymphoid cells. Several of the ligands and receptors of the TNF/LT family contribute to the formation of normal lymphoid tissue structure. For example, LTalpha (6), LTbeta (9), and TNFR-I (10) are each required for the formation of normal Peyer's patch structure, and all of these plus TNF (11) are required for the formation of clusters of follicular dendritic cells (FDC) within the primary and secondary follicles of the spleen white pulp. In mice deficient in these cytokines or receptors, there was failure to form mature isotype-switched Ig responses after immunization with T cell-dependent antigens (such as sheep RBCs [SRBCs] or keyhole limpet hemocyanin) administered without adjuvants (7, 11). These results, then, suggest that both TNF- and LT-expressing cells may interact with FDCs or FDC precursors to support their development into organized clusters within primary spleen follicles. Bone marrow (BM)-derived LTalpha -expressing cells are able to restore the formation of clusters of FDCs after they are transferred into LTalpha -deficient (LTalpha -/-) mice (13). These restored FDC clusters can then support the formation of germinal centers (GCs) and mature isotype-switched Ig responses when the reconstituted mice are immunized with SRBCs and other antigens. Thus, LTalpha produced by BM-derived cells is essential for the formation of clusters of FDCs, which in turn contributes a permissive environment for the development of mature B cell responses.

Our initial experiments indicated that when wild-type BM cells were transferred into LTalpha -/- recipients, FDC clusters formed in the spleen white pulp between 2 and 4 wk after cell transfer, and effective IgG responses could be detected after that. In contrast, when reconstitution of LTalpha -/- mice was with mature wild-type spleen cells, no detectable FDC clusters or IgG to SRBCs could be identified 10 d after cell transfer and immunization with SRBCs (13). This suggested that several weeks are required for LTalpha -expressing BM-derived cells to restore the microenvironment, including the formation of FDC clusters, for effective IgG responses. With this in mind, it is likely that short-term reconstitution experiments in which LTalpha -/- mice receive either mixed splenocytes or purified lymphocyte subsets will not be suitable for analysis of the cellular elements that control the formation of functional FDC clusters.

It is known that both T and B cells are required for the generation of GCs and for the production of class-switched antibodies in response to T-dependent antigens. Prior studies of nude mice using partially purified preparations of mature T cells have shown that only a small fraction of T cells are required to cooperate with B cells in the formation of GCs and an isotype-switched IgG response (14, 15). To eliminate problems with contamination of one lymphocyte lineage with another, we elected to define the requirement for LTalpha -expressing cell lineages by transfer of BM from donor animals with genetic ablation of individual cell lineages rather than exclusively by transfer of purified populations of splenic LTalpha -expressing lymphoid cell subsets. We show here that LTalpha -expressing B cells are essential for the recovery of primary, secondary, and memory humoral immune responses in LTalpha -/- mice. Once proper FDC clusters are formed by B cells expressing LTalpha , then LTalpha -deficient T cells can interact with B cells to generate productive GCs and class-switched antibody responses.

    Materials and Methods
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Abstract
Introduction
Materials & Methods
Results & Discussion
References

Mice.

C57BL/6J, 129Sv, recombination activating gene (RAG)- 1-/- (catalog No. JR2216; C57BL/6J-Rag1tm1Mom), B cell receptor (BCR)-/- (catalog No. JR2288; C57BL/6J-Igh-6tm1Cgn), and TCR-/- (catalog No. JR2122; C57BL/6J-Tcrbtm1Mom Tcrdtm1Mom) mice were obtained from The Jackson Laboratory (Bar Harbor, ME). LTalpha -/- mice (6) were maintained on a mixed 129Sv × C57BL/6 background and were bred under specific pathogen-free conditions.

Measurement of antigen-specific Ig.

Specific antibodies were measured and analyzed as previously described (16). In brief, Immulon 4 plates (Dynatech Laboratories, Inc., Chantilly, VA) were coated with SRBCs (150 µl at 5 × 107/ml) suspended in 0.25% glutaraldehyde in PBS. Diluted mouse sera were then added and incubated at 4°C for 1 h. Alkaline phosphatase-conjugated goat anti-mouse isotype-specific antisera (Southern Biotechnology Assoc., Birmingham, AL) were diluted 1:500 for IgM and 1:2,000 for total IgG or IgG subclasses, and 100 µl were added and incubated at 4°C for 1 h, followed by washing and addition of the alkaline phosphatase substrate p-nitrophenyl phosphate (Sigma Chemical Co., St. Louis, MO) at 1 mg/ml. The mean OD at 405 nm from triplicate wells was compared to a standard curve of titrated serum to calculate the relative units using linear regression analysis. The results represent mean ± SEM.

Transfer of Lymphocytes.

Whole spleen cell suspensions were prepared from single mouse donor by mincing with scissors and teasing the spleen between two frosted microscope slides. T and B cells were enriched using a nylon wool column as described (17). B cells were further purified by treatment with anti-Thy1.2 plus complement as previously described (18). These preparations contained 92-95% B cells, defined as IgM+B220+ by flow cytometry. There were no detectable contaminating T cells. For T cell reconstitution, preparations were >80% T cells, and contained <10% B cells. The contaminating B cells are unlikely to be significant because the recipient TCR-/- mice contain large numbers of endogenous B cells. Where indicated, recipients were prepared by irradiation with 750 rads 3 h before cell transfer. Where indicated, SRBCs were mixed together with the spleen cell suspensions before intravenous injection. Each recipient received 107 purified cells.

BM Transplantation.

Bone marrow was harvested and recipients were prepared as described previously (13, 18). Recipient mice were lethally irradiated with 1,050 rads and reconstituted with 5 × 106 donor BM cells. 6 wk after transplantation, recipients were immunized intraperitoneally with 108 SRBCs, and serum samples were collected 10 d after primary or secondary immunization.

Evaluation of Spleen Follicle Structure.

Spleens were harvested, embedded in O.C.T. compound (Miles, Elkhart, IN), and frozen in liquid nitrogen. Frozen sections (6-10 µm thick) were fixed in cold acetone. Endogenous peroxidase was quenched with 0.2% H2O2 in methanol. After washing, the sections were stained by first incubating with FITC-conjugated B220 and biotinylated Thy1.2 (PharMingen, San Diego, CA), biotinylated anti-complement receptor (anti-CR)1 (8C12; PharMingen), or biotinylated peanut agglutinin (PNA; Vector, Burlingame, CA), all at 1:50-1:100 dilutions. Horseradish peroxidase-conjugated rabbit anti-FITC (diluted 1:20; Dako, Glostrup, Denmark) and alkaline phosphatase-conjugated streptavidin (diluted 1:20; Zymed, South San Francisco, CA) was added 1 h later. Color development for bound alkaline phosphatase and horseradish peroxidase was with an alkaline phosphatase reaction kit (Vector) and with diaminobenzidine.

    Results and Discussion
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Abstract
Introduction
Materials & Methods
Results & Discussion
References
LTalpha -expressing B Cells, but Not LTalpha -expressing T Cells Are Required for Primary, Secondary, and Memory Ig Responses.

LTalpha is expressed by activated T cells, especially CD4+ T helper type 1 cells, and by activated B and NK cells (2). Both T and B cells are required to induce formation of GCs and class-switched antibody responses to T cell-dependent antigens. The current experiments were designed to determine which BM-derived cellular elements, namely T, B, or NK cells, are required to deliver the LTalpha -dependent signal(s) for both formation of GCs and for production of a mature, isotype-switched Ig response. We used BM from wild-type mice as a source of LTalpha -expressing cells of all marrow- derived lineages. BM from Ig µ heavy chain-targeted mice (BCR-/-) provided all marrow-derived LTalpha -expressing lineages except B cells, and bone marrow from mice deficient in both TCR-beta and TCR-delta (TCR-/-) provided all marrow-derived LTalpha -expressing lineages except T cells. BM from RAG-1-/- mice provided all marrow-derived LTalpha -expressing lineages except B and T cells. Compound BM chimeric animals were prepared by reconstituting lethally irradiated LTalpha -/- mice with a 1:1 mixture of BM from LTalpha -/- mice (to provide LTalpha -/- cells from all hematopoietic lineages) and wild-type, BCR-/-, TCR-/-, or RAG-1-/- mice. These reconstituted animals contained all hematopoietic lineages, but one or more of these lineages was incapable of expressing LTalpha .

Mice reconstituted with a mixture of LTalpha -/- and wild-type BM were able to generate a strong IgG anti-SRBC response when immunized intraperitoneally 6 wk after marrow transplant (Fig. 1 A). Thus, wild-type cells were dominant over LTalpha -/- cells for formation of an isotype-switched T cell-dependent antibody response. Similarly, mice reconstituted with a mixture of LTalpha -/- and TCR-/- BM were also able to generate a strong IgG anti-SRBC response. This indicates that LTalpha -expressing T cells are not required for the development of an isotype-switched antibody response. However, mice reconstituted with a mixture of LTalpha -/- and either BCR-/- or RAG-1-/- BM failed to generate an antigen-specific IgG response. Thus, LTalpha -expressing B lymphocytes are required for the recovery of an isotype-switched antibody response.


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Fig. 1.   LTalpha -expressing B cells can restore primary, secondary, and memory anti-SRBC IgG responses in LTalpha -/- mice. Groups of three to five 8-wk-old mice were lethally irradiated and reconstituted with 1:1 mixtures of BM from LTalpha -/- mice and either BCR-/-, TCR-/-, or RAG-1-/- mice as indicated. Lethally irradiated wild-type mice reconstituted with BM from wild-type donors and LTalpha -/- mice reconstituted with BM from LTalpha -/- donors served as controls. 6 wk after BM reconstitution, all mice were immunized intravenously with 108 SRBCs in PBS. Primary anti-SRBC IgG responses (A) were measured 10 d later by ELISA (16). For measurement of secondary responses (B), mice received a booster immunization of 108 SRBCs in PBS and sera were collected 7 d later. For measurement of memory responses (C), mice that had been reconstituted with the indicated mixtures of BM were primed with a single dose of 108 SRBCs and 7 d later, 5 × 107 splenocytes were transferred to sublethally irradiated (750 rads) normal C57BL/6 mice and the recipients were immediately challenged with the same dose of SRBCs. 7 d later, serum anti-SRBC IgG responses were determined. Data shown represent the means ± SEM of triplicate determinations from three to five mice. RU, relative units. Each experiment was repeated at least twice with similar results.

LTalpha -/- mice manifest impaired secondary (Fig. 1 B) and memory (Fig. 1 C) responses after challenge with SRBCs. To investigate whether LTalpha -expressing B cells were able to reconstitute these responses, the compound BM chimeric animals were evaluated further. Strong secondary and memory IgG responses were detected in mice reconstituted with a mixture of BM from LTalpha -/- and TCR-/- mice (Fig. 1, B and C). As expected, secondary and memory IgG responses were absent in mice that had been reconstituted with mixtures of LTalpha -/- and either BCR-/- or RAG-1-/- marrow (data not shown). These data indicate both that LTalpha -expressing B cells support the development of secondary and memory responses, and also that T cells do not require LTalpha expression to provide help for the responses. Although signals from T cells by membrane proteins such as CD40 ligand (CD40L) are essential for generating memory B cells, LTalpha from T cells is not essential to provide B cell help for these responses. Consistent with these data, we found in other experiments that LTalpha -/- mice could not generate memory B cells, but could generate memory T cells (data not shown).

LTalpha -expressing B Cells, but Not LTalpha -expressing T Cells Induce the Formation of the FDC Microenvironment.

Clusters of FDCs are prominent components of lymphoid follicles that are thought to support the formation of GCs that are required for the development of robust primary and secondary IgG responses in an essential fashion (19, 20). We have recently shown that the reconstitution of antigen-specific IgG responses in LTalpha -/- mice by transplantation of wild-type BM is closely associated with the recovery of FDC clusters (13). These prior studies demonstrated that BM-derived cells produced a population of LTalpha -expressing cells that was capable of supporting the development of clusters of FDCs within the splenic white pulp nodules. To define the essential LTalpha -expressing lineage responsible for delivering this signal, we analyzed the structures of spleen follicles from LTalpha -/- mice that had been lethally irradiated and reconstituted with a mixture of BM from LTalpha -/- mice and either BCR-/- or TCR-/- mice. FDC clusters were detected by immunohistochemistry using the anti-CR1 monoclonal antibody 8C12 (21), and GCs were detected by binding PNA (Fig. 2). Both FDC clusters and GCs were restored in LTalpha -/- mice that had received a mixture of BM cells from LTalpha -/- mice and TCR-/- mice. This demonstrated that it was not necessary for cells of the T lymphocyte lineage to express LTalpha for FDC clusters and GCs to form. In contrast, neither FDC clusters nor GCs were detected in mice that had received a mixture of BM from LTalpha -/- and BCR-/- mice. Thus, LTalpha -expressing B cells are required for formation of splenic primary follicles including clusters of FDCs. Although both T and B cells are required for GC formation and for production of IgG in response to T cell-dependent antigens like SRBCs, the signals provided by each of these cell populations have been incompletely defined. Our data demonstrate that interactions between LTalpha -expressing B cells from TCR-/- mice and LTalpha -deficient T cells from LTalpha -/- mice are capable of supporting GC formation, isotype class switching, and B cell memory in the reconstituted environment. Of particular interest, our data demonstrate that B cells in an important way use LTalpha to condition their lymphoid tissue microenvironment in a way that supports the development of effective IgG responses.


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Fig. 2.   Structure of spleen follicles in compound BM chimeric mice. After sera were collected from the mice shown in Fig. 1 A, the spleens were harvested and frozen sections were stained with anti-Thy1.2 (blue) and anti-B220 (brown) to visualize the T and B cell zones (A and B), anti-CR1 monoclonal antibody 8C12 (blue) and anti-B220 (brown) to visualize clusters of FDC (C and D), or PNA (blue) and anti-IgD (brown) to visualize the GC reaction (E and F). A, C, and E show spleen sections from LTalpha -/- mice reconstituted with mixtures of bone marrow from LTalpha -/- and BCR-/- mice; B, D, and F show spleen sections from LTalpha -/- mice reconstituted with mixtures of BM from LTalpha -/- and TCR-/- mice. Proper segregation of B and T cell zones was not restored in either compound BM chimera; however, both formation of FDC clusters and GC were restored in mice reconstituted with LTalpha -expressing B cells.

B Cells Can Induce the Formation of FDC clusters in the Absence of T Cells.

As observed in LTalpha -/- mice, the peripheral lymphoid tissues of scid mice are devoid of FDC clusters (21), suggesting that mature B and/or T lymphocytes are required for FDC cluster formation to occur. Using scid recipients, Kapasi et al. suggested that either T or B cells could partially reconstitute FDC cluster formation in lymph nodes, but that both cell populations were required for full restoration of FDCs (21). A special role for B cells inducing development of FDCs had been previously postulated by Cerny et al. (22). Additionally, Yoshida et al. showed, using an allogeneic system, that when graft versus host disease was suppressed by treatment of recipients with anti-T cell antibodies, that splenocytes (presumably with T cell function blocked) could restore endogenous FDC cluster formation in scid recipients (23). However, the ability of B or T cells alone to induce FDC clusters is difficult to assess because of the difficulties in defining pure cell populations in these studies. In addition, T lymphocytes (even in very small numbers) have been unequivocally demonstrated to be essential for the formation of antigen-driven GCs (14, 15). Experimental interference with T cell function either by selective T cell depletion or by blocking costimulatory signals such as those delivered by CD40-CD40L or B7- CD28 prevents the formation of GCs and the development of specific IgG responses (20, 24). It is of interest, therefore, that FDCs express CD40 (30), which has the potential to interact in a productive fashion with CD40L on T cells, and also that patients with a congenital deficiency of CD40L have lymph nodes with severe depletion of FDC clusters (25). These observations suggest that some CD40-CD40L interaction may be essential for the development of FDC clusters. It was, therefore, unexpected that we found that mice with targeted deficiency of CD40L (31), although they showed no formation of GC after intraperitoneal immunization with SRBCs, nevertheless manifested splenic primary follicles with clusters of FDC similar to those seen in normal mice (data not shown). This suggests that the development and/or maintenance of FDC clusters and segregated T and B cell zones may be independent of a CD40-CD40L interaction.

Because FDC clusters were preserved in CD40L-/- mice that have profound impairment of B-T cell interaction, we investigated whether, in fact, any B-T cell interaction was required for the formation of splenic FDC clusters. Sections from the spleens of TCR-/- and BCR-/- mice were stained with the anti-CR1 monoclonal antibody 8C12 to detect the presence of FDC clusters (Fig. 3). Strikingly, the spleens of TCR-/- mice manifest FDC clusters similar to those seen in wild-type mice. Spleen sections from BCR-/- mice showed no detectable clusters of FDCs. These data indicated both that LTalpha -expressing B cells are required for the formation of FDC clusters and that these B cells can support the formation of FDC clusters in the absence of T cells. That B cells are the only lymphoid cell type necessary for the induction of FDC clusters is suggested by our preliminary analysis of CD3epsilon transgenic mice. These mice lack NK and mature T cell activities (32, 33). Interestingly, immunohistochemical analysis of sections from their spleens shows clusters of FDCs within B cell zones, similar to those seen in the TCR-/- mice (data not shown), suggesting that neither NK or T cells are required for the development of FDC clusters.


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Fig. 3.   Presence of FDC clusters in TCR-/- but not BCR-/- mice. BCR-/- (A and B), TCR-/- (C and D), and wild-type (E and F) mice were immunized intraperitoneally with 108 SRBCs, and spleens were harvested 10 d later. Frozen sections were stained with anti-Thy-1.2 (blue) and anti-B220 (brown) to visualize the T and B cell zones (A, C, and E). FDC clusters were observed by staining with the anti-CR1/2 monoclonal antibody 8C12 (blue; B, D, and E).

The Microenvironment Established in the Absence of T Cells Can Support the Interactions of T and B Cells in the Formation of GCs and the Class-switched IgG Response.

As expected, when TCR-/- mice were immunized with SRBCs, although there was a substantial IgM anti-SRBC response, there was no development of morphologically defined GCs and no detectable production of IgG anti-SRBC antibody (data not shown). In contrast, when BM from TCR-/- was adoptively transferred into LTalpha -/- mice, there was full recovery of GC formation and ability to produce antigen-specific IgG (Figs. 1 and 2). These data indicated that LTalpha -/- T cells from the recipient animal could act together with the LTalpha -expressing B cells from the donor to form GCs and to support Ig class switching. Additional evidence that T cells can support the formation of GCs in an LTalpha -independent fashion was obtained by transfer of purified T cells from either wild-type or LTalpha -/- mice into FDC clusters containing TCR-/- recipients. Unirradiated TCR-/- mice were treated by infusion of 107 purified splenic T cells from either wild-type or LTalpha -/- donors together with an infusion of 108 SRBCs. 10 d later, both GCs (Fig. 4) and high levels of IgG anti-SRBC antibodies (data not shown) were detected in the TCR-/- recipients, irrespective of whether they received wild-type or LTalpha -/- T cells. This indicates that the FDC clusters that are found in TCR-/- mice are competent to support the formation of GCs and a productive isotype-switched Ig response once supplemental T cells are provided. In contrast to T cells from CD40L-/- mice, LTalpha -deficient T cells can activate B cells for the GC reaction and can support isotype switching once the proper microenvironment has been established by LTalpha -expressing B cells.


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Fig. 4.   Purified LTalpha -expressing and LTalpha -deficient T cells both restore GC formation in TCR-/- mice. Unirradiated TCR-/- mice were treated with an infusion of 107 purified T cells from the spleens of LTalpha -/- (B, D, and F) or wild-type mice (A, C, and E). At the same time, the mice were immunized with 108 SRBCs administered intravenously. The spleens of the recipients were harvested 10 d later, and frozen sections were stained as described for Fig. 2. A and B are stained for B (brown) and T (blue) cells; C and D are stained for B cells (brown) and FDC (blue); E and F are stained with B220 (brown) and PNA (blue).

Mature B Cells Are Sufficient for the Restoration of FDC Clusters.

The BM transfer studies described above indicate that LTalpha -expressing cells of the B cell lineage are required to induce formation of spleen FDC clusters. To investigate whether the mature B cell component of this lineage is sufficient to provide the LTalpha -dependent signal for FDC formation, we reconstituted unirradiated RAG-1-/- mice with an intravenous infusion of either 107 purified splenic B cells or 2.5 × 106 BM cells from TCR-/- donors. 3 wk after transfer, both groups of mice show similar splenic FDC clusters (Fig. 5). These data indicate that LTalpha -expressing mature B cells alone are sufficient to reconstitute formation of endogenous FDC clusters in the primary follicles. Interestingly, resting virgin B cells are thought to be negative for expression of LTalpha (29, 34). This implies, then, that the B cell must participate in a dialogue in which it is induced, presumably in the proper area of the white pulp, to express LTalpha , which then can deliver the signal for formation of FDC clusters. The nature of the signal that induces LTalpha expression, and the immediate target cell receiving the LTalpha signal, remain to be defined. The LT-dependent signal appears to be required not only for the induction, but also for the maintenance of FDC clusters. This is suggested by our prior data showing that FDC clusters disappear over the course of 2-3 wk after replacement of normal BM by LTalpha -/- BM (13). This, then, is a unique example of B cells providing a signal that serves to induce and maintain structural elements that support the further maturation of B cell functional responses.


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Fig. 5.   Similar reconstitution of FDC clusters in RAG-1-/- mice by transfer of BM or purified B cells. Unirradiated RAG-1-/- mice were treated with an infusion of 2.5 × 106 BM cells (A and C) or 107 purified spleen B cells (B and D) from TCR-/- donors. 3 wk later, the spleens were harvested and frozen sections were stained for B/T cell zones and FDC clusters as in Fig. 2, A-D.

Of particular interest in relation to the ability of B cells to induce FDC clusters within the lymphoid tissue compartment of the spleen are the prior descriptions of ectopic development of FDC-containing lymphoid follicles and GCs in certain chronic inflammatory conditions and autoimmune diseases. For example, patients with myasthenia gravis can manifest lymphoid follicles and GCs within the thymus (35). Similar follicles and GCs are found within the inflamed synovial tissues of patients with rheumatoid arthritis (36). These GCs contain clusters of FDCs similar to those found in normal lymphoid tissue GCs. We speculate that expression of LTalpha by B cells infiltrating these tissues may provide the initial signals for formation of FDC clusters that support the formation of these ectopic GCs. FDC clusters, however, do not colocalize with B cells throughout the entire B cell zones of peripheral lymphoid tissues. Rather, they form clusters near the centers of the primary B cell follicles and spare the periphery of these follicles. One possible explanation for this positioning is that local signals may regulate the expression of LTalpha within these B cell areas. Alternatively, this restricted positioning may imply that there are additional signals besides B cell-derived LTalpha that are required to induce the development and maintenance of FDC clusters. More complete understanding of the signals that regulate the formation and maintenance of FDC clusters may provide new opportunities for manipulation of the quality and magnitude of immune responses.

    Footnotes

Address correspondence to David D. Chaplin, Howard Hughes Medical Institute and Center for Immunology, Department of Internal Medicine, Washington University School of Medicine, St. Louis, MO 63110. Phone: 314-362-9047; Fax: 314-454-0486; E-mail: chaplin{at}im.wustl.edu

Received for publication 20 October 1997 and in revised form 12 December 1997.

1   Abbreviations used in this paper: anti-CR, anti-complement receptor; BCR, B cell receptor; BM, bone marrow; CD40L, CD40 ligand; FDC, follicular dendritic cell; GC, germinal center; LT, lymphotoxin; PNA, peanut agglutinin; RAG, recombination activity gene; SRBC, sheep RBC.

The authors thank David Randolph (Washington University School of Medicine, St. Louis, MO), Hector Molina (Washington University School of Medicine, St. Louis, MO), and Mitsuru Matsumoto (Ehime University School of Medicine, Ehime, Japan) for helpful discussions.

This work was supported by grant AI01431 (Y.-X. Fu) from the National Institutes of Health. D. Chaplin is an investigator of the Howard Hughes Medical Institute.

    References
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Abstract
Introduction
Materials & Methods
Results & Discussion
References

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