Correspondence to: Warwick J. Britton, Centenary Institute of Cancer Medicine and Cell Biology, Locked Bag No. 6, Newtown NSW 2042, Australia. Tel:61-2-9515-5210 Fax:61-2-9351-3968 E-mail:wbritton{at}medicine.usyd.edu.au.
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Abstract |
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Although the essential role of tumor necrosis factor (TNF) in the control of intracellular bac-terial infection is well established, it is uncertain whether the related cytokines lymphotoxin- (LT
3) and lymphotoxin-ß (LTß) have independent roles in this process. Using C57Bl/6 mice in which the genes for these cytokines have been disrupted, we have examined the relative contribution of secreted LT
3 and membrane-bound LTß in the host response to aerosol Mycobacterium tuberculosis infection. To overcome the lack of peripheral lymph nodes in LT
-/- and LTß-/- mice, bone marrow chimeric mice were constructed. LT
-/- chimeras, which lack both secreted LT
3 and membrane-bound LTß (LT
1ß2 and LT
2ß1), were highly susceptible and succumbed 5 wk after infection. LTß-/- chimeras, which lack only the membrane-bound LTß, controlled the infection in a comparable manner to wild-type (WT) chimeric mice. T cell responses to mycobacterial antigens and macrophage responses in LT
-/- chimeras were equivalent to those of WT chimeras, but in LT
-/- chimeras, granuloma formation was abnormal. LT
-/- chimeras recruited normal numbers of T cells into their lungs, but the lymphocytes were restricted to perivascular and peribronchial areas and were not colocated with macrophages in granulomas. Therefore, LT
3 is essential for the control of pulmonary tuberculosis, and its critical role lies not in the activation of T cells and macrophages per se but in the local organization of the granulomatous response.
Key Words: lymphotoxin, TNF, tuberculosis, granuloma, lung
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Introduction |
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The control of chronic intracellular bacterial infection is dependent on the activation and expression of cellular immunity (1). In the case of Mycobacterium tuberculosis infection, infected APCs activate T cells in the context of IL-12, leading to a Th1 pattern of T cell responses. Mycobacteria-specific T cells are recruited back to the initial site of infection in the lung (2), where they initiate the cascade of cellular and molecular events that control the infection. The expression of immunity requires the continued recruitment of T cells and macrophages into the lung, the migration and aggregation of these cells to form granulomatous lesions, and the release of IFN- by T cells (3), which in concert with TNF activate mycobactericidal mechanisms in infected macrophages (4). Granulomatous lesions are the hallmark of the inflammatory response to mycobacteria and are essential to control infection (1). The cytokine and chemokine signals modulating this inflammatory response are poorly understood, although TNF plays a critical role in orchestrating the movement of these cells once they enter infected tissues (5).
Lymphotoxin (LT) comprises two members of the TNF superfamily, LT and LTß. LT
is active as a secreted homotrimeric molecule (LT
3, also known as TNF-ß) (6), which binds not only to both of the TNF receptors (TNFRI and TNFRII) (7) (8) but also to the newly identified herpes virus entry mediator (HVEM) receptor (9). In comparison to TNF, which is produced by a wide range of cell types, LT
3 is produced primarily by CD4+ T cells, B cells, and NK cells (10). As LT
3 and TNF bind to TNFRI with similar affinity (11) and have
30% homology in amino acid sequence (12), the functional activity for LT
3 independent of TNF has been unclear. By contrast, LTß is a heterotrimeric molecule that exists in two forms, the major being LT
1ß2 and the minor LT
2ß1 (13). Both forms of LTß bind the unique LTß receptor (LTßR) (14), and LTß signaling through LTßR is essential for the formation of the peripheral lymphoid organs (15). Mice deficient in either LTß or LTßR lack peripheral lymph nodes and Peyer's patches and display disorganized splenic architecture.
Recently, the activity of LT3 during immune responses has been reexamined. Transgenic expression of the LT
gene under control of the rat insulin promoter led to the formation of chronic inflammatory lesions at the sites of transgene expression (16). These lesions resembled secondary lymphoid tissue, not only in their cellular composition and structure, but also in their ability to respond to Ag. Interestingly, TNFRI was the receptor mediating the formation of these lesions. LT
- and LTß-deficient mice have also been employed to investigate the independent functions of LT
3 and LTß in inflammatory pathologies. Targeted disruption of the gene for LT
results in loss of both secreted LT
3 and cell surface LTß complexes, whereas targeted disruption of the LTß gene results in loss of only cell surface LTß. Disruption of either LT
or LTß also results in the phenotypic loss of secondary lymphoid tissue. Using radiation bone marrow chimeras with gene-targeted and wild-type (WT) animals, normal secondary lymphoid organ function has been reconstituted, enabling the study of cytokine effector function at the target tissue level (17). In this manner, LT
3 was shown to have no independent role in the cellular inflammation or clinical course of experimental autoimmune encephalomyelitis (EAE), a model of tissue-specific autoimmune disease (17).
To determine whether LT3 or LTß independently contribute to the host response to M. tuberculosis infection, we have constructed radiation bone marrow chimeras, using as donors C57Bl/6 mice in which the genes for LT
or LTß have been disrupted. Transfer of bone marrow into irradiated mice resulted in repopulation of peripheral lymphoid tissues with leukocytes deficient in both LT
3 and LTß or deficient in LTß alone. Analysis of low dose aerosol M. tuberculosis infection in these mice demonstrated the essential role of LT
3 in the host response to mycobacterial infection. Although there was evidence of induction of Ag-specific T cell responses and activation of macrophages, mycobacterial growth was unrestrained, leading to the death of LT
-/- chimeric mice. By contrast, LTß-/- chimeric mice were able to control the infection normally. The inflammatory response in the lungs of LT
-/- chimeric mice was markedly abnormal, with failure to form distinct granulomas, indicating that LT
3 has an essential role in the cellular recruitment and organization underlying this process.
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Materials and Methods |
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Mice.
C57Bl/6 (Ly5.2), C57Bl/6.Ly5.1, and C57Bl/6.RAG-1-/- mice were obtained from Animal Resources Centre, and LT and LTß gene knockout mice on a C57BL/6 background have been previously described (17) (18). Adult (>6 wk old) mice were used in all experiments. Mice were housed under specific pathogenfree conditions at the Centenary Institute animal facility, or after infection in a Level 3 physical containment facility.
Generation of Radiation Bone Marrow Chimeras.
Radiation bone marrow chimeric mice were generated as in Riminton et al. (17). To monitor engraftment, C57Bl/6.Ly5.1 bone marrow was transferred into C57Bl/6.Ly5.2 recipient mice. Peripheral blood was analyzed by flow cytometry for the presence of the Ly5.1 congenic marker, and reconstitution was considered satisfactory when >95% of leukocytes were of donor type.
Aerosol Infection of Mice with M. tuberculosis.
A Middlebrook airborne infection apparatus (Glas-Col Inc.) delivered 100 bacilli of M. tuberculosis H37Rv (American Type Culture Collection no. 27294) to each mouse. The number of viable bacteria in target organs was determined by plating serial dilutions of organ homogenates on supplemented Middlebrook 7H11 nutrient agar (Difco Labs.). The data are expressed as the log10 of the mean number of bacteria recovered per organ.
Lung Preparations.
Mice were killed at several time points after aerosol M. tuberculosis infection. One lung was homogenized and serial dilutions spread on duplicate quadrants of bacterial plates. The other lung was minced and incubated with collagenase (10 U/ml; Worthington) and DNase (13 µg/ml; Boehringer Mannheim) to produce a cell suspension, as previously described (5).
Phenotypic Analysis of Pulmonary Infiltrates.
mAbs used for flow cytometry were: CD4 (CT-CD4; Caltag Laboratories), CD8 (CT-CD8; Caltag Laboratories), CD16/32 (2.4G2; BD PharMingen), CD44 (IM 7.8.1; Sigma-Aldrich), CD45RB (16A; Sigma-Aldrich), Ly-6G (RB6-8C5; BD PharMingen), biotinylated anti-Ly5.1, and streptavidinPE (Sigma-Aldrich).
T Cell Responses to Mycobacterial Ags.
Mediastinal lymph node or lung cell suspensions were suspended in culture medium (RPMI-1640; Sigma-Aldrich), 10% FCS (CSL Bioscience), 2 mM L-glutamine (Flow Laboratories), 50 mM 2-ME (Sigma-Aldrich), 10 mM HEPES (Sigma-Aldrich), and 10 mM sodium bicarbonate (BDH) and cultured alone or with purified protein derivative (PPD; 10 µg/ml) of M. tuberculosis (Statens Seruminstitut) for 72 h, and total IFN- production was measured by capture ELISA (5). The frequency of IFN-
producing cells was determined by ELISpot assay, as previously described (5). Delayed-type hypersensitivity (DTH) reactions were determined as the difference in swelling between PBS-injected footpads and PPD-injected footpads, as described in reference (5).
Generation of Bone Marrowderived Macrophages.
Macrophages were derived from bone marrow by culture in medium supplemented with 20% L929 fibroblast culture supernatant for 7 d at 37°C. Cells were stimulated with LPS (10 µg/ml; Sigma-Aldrich) and IFN- (100 U/ml; Boehringer Mannheim) for 72 h. In infection studies, cells were prestimulated with IFN-
(100 U/ml) or culture medium for 16 h and infected with M. tuberculosis H37Rv (multiplicity of infection 1:1), and the supernatants were harvested after 54 h.
Nitrite Measurements.
Serum nitrite was obtained by reducing serum nitrate to nitrite with nitrate reductase, and the nitrite concentrations in culture supernatants levels were determined using the Greiss reagent (reference (19); 3% phosphoric acid, 1% p-aminobenzene-sulphonamide, 1% n-1-napthylethylenediamide; Sigma-Aldrich).
Measurement of Bioactive TNF and Analysis of TNF mRNA by Reverse Transcriptase PCR.
Levels of biologically active TNF were measured using the WEHI 164 cytotoxicity assay (31). For analysis of TNF mRNA, total lung RNA was prepared from 3 wk postinfectionperfused lungs using RNAzol B (Tel-Test). cDNA was synthesized using SUPERSCRIPT II RNase H reverse transcriptase (RT; GIBCO BRL) and analyzed by RT-PCR using primers and methods as previously described (17).
Histological and Immunohistochemical Analysis.
Lung and liver tissues were fixed in 10% neutral buffered formalin, embedded in paraffin blocks, sectioned at 4 µm, and stained with hematoxylin and eosin. Coded slides were assessed blind on 37 criteria for differences in cellular infiltrate. A granuloma in the peripheral lung was defined as a collection of 10 or more macrophages and T lymphocytes.
Statistical Analysis.
Differences between the mean number of CFUs, number of granulocytes, and levels of nitrite and TNF were analyzed by Student's t tests.
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Results |
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LT- and LTß-deficient Chimeric Mice Generate Normal T Cell Responses after M. tuberculosis Infection.
To confirm the immune competence of the chimeric mice, their ability to mount comparable mycobacterial Ag-specific T cell responses after aerosol M. tuberculosis infection was examined. Mediastinal lymph node cells from all chimeric groups produced significant and comparable amounts of IFN- after both PPD stimulation (Fig 1 A) and mitogenic stimulation (data not shown). The frequency of Ag-specific IFN-
producing cells in both the lymph nodes and lungs of chimeric mice was also analyzed. All chimeric mice had comparable numbers of IFN-
producing cells both in the lungs (Fig 1 B) and in the draining lymph nodes (data not shown). The ability of the chimeric mice to mount Ag-specific DTH reactions was measured at 4 wk after infection. Chimeric mice were challenged with 10 µg of PPD in one footpad and the vehicle control in the other. Chimeric mice from all groups mounted similar DTH responses to mycobacterial proteins (Fig 1 C). Therefore, the deficiencies in either soluble or membrane forms of LT do not affect the potential of these chimeric mice to mount Ag-specific T cell responses after infection with M. tuberculosis.
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LT-deficient Chimeras Rapidly Succumb to Aerosol Tuberculosis.
Chimeric mice and normal unmanipulated WT mice were infected with virulent M. tuberculosis, and their clinical condition and bacterial growth was monitored over time. LT-/- chimeras appeared healthy to day 28 but then rapidly deteriorated, and all succumbed by day 38 (Fig 2 A). By contrast, both WT and LTß-/- chimeras controlled the same infectious dose and survived for >150 d. The number of mycobacteria recovered from the lungs of LT
-/- chimeras was comparable to that in WT chimeras for the first 3 wk of infection but was significantly increased from this time. At the time of death, there were 3log10 more bacteria in the lungs of LT
-/- chimeras compared with WT chimeras (Fig 2 B; P < 0.0001). In contrast, LTß-/- chimeras had comparable bacterial loads in the lungs to WT chimeras over the course of the infection. There was also increased dissemination of organisms into the spleens (Fig 2 C) and livers (Fig 2 D) of LT
-/-, but not LTß-/-, chimeras compared with WT chimeras. M. tuberculosisinfected control WT chimeric mice and normal WT mice showed comparable rates of survival and bacterial loads (data not shown).
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Recruitment of Leukocytes in Chimeric Mice.
The recruitment of leukocytes to the sites of infection is a critical event in the host response to tuberculosis. Therefore, the numbers of different lymphocyte subpopulations in the lungs were assessed over the course of infection. Comparable numbers of CD4+ (Table 1) and CD8+ (data not shown) T cells were recruited into the lungs of LT-/-, LTß-/-, and WT chimeric mice over the course of infection. Similar numbers of B lymphocytes were also observed (data not shown). To investigate the activation state of these T cells, the expression of CD44 and CD45RB was examined on CD4+ T cells. CD4+ T cells from LT
-/-, LTß-/-, and WT chimeric mice expressed similar levels of CD44highCD45RBlow expression (data not shown). Interestingly, the numbers of granulocytes (Ly-6G+ cells) recruited to the lungs of the chimeric mice differed. At 4 wk after infection, there were significantly more granulocytes (P < 0.005) in the lungs of LT
-/- chimeric mice compared with both WT and LTß-/- chimeric mice (Table 1).
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LT-deficient Chimeric Mice Produce Normal Amounts of Reactive Nitrogen Intermediates.
The antimicrobial mechanisms of activated mouse macrophages include the production of reactive nitrogen intermediates (RNI). Therefore, nitrite levels in the sera of the chimeric mice were analyzed throughout the course of infection to determine if LT3 plays a critical role in regulating this antimicrobial mechanism. LT
-/-, LTß-/-, and WT chimeric mice all had similar levels of serum nitrite (Fig 3 A). To determine if macrophages deficient in LT
and LTß have the potential to produce comparable amounts of RNI to WT macrophages, bone marrowderived macrophages from the three types of mice were generated. These macrophages were stimulated with LPS and IFN-
or were infected with M. tuberculosis, with and without pre-stimulation with IFN-
(Fig 3 B). Macrophages derived from LT
-/- and LTß-/- bone marrow produced amounts of RNI comparable to those of WT macrophages.
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TNF mRNA Expression and TNF Production by Macrophages Is Normal in LT-deficient Mice.
To exclude the possibility that the failure of LT-/- chimeric mice to control infection was due to a reduced production of TNF, both the expression of mRNA for TNF during infection of chimeric mice and the production of TNF by LT
-/- and LTß-/- macrophages were examined. Comparable levels of TNF mRNA was expressed in the lungs of LT
-/-, LTß-/-, and WT chimeric mice during infection (Fig 3 C). Macrophages derived from LT
-/-, LTß-/-, and WT mice produced similar amounts of TNF after either stimulation with LPS and IFN-
or infection with M. tuberculosis after prestimulation with IFN-
(Fig 3 D).
Granulomatous Response in LT-deficient Chimeric Mice.
The lungs of the different chimeric mice were examined histologically to determine whether the rate of development and pattern of cellular responses differed across the groups of chimeric mice. In WT chimeras and LTß-/- chimeric mice, the granulomatous response resembled that seen in normal WT mice after aerosol tuberculosis, so that by 4 wk after infection the granulomas in these groups were 0.40.8 mm in diameter (Fig 4A and Fig C). These granulomas consisted of intact macrophages, some lymphocytes, and only occasional neutrophils, with no necrosis (Fig 4D and Fig F). The lesions that formed in the lungs of LT-/- chimeric mice were markedly different. The peripheral lung lesions had twice the diameter (Fig 4 B) and consisted of collections of neutrophils and fewer macrophages than WT chimeric mice (Fig 4 E). Lymphocytes were absent from the lesions (Fig 4 E), and a moderate amount of necrosis was evident. In contrast to WT and LTß-/- chimeras, the lymphocytes in LT
-/- chimeras were restricted to perivascular and peribronchial regions (Fig 4 E). This pattern was confirmed by immunohistochemical identification of the lymphocytes with anti-CD3 staining (data not shown).
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Discussion |
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Although the genes for LT3 and TNF were identified at the same time (12), the functions of TNF have been more clearly defined than those for LT
3. LT
3 has been considered either as a mediator of inflammation or a functionally redundant form of TNF (20). Recently, with the advent of recombinant forms of LT
3, in vitro studies have delineated proinflammatory properties for LT
3 (21), although in vivo activity of LT
3, independent of TNF, has not been defined. This study demonstrates, for the first time, an essential function for secreted LT
3, but not membrane-bound LTß, in the control of pulmonary tuberculosis. TNF production was not impaired in the LT
- and LTß-deficient chimeric mice, with TNF mRNA being produced in the lungs of M. tuberculosisinfected LT
-/- and LTß-/- chimeric mice (Fig 3 C). Importantly, macrophages from LT
- and LTß-deficient mice demonstrated normal TNF secretion in response to both nonspecific activation and infection with M. tuberculosis (Fig 3 D). Moreover, LTß-deficient chimeric mice, produced in a similar fashion to LT
-/- chimeras, controlled M. tuberculosis infection in the same manner as chimeras reconstituted with WT bone marrow (Fig 2 A). Therefore, LT
3 is essential to control this chronic bacterial infection and acts independently of TNF, possibly through an additional receptor or mechanism. LT
3 has the potential to act at a number of steps in the host response to tuberculosis.
First, LT3 deficiency may cause T cell dysfunction. However, T cell activation and IFN-
release was normal in all chimeric groups (Fig 1). Second, LT
3 may participate in the T cellmediated activation of macrophage bactericidal mechanisms, such as the induction of inducible nitric oxide synthase (iNOS) and production of RNI. IFN-
synergizes with TNF (22) or LT
3 (23) to produce maximal activation of murine macrophages and the production of RNI, which have mycobactericidal activity both in vivo and in vitro (22). Both TNF and LT
3 can induce in vitro the nuclear translocation of nuclear factor (NF)-
B, resulting in the induction of iNOS gene transcription (24) (25). During M. tuberculosis infection, WT and LT
-/- chimeric mice demonstrated comparable levels of serum nitrite (Fig 3 A). Also, macrophages derived in vitro from LT
-/- and WT bone marrow produced similar levels of nitrite after nonspecific activation or infection with mycobacteria (Fig 3 B). Therefore, reduced capacity for macrophage activation, as measured indirectly by increased nitric oxide production, does not explain the susceptibility of LT
-/- chimeric mice to tuberculosis.
Third, LT3 may contribute to the inflammatory component of the effector response to mycobacterial infection. A striking feature of the LT
-/- chimeric mice was the failure to develop a normal granulomatous response after mycobacterial infection. Containment of M. tuberculosis infection in the lungs requires the recruitment of CD4+ and CD8+ T cells across the pulmonary endothelium, leukocyte migration through the infected tissues, and the colocalization of macrophages and lymphocytes to form granulomas. LT
-/- and WT chimeras displayed equivalent accumulation of T cells in the lungs (Table 1), and these cells showed similar patterns of activation/memory marker expression (data not shown) and IFN-
production (Fig 1). In the LT
-/- chimeras, however, the lymphocytes accumulated in the perivascular and peribronchial regions of the lung and failed to migrate into the infected tissues. As a result, the well defined granulomas evident in WT chimeras were replaced by large accumulations of neutrophils and necrotic material. These changes in cell migration and granuloma formation in LT
-/- chimeric mice may relate to the recently described in vitro proinflammatory activities of LT
3. Recombinant murine (rm)LT
3 induced the expression of the cell adhesion molecules vascular cell adhesion molecule-1, intercellular adhesion molecule-1, E-selectin, and mucosal addressin cell adhesion molecule on endothelial cells in vitro (26). Furthermore, rmLT
3 induces the expression of T cell and monocyte attracting chemokines RANTES (regulated upon activation, normal T cell expressed and secreted), IFN-
inducible protein-10, and monocyte chemoattractant protein-1 (26). Therefore, LT
3 has the potential to regulate the chemotactic signals that organize the cells into a mature granuloma, even though it is not a chemoattractant itself. As few studies into the chemokine-producing activity of LT
3 have been undertaken, it is possible that LT
3 may induce as yet unidentified chemokines and cytokines. Interestingly, LT
deficiency did not affect the acute cellular inflammation in the brain during EAE (18). This may represent differences in the intensity and chronicity of the inflammatory response, which are stronger and more prolonged after aerosol tuberculosis than that occurring during EAE, in addition to differences in the responding cell types and the organ involved in the inflammatory response.
Another facet of the dysregulated inflammatory response was the marked increase in granulocytes in the lungs of LT-/- compared with LTß-/- chimeric and WT chimeric control mice (Table 1). This contrasts with the mild influx of neutrophils that may have a beneficial role early after M. tuberculosis infection in normal mice (27). In other genetically deficient mice with increased susceptibility to M. tuberculosis, such as TNF-/- and IFN-
-/- mice, a similar large influx of neutrophils occurs (5) (28). The accumulation of activated neutrophils may contribute to the marked damage to the lungs during infection. Neutrophil migration and activation contributes to lung injury in acute respiratory distress syndrome patients (29). The oxidative products cause endothelial and epithelial cell injury, leading to increased protein permeability into alveoli and impaired lung function. The combination of tissue necrosis and the increased protein exudation in areas without tissue destruction contributed to the death of these mice.
In contrast to the absolute requirement for LT3 to control pulmonary tuberculosis, chimeric mice deficient in only membrane-bound LTß were able to mount a normal granulomatous response and contained M. tuberculosis infection. A recent study in which the action of LTß was blocked with a LTßRIg fusion protein during M. bovis (BCG) infection, found a modest, two- to threefold increase in bacterial numbers (30). These modest effects contrast with the profound susceptibility of LT
-/- chimeras, which showed greater than 1,000-fold increases in bacterial loads (Fig 3). Furthermore, any effects of LTßRIg therapy may be due to the neutralization of not only LTß, but also the cytokine LIGHT, which also signals through LTßR (31).
LT3 has been considered to mediate its activity through TNFRI and TNFRII. Nevertheless, TNF, which was expressed normally in the lungs of the LT
-/- chimeric mice (Fig 3 C), was unable to compensate for the lack of LT
3. Therefore, it is possible that LT
3 is signaling through an additional receptor. One possibility is the HVEM receptor, which has a wide tissue distribution being expressed predominantly on T cells, B cells, and monocytes (32). Signaling through HVEM not only induces activation of the transcription factors NF-
B and activator protein 1 (33) but also is thought to play a role in T cell activation (34). An alternate possibility is that LT
3 may be signaling through the same receptors as TNF, but the timing and site of production of LT
3 may be different to that for TNF. Although T cells, which are the major source of LT
3, are also able to produce TNF, the relative importance of T cellderived TNF, as compared with macrophage-derived TNF, in the immune response to tuberculosis is unclear. In summary, this model of chimeric mice deficient in individual members of the TNF/LT family of cytokines has identified an independent function for LT
3 in the host control of aerosol tuberculosis and will permit the further dissection of the mode of action of LT
3.
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Acknowledgements |
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This study was funded by the National Health and Medical Research Council of Australia. The support of the New South Wales Health Department through its research and development infrastructure grants program is gratefully acknowledged. D. Roach is a recipient of a University of Sydney Postgraduate Award.
Submitted: 5 July 2000
Revised: 8 November 2000
Accepted: 20 November 2000
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References |
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