The eye is protected by the ocular immunosurveillance system. We show that tear duct–associated lymphoid tissue (TALT) is located in the mouse lacrimal sac and shares immunological characteristics with mucosa-associated lymphoid tissues (MALTs), including the presence of M cells and immunocompetent cells for antigen uptake and subsequent generation of mucosal immune responses against ocularly encountered antigens and bacteria such as Pseudomonas aeruginosa. Initiation of TALT genesis began postnatally; it occurred even in germ-free conditions and was independent of signaling through organogenesis regulators, including inhibitor of DNA binding/differentiation 2, retinoic acid–related orphan receptor γt, lymphotoxin (LT) α1β2–LTβR, and lymphoid chemokines (CCL19, CCL21, and CXCL13). Thus, TALT shares immunological features with MALT but has a distinct tissue genesis mechanism and plays a key role in ocular immunity.
Mucosa-associated lymphoid tissues (MALTs), including nasopharynx-associated lymphoid tissue (NALT) and Peyer's patches (PPs), are gateways for the uptake of inhaled and ingested antigens from the lumen of the aerodigestive tract, and are considered to be the sites of induction of mucosal immune responses (Mestecky et al., 2003; Kiyono and Fukuyama, 2004). The ocular surface leading to the lacrimal sac and nasolacrimal duct also forms an interface with the outside environment. In fact, it has been proposed that conjunctiva-associated lymphoid tissue (CALT), together with tear duct–associated lymphoid tissue (TALT), organizes eye-associated lymphoid tissue to create mucosal surveillance and a barrier in the eye region of humans (Knop and Knop, 2000, 2001). Past investigations have focused on the identification and characterization of CALT (Gomes et al., 1997; Chodosh et al., 1998; Knop and Knop, 2000, 2005; Giuliano et al., 2002; Cain and Phillips, 2008). Mice and rats do not possess CALT, whereas other mammals (e.g., cats, dogs, and humans) do develop CALT (Chodosh et al., 1998). Rat conjunctivae, lacrimal glands, and harderian glands contain immunocompetent cells (e.g., CD4+ and CD8+ cells; Gomes et al., 1997); however, the immunocompetent cells do not form any organized microarchitecture at the conjunctiva and are thus diffusely located. Tears contain cytokines (e.g., IL-1, IL-4, IL-6, and TGF-β), antimicrobial peptides (e.g., lactoferrin and defensin), and secretory IgA; these secretions are an important arm of mucosal innate and acquired immunity, and respond to antigens that contact and invade the eye (Allansmith et al., 1985; Kijlstra, 1990; Gupta et al., 1996; Haynes et al., 1998; Nakamura et al., 1998; Uchio et al., 2000). Tear flow does not just provide mucosal protection at the ocular surface; it also connects the ocular surface with the nasal cavity via the tear duct, suggesting that tear flow is integral to regulating the homeostasis of the oculonasal mucosal barrier. On the other hand, the eye is considered to be an immune-privileged site, because the microenvironment of the eye is regulated by several complex aspects of the immune system (Stein-Streilein and Taylor, 2007). However, little information is currently available about the immunological nature of the eye-associated lymphoid tissue system—particularly the regulation of the tissue genesis of TALT and its immunological functions—despite the fact that TALT develops in humans (Knop and Knop, 2000, 2001).
Organogenesis of secondary lymphoid tissues, such as PPs and peripheral LNs (pLNs), is dependent on inflammatory cytokines, the release of which is mediated by lymphotoxin (LT) β receptor (LTβR) signals during the embryonic period (Mebius, 2003). The basis of LT-mediated lymphoid organ development at a molecular level was first shown in genetically manipulated Ltα−/− mice, which lack PPs and pLNs (De Togni et al., 1994). Injection of an agonistic LTβR antibody into Ltα−/− mice during a limited period in embryogenesis regenerates pLNs (Rennert et al., 1998). The physiological ligand of LTβR is a membrane-bound form of LTα1β2 produced by CD3−CD4+CD45+ lymphoid tissue inducer (LTi) cells expressing IL-7Rα (Mebius et al., 1997). IL-7Rα–mediated signals trigger LTi cells to produce LTα1β2, and Il-7rα−/− mice do not form PPs (Adachi et al., 1998b; Honda et al., 2001). In addition, deficiency of either inhibitor of DNA binding/differentiation 2 (Id2) or the retinoic acid–related orphan receptor (ROR) γt gene results in a lack of PPs and pLNs because the differentiation of CD3−CD4+CD45+ LTi cells is impaired (Yokota et al., 1999; Sun et al., 2000; Eberl et al., 2004). These facts indicate the importance of inflammation-related cytokines, as well as Id2- and RORγt-subordinated CD3−CD4+CD45+ LTi cells, in the organogenesis of lymphoid tissues, including PPs and pLNs (Kiyono and Fukuyama, 2004). However, NALT does not follow the general biological rule of the dependence of embryonic genesis on inflammatory cytokines (Fukuyama et al., 2002; Harmsen et al., 2002). NALT organogenesis, which occurs postnatally, is independent of LTβR-mediated signals and RORγt but does require Id2 (Fukuyama et al., 2002; Harmsen et al., 2002).
In this study, we provide evidence that TALT develops independently of organogenesis regulators, a finding that distinguishes TALT genesis from that of other lymphoid organs. In addition, we found that TALT plays a central role in the induction of antigen-specific immune responses against ocularly encountered antigens.
Identification of TALT in mice
TALT develops in the human tear duct (Knop and Knop, 2000, 2001; Paulsen et al., 2000, 2003), but to our knowledge no information is currently available on TALT in mice. To identify organized lymphoid tissue in the mouse tear duct and to elucidate its immunological and developmental features, we first examined the anatomy of this duct in mice. To visualize the position of the tear duct, we administered hematoxylin to mice in eye drops. We clearly observed the location of the tear duct where it connects the ocular surface to the nasal cavity (Fig. 1 A). In coronal and horizontal views, we were able to identify TALT in both the left and right side of the lacrimal sac in C57BL/6 WT mice (Fig. 1, B and C).
Postnatal development of TALT
The genesis of each type of lymphoid tissue occurs within a given time window: for example, PPs develop during late embryogenesis and NALT develops postnatally (Fukuyama et al., 2002; Mebius, 2003; Kiyono and Fukuyama, 2004). The initiation of intestinal isolated lymphoid follicles (ILFs) also occurs after birth, and the genetic background (e.g., whether the mouse is of the C57BL/6 or BALB/c strain) influences the postnatal time of initiation of tissue genesis (Hamada et al., 2002). To determine when TALT genesis is initiated and to evaluate the influence of genetic background on tissue genesis, we took tissue samples from both C57BL/6 and BALB/c mice at various pre- and postnatal stages for histological analysis. No sign of mononuclear cell accumulation was observed at embryonic day (E) 18 or postnatal day (D) 5 in C57BL/6 or BALB/c mice (Fig. 1 D and Fig. S1). In contrast, we detected accumulation of mononuclear cells at D10 in both C57BL/6 and BALB/c mice, indicating that the TALT development was initiated between D5 and D10, and that the different genetics of the two strains did not influence TALT organogenesis (Fig. 1 D and Fig. S1). To support the data, the initial appearance of mononuclear cells was noted at D7 in both C57BL/6 and BALB/c mice (Fig. 1 D and Fig. S1). Furthermore, pLN addressin (PNAd)–positive high endothelial venules (HEVs) developed at D10 but not at D5 and D7 (Fig. 1 E). These findings suggest that TALT develops postnatally, as does NALT. Unlike in the genesis of other lymphoid tissues (Mebius, 2003), expression of vascular cell adhesion molecule 1 (VCAM-1) was not observed at the TALT anlage (unpublished data).
To determine which cell population initially migrates to the TALT anlage, we analyzed the tissue genesis site at D5, D7, and D10 by confocal microscopy. The D5 anlagen did not contain any CD45+ cells, whereas the D7 TALT anlage possessed CD45+ cells (Fig. 1 F). CD3−CD4+CD45+ cells have been shown to be LTi cells (Mebius, 2003). Among the CD45+ cells in the D7 TALT anlage, we identified CD3−CD4+CD45+ cells and B220+ B cells (Fig. 1 F, D7). CD11c+ DCs were not found at D5 and D7. At D10, CD11c+ DCs and increased numbers of CD3−CD4+CD45+ cells were found in the TALT (Fig. 1 F). Because B220+ B cells were among the first cells to migrate at the TALT anlage (Fig. 1 F, D7), we examined B cell–deficient Igh6−/− mice for the development of TALT. The TALT genesis occurred normally, even in the B cell–deficient condition (Fig. S2 A). Further, TALT also developed in T cell–deficient Tcrβ−/−, Tcrδ−/− mice (Fig. S2 B). These findings show that B and T lymphocytes and DCs are dispensable for the initiation of TALT development.
Organogenesis of TALT does not require microbial stimulation
TALT has been identified in only 30–40% of humans examined (Paulsen et al., 2000, 2003; Knop and Knop, 2001), raising the possibility that environmental conditions, including microbial infections and allergic responses, are involved in the initiation of TALT development. In addition, our finding that TALT develops postnatally also points to the possible involvement of microbial stimulation in TALT genesis. However, we detected TALT in mice deficient in Toll-like receptor (TLR) signals, including Tlr2−/−, Tlr4−/−, and MyD88−/− mice (Fig. S2, C–E). Further, we found that germ-free mice developed TALT (Fig. 2 A). Thus, TALT organogenesis is most likely independent of microbial stimulation.
TALT development is independent of organogenesis regulators
We next determined the molecular requirements for TALT development. PPs and pLNs are not present in alymphoplasia (aly/aly) mice, which carry a null mutation of NF-κB–inducing kinase (NIK), resulting in a failure to transmit LTβR-mediated signals (Shinkura et al., 1999). However, our histological analysis showed that the TALT structure was preserved in aly/aly and Ltα−/− mice, although it was smaller than in WT TALT (Fig. 2, A and B; and Fig. S3). In addition, TALT was even observed in Il-7rα−/− mice, although the size was again small (Fig. 2 B and Fig. S3). Thus, the initiation of TALT development mediated by inducer cells was independent of the IL-7R and LTα1β2–LTβR–NIK pathway signaling cascades, whereas the maturation process of accumulating lymphocytes required the cytokine signaling cascade, as is the case with other lymphoid organs (Mebius, 2003; Kiyono and Fukuyama, 2004).
Lymphoid chemokines, including CXCL13, CCL19, and CCL21, play important roles in the migration of LTi cells to the sites of tissue genesis (Honda et al., 2001; Luther et al., 2003; Fukuyama et al., 2006). We therefore examined the involvement of these lymphoid chemokines in TALT genesis. The TALT structure was preserved in Cxcl13−/− mice, although they lacked some pLNs and had reduced numbers of PPs (Fig. 2 B; Ansel et al., 2000). TALT also developed well in plt/plt mice (Fig. 2 B), which carry null mutations of both the Ccl19 and Ccl21 genes (Nakano et al., 1998). Furthermore, the initiation of TALT formation was maintained in triple mutant (Cxcl13−/− plt/plt) mice (Fig. 2 B), confirming that these lymphoid chemokines are not required for the initiation of TALT organogenesis, although the TALT was smaller in the lymphoid chemokine–null condition than in WT (Fig. S3). These results supported the observation that an NIK-mediated pathway is required to recruit large numbers of lymphocytes to TALT.
We then addressed the involvement of Id2 and RORγt, key transcriptional regulators in the induction of lymphoid organogenesis by CD3−CD4+CD45+ LTi cells (Yokota et al., 1999; Sun et al., 2000; Eberl et al., 2004). Surprisingly, TALT formation was preserved in Id2−/− and Rorγt−/− mice (Fig. 2 B). Consistent with this finding, FACS and confocal microscopy analyses detected CD3−CD4+ LTi cells in the TALT anlage of Id2−/− and Rorγt−/− mice as well as in WT mice (Fig. 3, A and B). Furthermore, when we isolated these CD3−CD4+CD45+ cells from WT mice and examined the gene expression of the tissue genesis–associated transcription factors by RT-PCR, we found that CD3−CD4+CD45+ cells isolated from the TALT anlagen did not express either Id2 or Rorγt, whereas CD3−CD4+CD45+ cells isolated from the embryonic intestine, i.e., PP inducer cells, expressed both Id2 and Rorγt (Fig. 3 C). Thus, TALT organogenesis proceeds independently of Id2, RORγt, and LT. Therefore, TALT genesis is quite different from the genesis of other secondary lymphoid tissues, including PPs, pLNs, and NALT (Mebius, 2003; Kiyono and Fukuyama, 2004).
Microarchitecture of TALT
The structure of the MALT epithelium is characterized by the presence of follicle-associated epithelium (FAE; Kiyono and Fukuyama, 2004). Indeed, we were able to divide the epithelial layer of the lacrimal sac into two populations on the basis of its morphological structure (Fig. 4 A): TALT-FAE was characterized by a thin layer of squamous epithelium (Fig. 4 B), whereas the lacrimal sac epithelium had a multilayered and squamous morphology (Fig. 4 C). Interestingly, TALT-FAE lacked mucus-producing goblet cells and cilia (Fig. 4 B), a fact that distinguished this tissue from NALT-FAE, which has some goblet cells (Fig. 4 D). Instead, mucus-producing gland tissue was frequently observed on the conjunctiva (unpublished data). Confocal microscopic analysis of TALT revealed large numbers of B220+ B cells (Fig. 4 E) and CD11c+ DCs in the subepithelial dome region of the FAE (Fig. 4 F), as well as CD3+CD4+ T helper cells distributed around the B cell follicles (Fig. 4, G and H). These data indicate that TALT is composed of a highly compartmentalized and organized lymphoid structure. In accordance with the finding that neonatal TALT developed PNAd+ HEVs (Fig. 1 E), adult TALT HEVs expressed PNAd but not mucosal addressin cell adhesion molecule 1 (MAdCAM-1; Fig. 4 I and Fig. S4 A); this is similar to the case with NALT HEVs (Fig. 4 J and Fig. S4 B). These observations suggest that cellular trafficking to TALT and NALT is regulated via an L-selectin–PNAd interaction and is distinguishable from gut-trafficking mechanisms, which are dependent on α4β7 integrin/MAdCAM-1 (Kiyono and Fukuyama, 2004). These results indicate that TALT possesses many of the characteristic traits of organized MALT but is distinguished by the lack of goblet cells in its FAE region.
TALT is a site of immunological induction
To investigate the physiological function of TALT, we examined whether TALT takes up ocularly administered antigens. M cells, characterized by the M cell–specific mAb NKM16-2-4+ (Nochi et al., 2007), Ulex europaeus agglutinin (UEA) 1+, and wheat germ agglutinin−, were found in the FAE of TALT (Fig. 5 A). Electron microscopic analysis showed that TALT-FAE contained cells bearing the hallmarks of M cells: microvilli and a unique pocket formation with lymphocytes (Fig. 5, B and C). When mice were ocularly dosed with GFP-expressing Salmonella, we observed the uptake of Salmonella by UEA-1+ M cells (Fig. 5 D) as well as by CD11c+ DCs (Fig. 5 E). Moreover, when mice were ocularly challenged with Pseudomonas aeruginosa PAO1, large amounts of P. aeruginosa PAO1 were located within the TALT (Fig. 5 F). P. aeruginosa PAO1 was not detected in naive mice (Fig. 5 G). Mice ocularly challenged with P. aeruginosa PAO1 formed germinal centers (GCs; Fig. 5 H); this is an important immunological event for the initiation of hypersomatic mutations and Ig class switching, which enable the production of memory B cells with high-affinity B cell receptors (Kelsoe, 1996; Shapiro-Shelef and Calame, 2005). In contrast, GC formation was not present in the TALT of naive mice (Fig. 5 I; and Fig. 6, A and B). These data suggest that TALT is a preferential site for the uptake of ocularly encountered antigens/pathogens and for the subsequent induction of antigen-specific B cell responses.
Supporting this notion, immunization of the eyes with eye drops containing cholera toxin (CT), a well-known mucosal immunogen, resulted in the formation of GCs with a follicular DC (FDC) network in the TALT (Fig. 6, C and D). Interestingly, ocular immunization also induced GC formation in NALT (Fig. 6, E and F), suggesting that the anatomical connection through the tear duct lays the groundwork for a cooperative immunological network between TALT and NALT that responds to ocularly encountered antigens. Activation-induced cytidine deaminase (AID), an essential Ig class switch–related molecule, is expressed in organized lymphoid tissues, including NALT, PPs, and intestinal ILFs (Shikina et al., 2004). Parallel to our findings of GC formation after ocular immunization, confocal microscopy revealed the presence of AID-expressing cells in both TALT and NALT (Fig. 6, G, and H). Furthermore, RT-PCR analysis confirmed Aid expression in TALT and NALT but not in the nasal passage (NP; Fig. 6 I). Therefore, after ocular immunization with CT, increased numbers of IgA+B220− plasma cells were detected in the diffuse region of the tear duct (Fig. 6, J and K). An ELISPOT assay confirmed that some of these IgA+B220− plasma cells produced CT-specific IgA; cells producing IgA specific for the B subunit of CT (CT-B), but not IgG-forming cells, were found in single-cell preparations from the tear ducts of mice ocularly immunized with CT (Fig. 6 L and not depicted). In addition, the production of CT-B–specific IgG-forming cells was induced in the spleen by ocular immunization with CT (Fig. 6 M). Naive mice did not show any CT-B–specific Ig-producing cells (Fig. 6 N).
In addition, we found a high frequency of CT-B–specific CD4+ T cells in TALT using an MHC tetramer, consistent with the induction of antigen-specific antibody-producing cells after CT immunization (Fig. 7 A). It is important to note that the CT-B tetramer–reactive CD4+ T cells included CXCR5+ T follicular helper cells (Fig. 7 B). CT-B–specific CD4+ T cells were detected in NALT and draining LNs, such as the cervical and submandibular LNs, but at a lower frequency than in TALT (Fig. 7, A and B). Thus, it is plausible that TALT is the main gateway and inductive site for the initiation of antigen-specific T and B cell responses against ocularly encountered antigens. Collectively, these observations indicate that TALT is an important member of the MALT family. It has a lymphoid structure that is organized as an inductive site for antigen uptake and the initiation of antigen-specific mucosal immune responses with GC formation and Ig class switching, as well as the generation of antigen-specific CD4+ T cells.
Our purpose was to investigate the developmental features of TALT and to reveal the immunological importance of this tissue in immune surveillance for mucosal immunity. We found that the molecular requirements of TALT organogenesis were quite different from those of other secondary lymphoid organs. For example, the initiation of TALT organogenesis is independent of the IL-7R– and LTβR–NIK–mediated tissue genesis pathways, and thus, its structure was preserved in mice lacking other secondary lymphoid organs, such as Il-7rα−/−, Ltα−/−, and aly/aly mice (Table I). Furthermore, the TNF-related activation-induced cytokine (TRANCE)–mediated pathway, which is involved in pLN development (Kong et al., 1999), was dispensable for TALT genesis. Thus, the TALT structure was found in Trance−/− mice and in mice null for its signal transducer, TNF receptor–associated factor (TRAF) 6 (Fig. S5). However, these mice lacking secondary lymphoid organs (e.g., Il-7rα−/−, Ltα−/−, and aly/aly mice) had smaller TALT volumes than were found in WT mice. LTβR–NIK–mediated signals induce the production of lymphoid chemokines such as CXCL13, CCL19, and CCL21, and adhesion molecules, including VCAM-1 and PNAd (Dejardin et al., 2002; Browning et al., 2005). The immature formation of TALT in mice deficient in LTβR-associated molecules can therefore be explained by the lack of lymphoid chemokines and adhesion molecules involved in leukocyte migration. In support of this, the extent of the TALT in Cxcl13−/−plt/plt mice was smaller than that in Cxcl13−/− and plt/plt single- or double-mutant mice, as well as in WT mice. However, accumulation of some B lymphocytes was seen in these mutant mice (Fig. S3). Thus, we cannot eliminate the possibility that the migration stage of B lymphocytes may also operate independently of the LTβR–NIK pathway for TALT genesis.
CLN, cervical LN; MLN, mesenteric LN. +++, developed well; ++, developed with decreased number of lymphocytes; +, developed with few number of lymphocytes; −, absent; +/−, present or absent, depends on individual. *1, Yokota et al., 1999; Fukuyama et al., 2002; Boos et al., 2007; *2, Sun et al., 2000; Harmsen et al., 2002; Eberl and Littman, 2004; Eberl et al., 2004; Naito et al., 2008; Tsuji et al., 2008; *3, De Togni et al., 1994; Banks et al., 1995; Suzuki et al., 2000; Fukuyama et al., 2002; Hamada et al., 2002; Harmsen et al., 2002; Taylor et al., 2004; *4, Kanamori et al., 1996; Shinkura et al., 1999; Fukuyama et al., 2002; Hamada et al., 2002; *5, Peschon et al., 1994; Kanamori et al., 1996; Adachi et al., 1998b; Fukuyama et al., 2002; Hamada et al., 2002; Luther et al., 2003; *6, Ansel et al., 2000; Rangel-Moreno et al., 2005; Fukuyama et al., 2006; *7, Nakano et al., 1997; Rangel-Moreno et al., 2005; Fukuyama et al., 2006; and *8, Luther et al., 2003; Rangel-Moreno et al., 2005; Fukuyama et al., 2006.
One of the important findings of our study is that TALT genesis occurs in both Id2−/− and Rorγt−/− mice. TALT genesis takes place normally in Rorγt−/− mice despite the fact that CD3−CD4+CD45+ LTi cells, and as a consequence PPs and pLNs, are totally absent in these mice (Sun et al., 2000; Eberl et al., 2004). In addition, Id2 is the key transcriptional regulator for the induction and differentiation of CD3−CD4+CD45+ LTi cells (Yokota et al., 1999). Id2−/− mice do not develop any form of secondary lymphoid tissues, including pLNs, PPs, or NALT (Yokota et al., 1999; Fukuyama et al., 2002). However, TALT development is Id2 and RORγt independent (Table I). We still found that CD3−CD4+CD45+ cells, which we hypothesize to be TALT inducer cells, existed at TALT anlagen in both Id2−/− and Rorγt−/− mice, and we revealed that CD3−CD4+CD45+ cells isolated from TALT anlagen did not express either Id2 or Rorγt. A recent study showed that omental milky spots developed in the absence of LTi cells (Rangel-Moreno et al., 2009). Omental milky spots were found in Id2−/− and Rorγt−/− mice. However, this tissue development required the lymphoid chemokine CXCL13. Because the initiation of TALT development is independent of CXCL13, omental milky spots and TALT use different tissue genesis mechanisms. The organogenesis of secondary lymphoid tissues has been shown to require several processes, including the trafficking/accumulation of LTi cells, the differentiation/activation of specialized stromal cells, and the trafficking/accumulation of conventional lymphocytes (Mebius, 2003). In this light, the genesis of these tissues can be separated into at least two phases, initiation and maturation; in other words, the migration of LTi cells and lymphocytes, respectively, to the tissue development site. Our results indicate that the initiation of TALT genesis operates independently of the requirement for the classical tissue genesis–associated signaling cascade of IL-7R/LTβR–NIK because leukocytes, including B lymphocyte, already migrated to TALT without this pathway. Further, the unique CD3−CD4+CD45+ cells develop without a requirement for the LTi cell–associated transcriptional regulators Id2 and RORγt, and are identified as the first hematopoietic cell population that migrates to the TALT anlagen. To directly address the critical role of Id2- and RORγt-independent CD3−CD4+CD45+ cells (or TALT inducer cells) in the initiation of TALT genesis, our efforts are now directed toward finding and/or developing TALT-deficient mice for the necessary adoptive transfer experiment.
TALT organogenesis occurs after birth, as does NALT genesis (Fukuyama et al., 2002). In contrast, PPs and pLNs are initially generated during the embryonic period (Mebius, 2003). These findings suggest that secondary lymphoid tissue genesis can be chronologically separated into two categories: a prenatal group (PPs and pLNs) and a postnatal group (TALT and NALT). However, initiation of genesis of all of these tissues, including TALT, occurs independently of microbial stimuli.
Ocular surface antigens are taken up by NALT, and NALT might function as an inductive site for tear IgA production (Ridley Lathers et al., 1998). However, our findings suggest that TALT is a key inductive tissue for immune responses, because TALT is a more important site for the generation of antigen-specific T cells than NALT and, thus, contributes to mucosal immune responses against ocularly encountered antigens. In support of this suggestion, our study showed the presence of a mucosal gateway population of M cells in TALT that is capable of taking up ocularly administered bacterial antigens (e.g., Salmonella). Ocular infection with P. aeruginosa causes corneal ulcers and sometimes loss of vision (Liesegang, 1998), and we found P. aeruginosa given by ocular challenge within TALT, leading to the subsequent formation of GCs. These findings indicate that TALT plays an important role in ocular immune surveillance and protection, providing the first line of defense of the host's eyesight; we can therefore expect it to be equivalent in its capacity for immunosurveillance to the other well-known mucosal inductive tissues in the aerodigestive tract, NALT and PPs.
The lacrimal glands are effector sites for IgA production because their tissue contains large numbers of IgA-producing cells (Sullivan and Allansmith, 1984; Peppard and Montgomery, 1987; Saitoh-Inagawa, 2000). We also found that a large number of IgA+B220− plasma cells were distributed around the diffuse tissues of the NPs and in the tear duct in response to CT immunization via eye drops. Thus, TALT and various tissues of the tear duct are responsible for ocular immunity as inductive and effector sites, respectively.
In summary, our results demonstrated the presence of mouse TALT, providing the first definitive evidence for the existence of Id2-, RORγt-, and LTβR-independent lymphoid tissue genesis. In addition, TALT was shown to play an important role in the induction of antigen-specific immune responses and to function in immune surveillance in ocular immunity.
MATERIALS AND METHODS
C57BL/6 and BALB/c mice were purchased from Japan SLC; germ-free and aly/aly mice were purchased from CLEA Japan; and Ltα−/−, Igh6−/−, Tcrβ−/−, and Tcrδ−/− mice were purchased from the Jackson Laboratory. Il-7rα−/− mice were provided by Immunex Corp., and were also purchased from the Jackson Laboratory. Id2−/−, Rorγt−/−, Cxcl13−/−, Tlr2−/−, Tlr4−/−, MyD88−/−, Cxcl13−/−plt/plt, Trance−/−, and Traf6−/− mice were generated as previously described (Adachi et al., 1998a; Hoshino et al., 1999; Kong et al., 1999; Naito et al., 1999; Takeuchi et al., 1999; Yokota et al., 1999; Kurebayashi et al., 2000; Ebisuno et al., 2003; Fukuyama et al., 2006). Animal experiments were conducted in accordance with the guidelines of and with permission provided by the Animal Care and Use Committee of the University of Tokyo.
Histological analysis was performed as previously described (Fukuyama et al., 2002). The antibodies and lectins used for confocal microscopy analysis were as follows: FITC– or PE–anti-CD11c (HL3; BD), FITC–anti-CD3ε (145-2C11; BD), FITC–anti-IgA (C10-3; BD), PE–anti-B220 (RA3-6B2; BD), PE–anti-CD45 (30-F11; BD), PE– or APC–anti-CD4 (RM4-5; BD), FITC–anti-TCRβ (H57–597; BD), PE–anti-CXCR5 (2G8; BD), rabbit polyclonal anti-AID (H-80; Santa Cruz Biotechnology, Inc.), purified anti-FDC (FDC-M1; BD), purified anti-PNAd (MECA 79; BD), biotinylated anti–MAdCAM-1 (MECA-89; BD), biotinylated anti–VCAM-1 (429; BD), biotinylated peanut agglutinin (PNA; Vector Laboratories), rhodamine–UEA-1 (Vector Laboratories), Alexa Fluor 633–wheat germ agglutinin (Invitrogen), and FITC–NKM16-2-4 (Nochi et al., 2007). To visualize AID, FDC, MAdCAM-1, VCAM-1, PNAd, and PNA, FITC–anti–rabbit IgG (Santa Cruz Biotechnology, Inc.), FITC–anti–rat Ig κ chain (MRK-1; BD), FITC–anti–rat IgM (G53-238; BD), streptavidin-FITC (BD), and streptavidin-PE (eBioscience) were used as secondary antibodies or reagents. In some experiments, tissues were counterstained with DAPI (Sigma-Aldrich) to visualize the nucleus. P. aeruginosa PAO1 was detected with a rabbit polyclonal antibody specific for the bacterium (Abcam), followed by staining with FITC–anti–rabbit IgG (Santa Cruz Biotechnology, Inc.).
Ocular administration of bacteria.
GFP-Salmonella (Jang et al., 2004) and P. aeruginosa PAO1 (Parks and Hobden, 2005) were administered as ocular antigens. After a 30-min administration of GFP-Salmonella, the mouse's ocular surface was washed with 100 µg/ml gentamycin. P. aeruginosa PAO1 is characterized by motility, biofilm formation, acyl-homoserine lactone production, and virulence in a mouse infection model (Parks and Hobden, 2005). These bacteria were cultured in Luria broth medium at 37°C for 18 h and used for ocular administration, as previously described (Jang et al., 2004). PAO1 was given twice with an interval of 1 wk (Hazlett et al., 2001).
Immunization and analysis of antigen-specific immune responses.
Mice were ocularly immunized with 1 µg CT per eye (Sigma-Aldrich) in 5 µl PBS by eye drops three times at weekly intervals. Tissues or cells were collected from the heads of the ocularly immunized mice 7 d after the final immunization. To characterize CT-specific antibody responses, a CT-B–specific ELISPOT assay was used. In brief, 96-well plates (MultiScreen; Millipore) were coated with 2 µg/ml CT-B in 100 µl PBS (pH 7.4) per well for 16 h. The plates were washed three times with PBS and blocked with 100 µl of RPMI 1640 supplemented with 10% FCS for 30 min. After the blocking solution was discarded, 100 µl of cell suspension was applied to the well (tear duct, 104 cells/well; spleen, 106 cells/well). After incubation for 4 h, the plates were washed three times with PBS, followed by three washes with 0.1% Tween-PBS. The plates were incubated with horseradish peroxidase–conjugated anti–mouse IgA or IgG (1:1,000 dilution [vol/vol] in 0.1% Tween-PBS) for 16 h. After the plate had been washed with PBS six times, antibody-producing cells were visualized with AECB-500 and AECM-100 conjugate solutions (Moss, Inc.). Plates were incubated for 30 min and washed with water. The plates were allowed to dry, and spot pictures were taken with a microscope. To detect CT-B–specific T cells, a CT-B/I-Ab tetramer was prepared and used for flow cytometric analysis, as previously described (Chang et al., 2008).
Cell preparation and RT-PCR.
CD3−CD4+CD45+ cells were isolated from mucosa-associated tissues as previously described (Fukuyama et al., 2006). In some experiments, mononuclear cells were isolated from the TALT, NALT, and NPs of immunized mice by mechanical dissociation (Fukuyama et al., 2002). Total RNA was extracted for RT-PCR as previously described (Shikina et al., 2004). The sequences of primers used were as follows: Id2, (sense) 5′-TCTGAGCTTATGTCGAATGATAGC-3′ and (anti-sense) 5′-CACAGCATTCAGTAGGCTCGTGTC-3′; Rorγt, (sense) 5′-ACCTCCACTGCCAGCTGTGTGCTGTC-3′ and (anti-sense) 5′-TTGTTTCTGCACTTCTGCATGTAGACTGTCCC-3′; Gapdh, (sense) 5′-TGAACGGGAAGCTCACTGG-3′ and (anti-sense) 5′-TCCACCACCCTGTTGCTGTA-3′; Aid, (sense) 5′-GGCTGAGGTTAGGGTTCCATCTCAG-3′ and (anti-sense) 5′-GAGGGAGTCAAGAAAGTCACGCTGGA-3′; and β-actin, (sense) 5′-TGGAATCCTGTGGCATCCATGAAA-3′ and (anti-sense) 5′-TAAAACGCAGCTCAGTAACAGTCC-3′.
Electron microscopy analysis.
Electron microscopy was performed as previously described (Jang et al., 2004). Head tissue containing the tear ducts was prepared and fixed in a solution containing 0.5% glutaraldehyde, 4% paraformaldehyde, and 0.1 M of sodium phosphate buffer (pH 7.6) on ice for 1 h. After washes with 4% sucrose in 0.1 M of phosphate buffer, the tissue was decalcified with 2.5% EDTA solution for 5 d. After three washes, the samples were fixed with 2% osmium tetraoxide on ice for 1 h and dehydrated with a series of ethanol gradients. For scanning electron microscopy, dehydrated tissues were freeze embedded in t-butyl alcohol and freeze dried, and then coated with osmium and observed under a scanning electron microscope (S-4200; Hitachi). For transmission electron microscopy, the tissues were embedded in Epon 812 resin mixture, and ultrathin (70-nm) sections were cut with an ultramicrotome (Reichert Ultracut N; Leica). The ultrathin sections were stained with 2% uranyl acetate in 70% ethanol for 5 min at room temperature and then in Reynold's lead for 5 min at room temperature. Sections were analyzed with a transmission electron microscope (H-7500; Hitachi).
Online supplemental material.
Fig. S1 shows postnatal organogenesis of TALT on BALB/c mice. Fig. S2 shows development of TALT in B cell– or T cell–null mice and in TLR signaling–null conditions. Fig. S3 shows the lymphoid structure of TALT in mice lacking molecules related to lymphoid tissue genesis. Paraffinized sections were prepared from 8-wk-old mice and stained with the indicated antibodies (PNAd and B220) for confocal microscopy analysis. Arrows indicate PNAd-expressing HEVs. Fig. S4 shows the absence of MAdCAM-1 in TALT and NALT. TALT (A) and NALT (B) of 8-wk-old C57BL/6 mice were stained with DAPI and an anti–MAdCAM-1 antibody, and confocal microscopy analysis was performed. PPs of 10-d-old mice were analyzed as a positive control for anti–MAdCAM-1 antibody (C). Fig. S5 shows the independence of TALT genesis in TRANCE-Traf6 signaling. TALT of 2–3-wk-old Trance-deficient and Traf6, Tcrb double-deficient mice was analyzed histologically with hematoxylin and eosin (HE) staining. Traf6+/−, Tcrb−/− mice were examined as a control.
We thank Dr. K. McGhee of the Medical College of Georgia for editorial help.
This work was supported by grants-in-aid from the Ministry of Education, Culture, Sports, Science, and Technology (MEXT), the Ministry of Health and Welfare of Japan and the Global Center of Excellence Program “Center of Education and Research for the Advanced Genome-Based Medicine For Personalized Medicine and the Control of Worldwide Infectious Diseases,” and an “Academic Frontier” project for private universities matching-fund subsidy from MEXT. T. Nagatake, S. Fukuyama, and D.-Y. Kim were supported by research fellowships from the Japan Society for the Promotion of Science for Graduate Students, Young Scientists, and Foreign Researchers, respectively. A.M. Jetten was supported by the Intramural Research Program of the National Institute of Environmental Health Sciences (grant Z01-ES-101586).
The authors declare that they have no competing financial interests.
activation-induced cytidine deaminase
conjunctiva-associated lymphoid tissue
hematoxylin and eosin
high endothelial venule
inhibitor of DNA binding/differentiation 2
isolated lymphoid follicle
lymphoid tissue inducer
mucosal addressin cell adhesion molecule 1
mucosa-associated lymphoid tissue
nasopharynx-associated lymphoid tissue
retinoic acid–related orphan receptor
tear duct–associated lymphoid tissue
TNF receptor–associated factor
TNF-related activation-induced cytokine
Ulex europaeus agglutinin
vascular cell adhesion molecule 1