By
From the * Department of Neurosurgery and Section of Clinical Immunology, University Hospital
Zürich, CH-8091 Zürich, Switzerland; § Swiss Federal Institute of Technology, Institute of Toxicology,
CH-8603 Schwerzenbach, Switzerland;
Department of Neurology and ¶ Department of Pathology,
Division of Neuropathology, University of Pennsylvania, Philadelphia, Pennsylvania 19104
Immunization of mice with myelin components results in experimental autoimmune encephalomyelitis (EAE), which is mediated by myelin-specific CD4+ T cells and anti-myelin antibodies. Tumor necrosis factor (TNF-
) and lymphotoxin
(LT-
) are thought to be involved
in the events leading to inflammatory demyelination in the central nervous system. To ascertain this hypothesis 129 × C57BL/6 mice with an inactivation of the tnf and lta genes (129 × C57BL/6
/
) and SJL/J mice derived from backcrosses of the above mentioned mutant mice
(SJL
/
) were immunized with mouse spinal cord homogenate (MSCH) or proteolipid protein. Both 129 × C57BL/6
/
mice and SJL
/
mice developed EAE. In SJL
/
mice immunized with MSCH, a very severe form of EAE with weight loss, paralysis of all four limbs, and
lethal outcome was observed. The histologic hallmark was an intense perivascular and parenchymal infiltration with predominantly CD4+ T cells and some CD8+ T cells associated with
demyelination in both brain and spinal cord. These results indicate that TNF-
and LT-
are
not essential for the development of EAE.
Experimental autoimmune encephalomyelitis (EAE) is a
T cell-mediated inflammatory disease of the central
nervous system (CNS). It is induced in experimental animals by either active immunization with CNS homogenate,
myelin proteins, or the adoptive transfer of myelin basic
protein (MBP)-specific CD4+ T cell lines. In SJL mice immunized with myelin components, the histologic hallmarks
of the disease comprise a perivascular and parenchymal inflammation with infiltration of CD4+ T cells, activation of
macrophages and microglial cells, and various degrees of
demyelination. Recent work has suggested that TNF- and
lymphotoxin (LT)- In this study we have investigated the influence of TNF-
and LT- Mice.
Female SJL/J (H-2s) mice were purchased from Biological Research Laboratories Ltd. (Füllinsdorf, Switzerland). 129 SV/EV × C57BL/6 with inactivated tnf and lta genes (called 129 × B6 Induction of EAE.
Mice were immunized either with mouse
spinal cord homogenate (MSCH; 18) or proteolipid protein (PLP)
peptide in CFA according to a modified method of Brown and
McFarlin (19) and Al-Sabbagh et al. (20), respectively. On day 0, each mouse received 0.3 ml of a mixture of 5.0 mg MSCH in
0.15 ml PBS (pH 7.4) or 0.2 mg PLP peptide 139-151 (HSLGKWLGHPDKF, synthesized by Chiron Technologies, Clayton,
Victoria, Australia) dissolved in 0.15 ml PBS and 0.75 mg of Mycobacterium tuberculosis, (H37Ra; Difco, Detroit, MI) in 0.15 ml
incomplete Freund's adjuvant (Difco). The inoculum of 0.3 ml
was injected at 50 µl in each hind footpad and in each of four
spots on the back (two anterior, two posterior, on each side). On
the day of immunization and 2 d later, 1010 heat-inactivated Bordetella pertussis (Calbiochem Corp., La Jolla, CA) were injected
intraperitoneally in 0.4 ml pertussis diluent (0.015 M Tris, 0.5 M
NaCl, and 0.017% (vol/vol) Triton X-100 in distilled water; reference 21).
Clinical Evaluation of EAE.
After the encephalitogenic challenge, mice were monitored, weighed daily, and disease severity
was scored on a scale of 0 to 5, with 0.5 points for intermediate
clinical findings. The score was designated as follows: 0, no detectable signs of EAE; 1, weakness of the tail; 2, definite tail and
partial hind limb paralysis; 3, complete paralysis of the hind limbs
often associated with incontinence; 4, total paralysis of hind and
forelimbs (mice at grade 4 for >1 d were euthanized); 5, moribund or death.
Histological Analysis.
Animals were perfused under anesthesia
through the heart either with Ringer's solution (for cryosections,
flow cytometry, and reverse transcriptase (RT)-PCR) or with 4%
paraformaldehyde in buffered PBS (for paraffin sections) and spleen,
brain, and spinal cord were dissected out. Paraffin-embedded tissue sections were stained with hematoxylin and eosin and for the
degree of demyelination with Luxol fast blue. Tissue-Tek-embedded sections were stained with anti-CD4 mAb (GK1.5; PharMingen), anti-CD8 mAb (5H10-1; PharMingen), anti-F4/80 mAb
(C1:A3-1; Serotec Ltd., Oxford, U.K.) and corresponding isotype-matched primary mAbs. The labeled streptavidin-biotin
technique (DAKO Diagnostics AG, Zug, Switzerland) was chosen for visualization.
RT-PCR Analysis for TNF- Irrespective of whether the tnf and lta genes are inactivated or not, 129 × C57BL/6 mice, which had been immunized with MSCH, developed a mild form of EAE with
mean clinical scores of 1 (Table 1). The disease started between days 11 and 17. None of the mice progressed to severe EAE. Histologic analysis revealed a few perivascular cuffs, predominantly in spinal cord, but no demyelination.
The same clinical and histological picture emerged when
studying SJL/J mice which were immunized with MSCH.
However, when using PLP as the immunogen, SJL/J mice
suffered from a more severe form of EAE, which progressed to a mean disease score of 2.2 ± 1.2 (Table 1).
Mice with severe disease (clinical score >2) had histologic evidence for perivascular and parenchymal infiltration of
CD4+ T cells and demyelination (data not shown).
Table 1.
>EAE in TNF and LT-, also known as TNF-
, may play a
pivotal role in EAE, since both TNF- and LT-
messenger
RNA and protein have been identified in the CNS in the
acute phase of the disease (1). Furthermore, the administration of soluble type I receptor of TNF, as well as antibodies to TNF- and LT-
, prevent the development of
EAE in rodents immunized with MBP or injected with encephalitogenic T cells (6). The ability of MBP-specific T
cells to transfer the disease was found to be positively correlated with the amount of TNF- and/or LT-
produced
by the T cells (10). TNF-
is produced in high amounts by
astrocytes from EAE-susceptible Lewis rats, but not from
EAE-resistant Brown-Norway rats (11). Demyelination has
been suggested to be due to the action of TNF- and LT-
because both cytokines mediate oligodendrocyte and myelin damage in vitro (12, 13). Likewise, upon overexpression in
the CNS of transgenic mice, TNF-
causes demyelination
(14). Furthermore, injections of TNF-
lead to prolongation
of EAE or can induce relapses in SJL mice that have been
partially or completely recovered from acute EAE (15, 16).
on the course of EAE using mice having a simultaneous deletion of the tnf and lta genes (17). Despite previous evidence for a pathogenetic role of both TNF- and
LT-
in EAE, we find TNF- and LT-
double-deficient
mice to be highly susceptible to acute EAE.
/
, H-2b) have been described recently (17) and were bred
under specific pathogen-free (SPF) conditions. These mice were
backcrossed onto the SJL/J (H-2s) background for six generations
and are called SJL
/
throughout this paper. Mice homozygous
for inactivation of both the tnf and lta genes were obtained by intercrossing heterozygous animals. Homozygous animals were
identified by a diagnostic PCR on genomic DNA described for
the 129 × B6
/
mice (17) and a negative PCR result using the
following primer pair: 5
-TCT CAT CAG TTC TAT GGC
CC-3
and 5
-GGG AGT AGA CAA GGT ACA AC-3
, proving the lack of the deleted genes. The knockout phenotype was
also ascertained by the lack of lymph nodes and altered splenic
microarchitecture (17). Flow cytometric analysis of splenocytes
showed SJL
/
mice to be predominantly of the H-2b haplotype
(FITC anti-mouse H-2Db, clone KH95; PharMingen, San Diego,
CA), and not H-2s (FITC anti-mouse H-2Ds, clone KH43; PharMingen). Animals were housed under SPF conditions up to 8 wk of age and then transferred to conventional housing where
they were immunized at 10-20 wk of age. Paralyzed animals were
given easy access to food and water.
, LT-
, IFN-
, and GAPDH.
Total RNA was isolated from frozen tissue according to Chomczynski and Sacchi (22). 10 µg of total RNA was mixed with 2 µg oligo dT primer (Boehringer Mannheim, Rotkreuz, Switzerland) in a volume of 10 µl RNase free water and denatured for 5 min at 70°C. Cooling on ice allowed annealing of RT primers.
Reverse transcription was performed in a total volume of 30 µl
containing 6 nmol dNTPs, 0.3 nmol dithiothreitol, 25 units
RNAguard (Pharmacia, Dübendorf, Switzerland) and 100 U
Moloney murine leukemia virus RT (GIBCO, Basel, Switzerland) for 4 h at 37°C. The reaction was terminated by incubation
at 95°C for 5 min followed by 5 min at 4°C. The PCR reaction
mix consisted of 2 µl RT reaction mix, 2.5 µl PCR buffer, 2.5 µl 12 mM MgCl2, 2 µl 10 µM primer mix, 2.5 µl 2 mM dNTP
mix, and 0.5 units Taq polymerase (0.5 U in 11.4 µl; Appligene,
Oncor, Basel, Switzerland) were added at 55°C after an initial denaturation at 95°C for 1 min. A two-step PCR with denaturation
for 15 s at 94°C and annealing for 30 s at 55°C was done for 30 or
35 cycles with a final extension at 72°C for 5 min. PCR products
were visualized in 2% agarose gels containing ethidium bromide.
The following mouse specific primers were used for PCR: TNF-
sense primer, 5
-TCTCATCAGTTCTATGGCCC-3
; TNF-
antisense primer, 5
-GGGAGTAGACAAGGTACAAC-3
; LT-
sense primer, 5
-CCCATCCACTCCCTCAGAAG-3
; LT-
antisense primer, 5
-CGCACTGAGGAGAGGCACAT-3
; IFN-
sense primer, 5
-GCTCTGAGACAATGAACGCT-3
; IFN-
antisense primer, 5
-AAAGAGATAATCTGGCTCTGC-3
;
GAPDH sense primer, 5
-CCACCACCCTGTTGCTGTAG3
; GAPDH antisense primer, 5
-CCATCAACGACCCCTTCATT-3
.
-deficient mice
Genotype
Haplotype
H-2
TNF-
LT-
Age
Immunized
with
Number
sick/total*
Mean day
of onset
Mean max.
clinical score§
Mortality
wk
%
129 × B6
b
+/+
+/+
11
MSCH
5/5
14.6 ± 0.9
1.1 ± 0.2
0
129 × B6
b
/
/
11
MSCH
5/5
13.8 ± 1.1
1.0 ± 0
0
SJL/J
s
+/+
+/+
12-15
MSCH
3/8
15.7 ± 1.5
1.0 ± 0
0
SJL/J
s
+/+
+/+
10-12
PLP
8/8
12.3 ± 1.3
2.2 ± 1.2
25
SJL/J
b
/
/
15-20
MSCH
8/8
13.0 ± 2.3
3.9 ± 1.6
100
SJL/J
b
/
/
12-15
PLP
6/6
16.3 ± 3.7
1.8 ± 1.3
16.7
*
Number of animals with clinical signs per total in experiment.
Day of onset of clinical signs (mean ± SEM).
§
Based only on those animals with clinical disease (mean ± SEM).
To investigate the influence of TNF- and LT- in the
prototype mouse model of EAE, the TNF- and LT-
double-deficient (129 × B6
/
) mice were backcrossed into
SJL/J. In these SJL
/
mice, the extent of disease was comparable when immunized with PLP (Table 1). However,
immunization of SJL
/
mice with MSCH resulted in a
dramatic acute form of EAE. Clinically, all eight mice
showed the development of an ascending paralysis affecting
the tail and all four limbs, which uniformly led to death of
the animals. Their weights, which were monitored at daily intervals, were found to increase from 21.7 ± 2.7 g at the
day of immunization to a maximum of 23.3 ± 2.1 g between days 9 and 13. Thereafter weight loss was dramatic,
with a 17% decrease at the day of death of the animal
(mean ± SEM: 19.4 ± 2.9 g). The development of
cachexia in EAE is a well-established feature and may be
attributed to excessive production of TNF, which has been named cachectin due to its capability to initiate weight loss when injected into mice (23). However, the observation of
cachexia in TNF- and LT-
-deficient mice with EAE shows
that loss of weight is due to other mechanisms, e.g., dysfunction of brain centers regulating food intake.
Histologic examination of SJL/
mice immunized with
MSCH and a disease score of 3 to 5 showed perivascular
and parenchymal cell infiltrates and demyelination in both
brain and spinal cord. Demyelination was patchy and confined to areas of cell infiltrates. In SJL
/
mice with EAE
induced by immunization with PLP, there was only minimal demyelination despite impressive cellular infiltrates. By
immunohistochemistry, the infiltrates were found to consist mainly of CD4+ T and some CD8+ T lymphocytes
(Fig. 1).
As expected, TNF- and LT- transcripts as measured by
RT-PCR were absent in brain, spinal cord, and spleen in
the diseased mutant mice (Fig. 2). In agreement with other
reports, the acute phase of EAE in the wild-type controls is
paralleled by expression of both cytokine genes in the CNS
(1). No difference was noted when assessing the expression of the IFN-
gene, which was also detected in the
CNS in TNF- and LT-
knockout mice (Fig. 2). The detection of expression of IFN-
in mice with severe EAE is
of note since evidence is accumulating that IFN-
has a
rather beneficial influence on the disease course. Genetic
inactivation of the IFN-
receptor gene rendered EAEresistant mice susceptible (24). Likewise, a more aggressive
disease is observed in IFN-
knockout mice (25, 26).
Our results are remarkable for two reasons. First, it is interesting that TNF- and LT- deficient mice are able to
generate an autoimmune response to CNS myelin. This
finding was not per se to be expected since TNF- and
LT-
-deficient mice not only have an abnormal spleen microarchitecture, blood lymphocytosis, and absence of lymph
nodes, but also functional alterations (17). These include
defects in T cell-dependent and -independent immune responses against sheep red blood cells and dinitrophenol-alanyl-glycyl-glycyl-Ficoll, respectively, and a corresponding
lack of germinal center formation (27, 28). In addition the
CTL response to vaccinia virus and lymphocytic choriomeningitis virus was found to be reduced (17). Since after
in vivo priming the secondary CTL response to lymphocytic choriomeningitis virus in vitro was much more pronounced, it has been suggested that in vivo preformed virus-specific precursor CTL require a prolonged activation
period in vitro to become competent effector cells. On the
humoral site, the SRBC response in TNF- and LT-
-deficient mice was reduced for IgM, IgG1, and IgG2b class Igs.
These may be of importance since antimyelin antibodies
led to demyelination in T cell adoptive transfer EAE (29).
However, recent experiments with genetically B cell-deficient mice that were immunized with an MBP encephalitogenic peptide have shown that B cells are not required
for the activation of encephalitogenic T cells, and hence
the induction of EAE (30).
The data presented here provide evidence that autoimmunity to myelin can be induced in the absence of TNF-
and LT- and in the context of the above mentioned
structural and functional deficiencies of the immune system
present in these mutant mice. The second feature of interest from our data is the observation that the autoimmune
response to CNS myelin leads to EAE with CNS inflammation and demyelination. This is in contrast to the expectations which are based on (a) detection of TNF- and LT-
at the lesion site in EAE, (b) the induction of relapses of
EAE by injection of TNF-
, and (c) prevention of EAE by
anti-TNF antibodies or soluble TNF type I receptors (1-
16). The demonstration of CD4+ T cells in CNS lesions of
TNF- and LT-
knockout mice with EAE indicates the
generation of sufficient numbers of autoimmune CD4+ T
cells, which are able to adhere to CNS endothelium and to
penetrate into the tissue. Thus, these steps, which are required for induction of EAE, are independent of the action
of TNF- and LT-
. Alternatively, in their absence, other
cytokines may compensate for the defect. It is of note that
three other studies did not come to the conclusion that
TNF- and LT-
function as key mediators in EAE. In SJL
and B10.PL mice immunized with synthetic MBP peptides, spinal cord lesions were negative for cells expressing
TNF (31). Furthermore, TNF delivered by using a recombinant vaccinia virus system did not enhance, but rather inhibited the development of EAE (32). In the same experimental paradigm, anti-TNF antibodies either enhanced,
had no effect or inhibited EAE, depending on the antibody investigated (21, 32). Thus, the antibodies used in different studies may show variable cross-reactivity with other immunomodulating molecules of the TNF superfamily. In mice
with Theiler's virus encephalomyelitis, the administration
of rTNF dramatically reduced the extent of demyelination
without influencing the CNS virus titers (33). Rather than
causing demyelination, TNF-
and IFN-
seem to affect
remyelination by inhibition of growth and differentiation of oligodendrocytes (34).
With the generation of gene knockout mice, a new area
has been opened to study the involvement of distinct gene
products in experimental murine disease models. Studies
using mice carrying an inactivated IFN- (25, 26) or its receptor (24) gene have generated results contradicting the
current view on EAE. The same holds true for the TNF-
and LT-
knockout mice presented here. One explanation
for these contradicting results might be that the immune
system of knockout mice becomes biased in a way to favor
compensatory mechanisms leading to the observed outcome. It is therefore tempting to speculate that conditional
knockout mice, allowing for the temporal and spatial inactivation of a gene (35), might lead to more accurate results
in regard of cytokine-mediated pathogenesis, not only in
EAE, but many other pathologies.
EAE is used as an animal model to study the inflammatory process in multiple sclerosis (MS). TNF- and LT-
have been identified in acute and chronic active MS lesions, but were absent from chronic silent lesions (36). Furthermore, an increase in production of TNF by peripheral
blood mononuclear cells in vitro often precedes acute relapses in patients with MS (37). The data presented here
may question the immunopathogenic role attributed to
TNF- and LT-
in this human demyelinating disease.
Address correspondence to Dr. Karl Frei, Department of Neurosurgery, University Hospital Zürich, Rämistr. 100, CH-8091 Zürich, Switzerland, or to Dr. Adriano Fontana, Section of Clinical Immunology, University Hospital Zürich, Häldeliweg 4, CH-8044 Zürich, Switzerland.
Received for publication 12 February 1997 and in revised form 14 April 1997.
We thank Mrs. R. Muljana for performing the histology, Mrs. J. von Arx for expert breeding of the SJL/
mice and Dr. M. Hoechli (Laboratory for Electron Microscopy, University of Zürich, Zürich, Switzerland)
for his excellent assistance in digital image processing.
This work was supported by the Swiss National Science Foundation (grants 32-33966.92 to H.-P. Eugster and 31-42900.95 to A. Fontana). C.S. Constantinescu is supported by the National Institutes of Health (grant K11HD-01049).
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