Lymphoid Chemokine B Cell-Attracting Chemokine-1 (CXCL13) Is Expressed in Germinal Center of Ectopic Lymphoid Follicles Within the Synovium of Chronic Arthritis Patients

Kenrin Shi, Kenji Hayashida, Motoharu Kaneko, Jun Hashimoto, Tetsuya Tomita, Peter E. Lipsky, Hideki Yoshikawa and Takahiro Ochi
J Immunol January 1, 2001, 166 (1) 650-655; DOI: https://doi.org/10.4049/jimmunol.166.1.650

Abstract

A unique feature in inflammatory tissue of rheumatoid arthritis (RA) is the formation of ectopic lymphoid aggregates with germinal center (GC)-like structures that can be considered to contribute to the pathogenesis of RA, because local production of the autoantibody, rheumatoid factor, is thought to be a causative factor in tissue damage. However, the factors governing the formation of GC in RA are presently unknown. To begin to address this, the expression of B cell attracting chemokine (BCA-1) (CXCL13), a potent chemoattractant of B cells, was examined in the synovium of patients with RA or with osteoarthritis (OA). Expression of BCA-1 mRNA was detected in all RA samples, but in only one of five OA samples. Lymphoid follicles were observed in four of seven RA samples and in two of eight OA samples, and in most of them BCA-1 protein was detected in GC. BCA-1 was not detected in tissues lacking lymphoid follicles. Notably, BCA-1 was detected predominantly in follicular dendritic cells in GC. CD20-positive B cells were aggregated in regions of BCA-1 expression, but not T cells or macrophages. These data suggest that BCA-1 produced by follicular dendritic cells may attract B cells and contribute to the formation of GC-like structures in chronic arthritis.

B cell attracting chemokine-1 (BCA-1)3 (CXCL13; Ref. 1), a ligand of CXCR-5, is classified as a lymphoid chemokine and is a potent B cell chemoattractant, because CXCR-5 is highly expressed by naive B cells (2, 3). BCA-1 is thought to be expressed predominantly by follicular dendritic cells (FDC) in secondary lymphoid tissues and organs such as lymph nodes and spleen and to play an important role in attracting naive B cells to form germinal centers (GC) in such organs (4, 5).

Rheumatoid arthritis (RA) is a chronic inflammatory autoimmune disease. Within the inflamed synovium, there is an accumulation of lymphoid and myeloid cells, including T cells, B cells, and monocytes. The local activation of these cells is thought essential in perpetuating chronic inflammation and accelerating joint damage (6, 7). T cells and B cells in RA synovium frequently accumulate underneath the synovial surface and organize into lymphocyte aggregates with certain features of GC (8, 9), including the local differentiation of FDC and plasma cells (PC) and the production of large amounts of Ab (10, 11). The development of these structures appears to contribute to the pathogenesis of the disease by leading to the local production of the autoantibody, rheumatoid factor.

The mechanism underlying the formation of lymphocyte aggregates and GC-like structures in RA synovium has not been elucidated. In the present study, we explored the hypothesis that local expression of BCA-1 might play a role. BCA-1 expression in synovia of RA and osteoarthritis (OA) was assessed, and its distribution and relationship to the location of T cells, B cells, macrophages, and FDC were examined. BCA-1 was expressed by FDC in GC of RA and OA synovia and was found in regions of B cell aggregation. Therefore, BCA-1 may play a central role in attracting B cells to form GC in the synovium of patients with chronic arthritis.

Materials and Methods

Tissue samples

Tissue samples were obtained from seven patients with RA (mean age, 54.4 years; range, 29–71 years) and eight patients with knee OA (mean age, 74.1 years; range, 65–86 years) during surgeries. RA was diagnosed according to the American College of Rheumatology (ACR) criteria for the classification of RA (12), and OA was diagnosed according to ACR criteria for the classification of OA of the knee (13). Tissue samples of normal inguinal lymph nodes were obtained from nonarthritic patients during other surgeries.

Primary Abs

Goat anti-human BCA-1 (R&D Systems, Minneapolis, MN) was used to detect BCA-1. For detection of FDC, Abs for CD21 (clone 1F8; Dako, Glostrup, Denmark) and for dendritic reticulum cells (DRC) (clone R4/23; Dako) were used. mAbs directed against CD3-positive T cells (clone PS1; Medac, Hamburg, Germany), CD20-positive B cells (clone L26; Dako), and CD68-positive macrophages (clone KP1; Dako) were also used.

Primary Abs against another lymphoid chemokine, secondary lymphoid tissue chemokine (SLC) (CCL21; R&D Systems), were also used for immunohistochemistry in RA synovium as well as in normal inguinal lymph nodes as a control.

RNA isolation and RT-PCR

RA and OA tissues obtained at surgery were minced and weighed. One milligram of the tissue was dissolved with 1 ml of Isogen (Nippongene, Tokyo, Japan) and sonicated. RNA was extracted in accordance with the company’s directions. Two micrograms of the extracted RNA was treated with DNase I (Life Technologies, Rockville, MD) to eliminate DNA and reverse-transcribed by SuperScript II reverse-transcriptase (Life Technologies) at 42°C for 70 min using oligo (dT) as a primer (Amersham Pharmacia Biotech, Piscataway, NJ). PCR was conducted with Taq DNA polymerase (AmpliTaq Gold; Perkin-Elmer Applied Biosystems, Foster City, CA) using 1–3 μl of cDNA (1.5 mM of MgCl2) on a PCR thermal cycler (PC-700; Astec, Fukuoka, Japan). The primer pair for BCA-1 was CAG AAT CCT CTG GAA CTT GAG G (5′) and CTT CCA GAC ATT CGG AGA CC (3′), and that of β-actin was GTC CTC TCC CAA GTC CAC ACA (5′) and CTG GTC TCA AGT CAG TGT ACA GGT AA (3′). Annealing temperatures used for the amplifications were 56°C for β-actin and 58°C for BCA-1. PCR products were resolved by electrophoresis on 1.5% agarose gels and identified with ethidium bromide staining. To adjust the amount of cDNA of each sample precisely, β-actin expression was examined first using 26–30 cycles of RT-PCR to amplify 0.1, 0.2, and 0.3 μl of cDNA. After resolving the PCR products on agarose gels and identifying the relevant bands with ethidium bromide, the optimal amounts of cDNA for analysis were determined. Chemokine expression in this amount of cDNA was examined using 35, 38, and 40 cycles of PCR amplification, and the results in the linear part of the amplification curve are indicated in Fig. 1.

FIGURE 1.
FIGURE 1.

BCA-1 mRNA is uniformly expressed in RA synovium. All five RA and one of five OA samples expressed BCA-1 mRNA. Total RNA extracted from freshly isolated synovial tissue of patients with RA or OA was reverse-transcribed and subjected to PCR using specific primers. The optimal amount of cDNA, which was determined for each sample by β-actin expression, was subjected to PCR for detecting BCA-1. PCR products were electrophoresed on agarose gel and identified with ethidium bromide staining.

Immunohistochemistry

Tissues from RA and OA patients were embedded in Tissue Tek (Sakura, Tokyo, Japan), and stored at −80°C until use. The tissue was cut into 4- to 7-μm sections with a cryostat, dried at room temperature for 1 h, and fixed in 2% paraformaldehyde at 4°C for 8 min. Normal inguinal lymph nodes were treated in the same manner.

For detection of CD3 and CD20, tissue sections were boiled in 10 mM sodium citrate buffer (pH 6.0) in a 90°C water bath for 90 min to unmask the Ags.

After blocking endogenous peroxidase and nonspecific Ags, primary Abs were applied onto tissue sections. Tissues were incubated for 2 h at room temperature for detection of CD3, CD20, CD21, DRC, and CD68 and for 24 h at 4°C for detection of BCA-1 and SLC. Isotype-matched Abs were used for control staining.

Thereafter, detection using the streptavidin biotin-peroxidase complex technique (Histofine SAB-PO Kit; Nichirei, Tokyo, Japan) was conducted. Finally, the sections were developed in 3,3′-diaminobenzidine tetrahydrochloride (Dojindo Laboratories, Kumamoto, Japan) and counterstained with hematoxylin.

Two-color immunofluorescence staining

To determine the expression of BCA-1 by FDC, two-color immunofluorescence staining was performed with CD21 and with DRC, respectively. Two primary Abs raised in different species (BCA-1, goat; CD21 and DRC, mouse) were diluted together and applied onto tissue sections for 24 h at 4°C. Isotype-matched Abs were used for negative control.

FITC-conjugated rabbit anti-goat IgG (Wako, Osaka, Japan) was used as the secondary Ab for BCA-1, and rhodamine-conjugated rabbit anti-mouse Igs (Dako) for CD21 or DRC. Secondary Abs were diluted together and applied onto each tissue section for 30 min at room temperature. Finally, slides were coverslipped with PBS-glycerol with antifading agents (p-phenylenediamine dihydrochloride; Sigma, St. Louis, MO) and observed under a fluorescence microscope (E800; Nikon, Tokyo, Japan) equipped with a standard mercury lamp power supply.

Results

BCA-1 mRNA is expressed in RA and OA tissues

Expression of BCA-1 mRNA was assessed by RT-PCR using mRNA directly extracted from RA and OA tissues (Fig. 1). All samples from RA patients expressed BCA-1, whereas only one of five samples from OA patients expressed BCA-1.

BCA-1 is expressed in lymphoid follicles of RA and OA synovium

The location of BCA-1 protein expression was determined by immunohistochemistry (Fig. 2). BCA-1 was mostly expressed in lymphoid follicles in RA synovium, but no expression of BCA-1 was recognized in areas of diffuse lymphoid cell infiltration. Notably, BCA-1 was also detected in a few OA synovia with follicular lymphocytic infiltrates, but not so obviously as was observed in RA. No expression of BCA-1 was detected in OA synovia without lymphoid follicle formation.

FIGURE 2.
FIGURE 2.

BCA-1 is focally expressed in lymphoid follicles of RA synovium. Sections of follicular (A–D) and diffuse (E and F) lymphoid aggregation infiltrates in RA synovium, as well as in OA synovium (G and H), are shown. Focal expression of BCA-1 is observed in lymphoid follicles in RA synovium (B and D), whereas almost no expression is recognized in the area of diffuse lymphocytic aggregation in RA (F) or OA synovium (H). A, E, and G, Hematoxylin and eosin staining. B, D, F, and H, Immunohistochemistry for BCA-1. Higher magnification of the area outlined in B is shown in D. C, Immunohistochemistry with control goat IgG. Original magnification: AC and EH, ×200; D, ×600.

Histological characteristics of the synovium and BCA-1 expression

Histological characteristics of each sample were assessed to determine whether it contained a follicular and/or diffuse lymphocyte infiltrate (Table I). Of seven RA samples, four contained follicular and five diffuse infiltrates. Three of the samples contained both, and one contained no lymphocyte infiltrates. Of eight OA samples, two contained follicular, one diffuse, and five no lymphocytic infiltration.

View this table:
Table I.

Histological characteristics of patients synovial tissue

BCA-1 was detected in each of the synovia with follicles, but not in those without. The expression of BCA-1 was examined in each lymphoid follicle, and BCA-1 positivity was calculated as the ratio of the number of BCA-1-positive follicles to the total number of follicles. The ratio was 92% in RA and 60% in OA.

BCA-1 is expressed in the area of B cell accumulation in lymphoid follicles

Immunohistohemistry for CD3, CD20, or CD68 demonstrated an accumulation of CD20-positive B cells in the central area of almost all lymphoid follicles. CD3-positive T cells were aggregated at the boundary of lymphoid follicles, and CD68-positive macrophages did not present remarkable expression within lymphoid follicles (Fig. 3). BCA-1 expression was almost compatible with the accumulation of B cells, and the positivity, which was expressed as the ratio of the number of BCA-1-positive follicles to the number of follicles with B cell accumulation, was 100% in RA and 60% in OA (Table I). Notably, aggregations of CD20-positive cells were not found in regions that did not express BCA-1 in RA.

FIGURE 3.
FIGURE 3.

BCA-1-expressing cells reside within B cell aggregates. Immunohistochemistry of sections derived from RA synovium either of follicular (A–E) or of diffuse (F–J) lymphoid infiltrates was conducted to detect BCA-1 (A and F), CD20 (B and G), CD3 (C and H), and CD68 (D and I). BCA-1 expression is focally observed in the central area of lymphoid follicles (A), where CD20-positive B cells are densely accumulated (B). CD3-positive T cells are aggregated at the boundary of the follicle (C), and CD68-positive macrophages do not present remarkable expression within the follicle (D). BCA-1 expression was not recognized in the area of diffuse lymphocytic aggregation in RA synovium (F), where CD3-positive T cells predominantly infiltrate (H), as compared with CD20-positive B cells (G). E and J, Hematoxylin and eosin staining. Original magnification: ×200.

BCA-1 is expressed in FDC in GC

BCA-1-positive cells were usually found in the central area of lymphoid follicles, which could be regarded as GC due to the accumulation of B cells. CD21-positive cells and DRC-positive cells were also enriched in those regions (Fig. 4). Furthermore, two-color immunofluorescence staining demonstrated that BCA-1-positive cells were observed in the center of lymphoid follicles and colocalized with the expression of CD21 and DRC, respectively (Fig. 5). These findings demonstrated that BCA-1 is expressed by FDC in GC, the B cell-rich area of lymphoid follicles.

FIGURE 4.
FIGURE 4.

BCA-1 is expressed in FDCs in the GC. Immunohistochemistry of serial sections derived from RA synovium with follicular lymphocytic aggregates was conducted for the detection of BCA-1 (B and C), CD21 (D), and DRC (E). A subset of CD21-positive and DRC-positive cells express BCA-1 in lymphoid follicles in RA synovium. Higher magnification of the area outlined in B is shown in C. A, Hematoxylin and eosin staining. Original magnification: A, B, D, and E, ×200; C, ×400.

FIGURE 5.
FIGURE 5.

Cells expressing BCA-1 are identical with FDCs in the GC. Colocalization of BCA-1 with CD21 and DRCs in the central area of the lymphoid follicle is shown. Two-color immunofluorescence staining of BCA-1 with CD21 (A and B) and with DRC (C and D) was performed, respectively. BCA-1 expression (A and C; FITC, green staining) was observed in FDC characterized by specific staining with CD21 and DRC (B and D, respectively; rhodamine, red staining). Original magnification: ×400.

SLC is not detected in synovium of RA

Immunohistochemistry for another lymphoid chemokine, SLC, showed no notable expression in RA synovium. SLC was not detected even in the area that was rich in CD3-positive T cells in RA synovium, although it was observed to express in T cell-rich areas of normal inguinal lymph nodes that we examined as a positive control (Fig. 6).

FIGURE 6.
FIGURE 6.

Another lymphoid chemokine, SLC, is not expressed in RA synovium. Tissue sections from normal inguinal lymph nodes and RA synovia were examined for detection of SLC by immunohistochemistry. Expression of SLC was observed in lymph nodes where CD3-expressing T cells were observed (A and B). However, SLC was not detected in RA synovia even in the area that was rich in CD3-positive T cells (C and D). A and C, Immunohistochemistry for SLC. B and D, Immunohistochemistry for CD3. Original magnification: ×200.

Discussion

In the present study, we demonstrated that BCA-1 was expressed, most likely by FDC, in GC in the synovium of RA as well as OA and could contribute to lymphoid follicle formation. This paper is the first demonstration of BCA-1 expression in ectopic lymphoid follicles of chronic inflammatory sites.

Lymphoid follicles are usually observed in secondary lymphoid tissues and organs, such as spleen, tonsils, lymph nodes, and mucosa-associated lymphoid tissues, and are thought to be essential structures for the normal immune response in which Ag-specific B and T cells are expanded against Ags. Lymphoid follicle formation is also observed ectopically in chronic inflammatory sites. Although there is no knowledge of the true role of an ectopic lymphoid follicle in chronic inflammation, it could contribute to Ag presentation in situ, to clonal expansion of Ag-specific B and T cells, and to rendering an acute inflammation into a chronic one (10, 11, 14).

RA is a representative chronic inflammatory arthritis, the pathological mechanism of which could be thought of as being an acute inflammation at the onset, followed by progression of the chronic process (6). Although the mechanism underlying the change of the inflammatory course from acute to chronic has not been elucidated, an immune response to Ag proteins derived from joint structures might be one of the causes of prolonged inflammation. From this point of view, the formation of lymphoid follicles, especially those with GC, which is a typical histological feature of RA synovium, seems an important process in the development of chronic arthritis.

The literature illustrates that lymphoid follicles with GC consist of naive B cells in the central zone surrounded by mature B cells, PCs, and CD4-positive T cells in RA synovium, and there, naive B cells are specifically selected, activated, and clonally expanded, exhibiting isotype switching and somatic hypermutation (8, 9, 10, 11). PCs in RA synovium have been reported to synthesize high amounts of Igs, including rheumatoid factor, which is thought to participate in the pathogenesis of tissue damage (6, 15, 16, 17). Moreover, rheumatoid synoviocytes are reported to support the terminal differentiation of B cells into mature PCs in vitro (18). Based on this knowledge, B cell development in GC might be one of the essential courses in the pathogenesis of RA.

In the formation of GC as well as in the events necessary for B cell development, FDCs are supposed to be involved (19). It is also reported that FDC contribute to the apoptosis of B cells in GC via Fas-Fas ligand (20). As shown in Fig. 3, B cells are localized around BCA-1 expression in the central area of lymphoid follicles in RA synovium. Moreover, FDC characterized by CD21 and DRCs has been observed to express BCA-1 in GC of the follicles (Figs. 4 and 5). These results indicate that FDC might play crucial roles in constructing GC in RA synovium and that BCA-1 produced by FDC might act as a potent chemoattractant of naive B cells into the synovium.

In this study, BCA-1 expression was recognized in all RA samples, although the formation of lymphoid follicles was observed histologically in four of seven RA patients. The most explanatory reason for this discrepancy could be the sampling issue; the part without lymphoid follicles might be used for histological analysis, whereas another part of such tissues might include lymphoid follicles. A divergence in transcription and translation might also be present.

Recently, several lymphoid chemokines, which are mainly expressed in secondary lymphoid tissues and organs, have been found, and their role in the organization of secondary lymphoid tissue has been elucidated (4, 5). Their potent chemotaxis and constitutive expression in lymphoid organs suggest that lymphoid chemokines may play important roles in the generation and maintenance of the architecture of the immune system.

BCA-1 was first reported in 1998 with its specific expression in lymphoid organs, especially in GC in secondary lymphoid tissues and organs (2, 4). BCA-1 is a potent chemoattractant of B cells and is produced by FDC in lymphoid organs. Because CXCR5, the specific receptor of BCA-1, is mostly expressed by B cells, FDC may produce BCA-1 to attract B cells and initiate the formation of GC in lymphoid organs. Recently, BCA-1 expression was recognized in mucosa-associated lymphoid tissues with Helicobacter pylori infection (21). In addition, BCA-1 was detected in chronic inflammation induced by lymphotoxin-α in a transgenic mouse model (22). These reports suggest that BCA-1 may contribute to the development of chronic inflammation.

The origin of FDC is controversial. Kapasi et al. (23) reported that precursors of FDC exist in bone marrow, move into target organs, and differentiate into FDC, while Humphery et al. (24) and Yamakawa et al. (25) did not support the idea that FDC originate from bone marrow. According to previous reports using knockout mice, lymphotoxin-α and TNFRI play a crucial role in establishing FDC in vivo (26, 27, 28, 29, 30).

RA fibroblast-like synoviocytes are known to produce pro-inflammatory chemokines such as IL-8, monocyte chemoattractant protein-1, epithelial neutrophil activating peptide-78, macrophage inflammatory protein-1β, and RANTES (31, 32, 33, 34, 35). Furthermore, Lindhout et al. (36) reported that RA fibroblast-like synoviocytes stimulated with TNF-α and IL-1β had intrinsic properties of FDC. However, in this study, BCA-1 was not expressed in fibroblast-like cells in synovium. Moreover, RA fibroblast-like synoviocytes stimulated with pro-inflammatory cytokines including IL-1β, TNF-α, and lymphotoxin-α did not show BCA-1 expression (data not shown). Further investigation is necessary to address the problem of which cell in RA synovium is the precursor of FDC.

Recently, several investigators have reported inflammatory features of OA. Krenn et al. (37) demonstrated highly mutated VH genes in B cells, with a characteristic arrangement of B cells and PCs. Nakamura et al. (38) reported the infiltration of T cells in the synovium of OA in the early stage as well as the restricted TCR usage of Vβ-chain among those T cells. These findings suggest that OA can be regarded as one of the chronic inflammatory diseases with a certain immune response resembling autoimmune diseases like RA, although the clinical feature of inflammation is not so severe.

In this study, formation of a few lymphoid follicles with BCA-1 expression was recognized in two of eight OA synovia. The aggregation of CD20-positive B cells was also observed in those lymphoid follicles. The synovium of these patients apparently showed inflammatory changes including villous formation and looked like RA synovium. Although we diagnosed these patients as OA simply by their clinical features and by ACR criteria for the classification of OA, they might have possessed inflammatory properties similar to those in RA in their pathological process. Further follow-up will be necessary to diagnose these patients precisely.

In this study, we examined the expression of lymphoid chemokines other than BCA-1 in RA synovium. Because the expression of SLC was detected by immunohistochemistry in T cell-rich areas of normal lymph nodes but not in RA synovium, even in the area with abundant T cells, SLC might not contribute to T cell accumulation in RA synovium.

Many chemokines have been reported and they are classified into two groups as pro-inflammatory chemokines and lymphoid chemokines. BCA-1 has been classified as a lymphoid chemokine so far, but the results of this study showed its marked expression in chronic inflammatory sites. BCA-1 may play an important role in the induction of immune response in chronic inflammatory diseases, especially in autoimmune diseases such as RA. Further investigation of lymphoid chemokines in inflammatory conditions will be necessary to better understand the immunological pathogenesis in such diseases.

Footnotes

  • 1 This work was supported by a grant from the Organization for Pharmaceutical Safety and Research, Tokyo, Japan.

  • 2 Address correspondence and reprint requests to Dr. Kenji Hayashida, Department of Orthopedic Surgery, Osaka University Medical School, 2-2 Yamadaoka, Suita, Osaka 565-0871, Japan. E-mail address: hkenji{at}mc.neweb.ne.jp

  • 3 Abbreviations used in this paper: BCA-1, B cell attracting chemokine-1; ACR, American College of Rheumatology; DRC, dendritic reticulum cell; FDC, follicular dendritic cell; GC, germinal center; OA, osteoarthritis; PC, plasma cell; RA, rheumatoid arthritis; SLC, secondary lymphoid tissue chemokine.

  • Received July 10, 2000.
  • Accepted October 9, 2000.

References

  1. Zlotnik, A., O. Yoshie. 2000. Chemokines: a new classification system and their role in immunity. Immunity 12: 121
    OpenUrlCrossRefPubMed
  2. Legler, D. F., M. Loetscher, R. S. Roos, I. Clark-Lewis, M. Baggiolini, B. Moser. 1998. B cell-attracting chemokine 1, a human CXC chemokine expressed in lymphoid tissues, selectively attracts B lymphocytes via BLR1/CXCR5. J. Exp. Med. 187: 655
    OpenUrlAbstract/FREE Full Text
  3. Gunn, M. D., V. N. Ngo, K. M. Ansel, E. H. Ekland, J. G. Cyster, L. T. Williams. 1998. A B-cell-homing chemokine made in lymphoid follicles activates Burkitt’s lymphoma receptor-1. Nature 391: 799
    OpenUrlCrossRefPubMed
  4. Cyster, J. G.. 1999. Chemokines and cell migration in secondary lymphoid organs. Science 286: 2098
    OpenUrlAbstract/FREE Full Text
  5. Melchers, F., A. G. Rolink, C. Schaniel. 1999. The role of chemokines in regulating cell migration during humoral immune responses. Cell 99: 351
    OpenUrlCrossRefPubMed
  6. Harris, E. D., Jr. 1990. Rheumatoid arthritis: pathophysiology and implications for therapy. N. Engl. J. Med. 322: 1277
    OpenUrlCrossRefPubMed
  7. Krane, S. M.. 1993. Mechanisms in tissue destruction in rheumatoid arthritis. D. J. McCarty, Jr, and W. J. Koopman, Jr, eds. Arthritis and Allied Conditions 12th Ed.763 Lea & Febiger, London, U.K.
  8. Klimiuk, P. A., J. J. Goronzy, J. Bjornsson, R. D. Beckenbaugh, C. M. Weyand. 1997. Tissue cytokine patterns distinguish variants of rheumatoid synovitis. Am. J. Pathol. 151: 1311
    OpenUrlPubMed
  9. Wagner, U. G., P. J. Kurtin, A. Wahner, M. Brackertz, D. J. Berry, J. J. Goronzy, C. M. Weyand. 1998. The role of CD8+CD40L+ T cells in the formation of germinal centers in rheumatoid synovitis. J. Immunol. 161: 6390
    OpenUrlAbstract/FREE Full Text
  10. Schroder, A. E., A. Greiner, C. Seyfert, C. Berek. 1996. Differentiation of B cells in the nonlymphoid tissue of the synovial membrane of patients with rheumatoid arthritis. Proc. Natl. Acad. Sci. USA 93: 221
    OpenUrlAbstract/FREE Full Text
  11. Kim, H. J., V. Krenn, G. Steinhauser, C. Berek. 1999. Plasma cell development in synovial germinal centers in patients with rheumatoid and reactive arthritis. J. Immunol. 162: 3053
    OpenUrlAbstract/FREE Full Text
  12. Arnett, F. C., S. M. Edworthy, D. A. Bloch, D. J. McShane, J. F. Fries, N. S. Cooper, L. A. Healey, S. R. Kaplan, M. H. Liang, H. S. Luthra, et al 1988. The American Rheumatism Association 1987 revised criteria for the classification of rheumatoid arthritis. Arthritis Rheum. 31: 315
    OpenUrlCrossRefPubMed
  13. Altman, R., E. Asch, D. Bloch, G. Bole, D. Borenstein, K. Brandt, W. Christy, T. D. Cooke, R. Greenwald, M. Hochberg, et al 1986. Development of criteria for the classification and reporting of osteoarthritis: classification of osteoarthritis of the knee. Arthritis. Rheum. 29: 1039
    OpenUrlCrossRefPubMed
  14. Stott, D. I., F. Hiepe, M. Hummel, G. Steinhauser, C. Berek. 1998. Antigen-driven clonal proliferation of B cells within the target tissue of an autoimmune disease. J. Clin. Invest. 102: 938
    OpenUrlCrossRefPubMed
  15. Panush, R. S., N. E. Bianco, P. H. Schur. 1971. Serum and synovial fluid IgG, IgA and IgM antigammaglobulins in rheumatoid arthritis. Arthritis Rheum. 14: 737
    OpenUrlCrossRefPubMed
  16. Bankhurst, A. D., G. Husby, R. C. Williams, Jr. 1976. Predominance of T cells in the lymphocytic infiltrates of synovial tissues in rheumatoid arthritis. Arthritis. Rheum. 19: 555
    OpenUrlCrossRefPubMed
  17. Vaughan, J. H.. 1993. Pathogenetic concepts and origins of rheumatoid factor in rheumatoid arthritis. Arthritis Rheum. 36: 1
    OpenUrlCrossRefPubMed
  18. Dechanet, J., P. Merville, I. Durand, J. Banchereau, P. Miossec. 1995. The ability of synoviocytes to support terminal differentiation of activated B cells may explain plasma cell accumulation in rheumatoid synovium. J. Clin. Invest. 102: 938
    OpenUrl
  19. Lindhout, E., G. Koopman, S. T. Pals, C. de Groot. 1997. Triple check for antigen specificity of B cells during germinal centre reactions. Immunol. Today 18: 573
    OpenUrlCrossRefPubMed
  20. Hur, D. Y., D. J. Kim, S. Kim, Y. I. Kim, D. Cho, D. S. Lee, Y. Hwang, K. W. Bae, K. Y. Chang, W. J. Lee. 2000. Role of follicular dendritic cells in the apoptosis of germinal center B cells. Immunol. Lett. 72: 107
    OpenUrlCrossRefPubMed
  21. Mazzucchelli, L., A. Blaser, A. Kappeler, P. Scharli, J. A. Laissue, M. Baggiolini, M. Uguccioni. 1999. BCA-1 is highly expressed in Helicobacter pylori-induced mucosa-associated lymphoid tissue and gastric lymphoma. J. Clin. Invest. 104: 49
    OpenUrlCrossRefPubMed
  22. Hjelmstrom, P., J. Fjell, T. Nakagawa, R. Sacca, C. A. Cuff, N. H. Ruddle. 2000. Lymphoid tissue homing chemokines are expressed in chronic inflammation. Am. J. Pathol. 156: 1133
    OpenUrlCrossRefPubMed
  23. Kapasi, Z. F., D. Qin, W. G. Kerr, M. H. Kosco-Vilbois, L. D. Shultz, J. G. Tew, A. K. Szakal. 1998. Follicular dendritic cell (FDC) precursors in primary lymphoid tissues. J. Immunol. 160: 1078
    OpenUrlAbstract/FREE Full Text
  24. Humphrey, J. H., D. Grennan, V. Sundaram. 1999. The origin of follicular dendritic cells in the mouse and the mechanism of trapping of immune complexes on them. Histol. Histopathol. 14: 135
    OpenUrlPubMed
  25. Yamakawa, M., Y. Imai, M. Dobashi, T. Kasajima. 2000. Development of follicular dendritic cells: a study using short-term bone marrow cell grafting in SCID mice. Eur. J. Immunol. 14: 859
    OpenUrl
  26. Matsumoto, M., Y. X. Fu, H. Molina, G. Huang, J. Kim, D. A. Thomas, M. H. Nahm, D. D. Chaplin. 1997. Distinct roles of lymphotoxin α and the type I tumor necrosis factor (TNF) receptor in the establishment of follicular dendritic cells from non-bone marrow-derived cells. J. Exp. Med. 186: 1997
    OpenUrlAbstract/FREE Full Text
  27. Ngo, V. N., H. Korner, M. D. Gunn, K. N. Schmidt, D. S. Riminton, M. D. Cooper, J. L. Browning, J. D. Sedgwick, J. G. Cyster. 1999. Lymphotoxin α/β and tumor necrosis factor are required for stromal cell expression of homing chemokines in B and T cell areas of the spleen. J. Exp. Med. 189: 403
    OpenUrlAbstract/FREE Full Text
  28. Tkachuk, M., S. Bolliger, B. Ryffel, G. Pluschke, T. A. Banks, S. Herren, R. H. Gisler, M. H. Kosco-Vilbois. 1998. Crucial role of tumor necrosis factor receptor 1 expression on nonhematopoietic cells for B cell localization within the splenic white pulp. J. Exp. Med. 187: 469
    OpenUrlAbstract/FREE Full Text
  29. Gonzalez, M., F. Mackay, J. L. Browning, M. H. Kosco-Vilbois, R. J. Noelle. 1998. The sequential role of lymphotoxin and B cells in the development of splenic follicles. J. Exp. Med. 187: 997
    OpenUrlAbstract/FREE Full Text
  30. Fu, Y. X., G. Huang, Y. Wang, D. D. Chaplin. 1998. B lymphocytes induce the formation of follicular dendritic cell clusters in a lymphotoxin α-dependent fashion. J. Exp. Med. 187: 1009
    OpenUrlAbstract/FREE Full Text
  31. Koch, A. E., S. L. Kunkel, J. C. Burrows, H. L. Evanoff, G. K. Haines, R. M. Pope, R. M. Strieter. 1991. Synovial tissue macrophage as a source of the chemotactic cytokine IL-8. J. Immunol. 147: 2187
    OpenUrlAbstract
  32. Koch, A. E., S. L. Kunkel, L. A. Harlow, B. Johnson, H. L. Evanoff, G. K. Haines, M. D. Buridick, R. M. Pope, R. M. Strieter. 1992. Enhanced production of monocyte chemoattractant protein-1 in rheumatoid arthritis. J. Clin. Invest. 90: 772
    OpenUrlCrossRefPubMed
  33. Koch, A. E., S. L. Kunkel, L. A. Harlow, D. D. Mazarakis, G. K. Haines, M. D. Burdick, R. M. Pope, R. M. Strieter. 1994. Epithelial neutrophil activating peptide-78: a novel chemotactic cytokine for neutrophils in arthritis. J. Clin. Invest. 94: 1012
    OpenUrlCrossRefPubMed
  34. Koch, A. E., S. L. Kunkel, M. R. Shah, R. Fu, D. D. Mazarakis, G. K. Haines, M. D. Burdick, R. M. Pope, R. M. Strieter. 1995. Macrophage inflammatory protein-1β: a C-C chemokine in osteoarthritis. Clin. Immunol. Immunopathol. 77: 307
    OpenUrlCrossRefPubMed
  35. Robinson, E., E. C. Keystone, T. J. Schall, N. Gillett, E. N. Fish. 1995. Chemokine expression in rheumatoid arthritis (RA): evidence of RANTES and macrophage inflammatory protein (MIP)-1β production by synovial T cells. Clin. Exp. Immunol. 101: 398
    OpenUrlPubMed
  36. Lindhout, E., M. van Eijk, M. van Pel, J. Lindeman, H. J. Dinant, C. de Groot. 1999. Fibroblast-like synoviocytes from rheumatoid arthritis patients have intrinsic properties of follicular dendritic cells. J. Immunol. 162: 5949
    OpenUrlAbstract/FREE Full Text
  37. Krenn, V., F. Hensel, H. J. Kim, M. M. Souto Carneiro, P. Starostik, G. Ristow, A. Konig, H. P. Vollmers, H. K. Muller-Hermelink. 1999. Molecular IgV(H) analysis demonstrates highly somatic mutated B cells in synovialitis of osteoarthritis: a degenerative disease is associated with a specific, not locally generated immune response. Lab. Invest. 79: 1377
    OpenUrlPubMed
  38. Nakamura, H., S. Yoshino, T. Kato, J. Tsuruha, K. Nishioka. 1999. T-cell mediated inflammatory pathway in osteoarthritis. Osteoarthritis Cartilage 7: 401
    OpenUrlCrossRefPubMed
Back to top

In this issue

Print
Download PDF
Article Alerts
Email Article
Citation Tools

Jump to section