Exacerbation of Autoantibody-Mediated Hemolytic Anemia by Viral Infection

doi:10.1128/JVI.74.13.6045-6049.2000

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Journal of Virology, July 2000, p. 6045-6049, Vol. 74, No. 13
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Exacerbation of Autoantibody-Mediated Hemolytic Anemia by Viral Infection

Mory Meite,¹^, Sabine Léonard,¹^, Mohammed El Azami El Idrissi,¹^,^§ Shozo Izui,² Pierre L. Masson,¹ and Jean-Paul Coutelier¹^,^*

Unit of Experimental Medicine, Christian de Duve Institute of Cellular Pathology, Université Catholique de Louvain, 1200 Brussels, Belgium,¹ and Department of Pathology, Centre Médical Universitaire, Université de Genève, Geneva, Switzerland²

Received 22 November 1999/Accepted 29 March 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Strong enhancement of the pathogenicity of an antierythrocyte monoclonal antibody was observed after infection of mice withlactate dehydrogenase-elevating virus. While injection of theantierythrocyte antibody alone induced only moderate anemia, concomitantinfection with this virus, which is harmless in most normal mice,led to a dramatic drop in the hematocrit and to death of infectedanimals. In vitro and in vivo analyses showed a dramatic increasein the ability of macrophages from infected mice to phagocytoseantibody-coated erythrocytes. These results indicate that virusescan trigger the onset of autoimmune disease by enhancing the pathogenicityof autoantibodies. They may explain how unrelated viruses couldbe implicated in the etiology of autoantibody-mediated autoimmunediseases.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

A causal connection between viral infection and the development of clinical pathology has long been suspected for a numberof autoimmune diseases mediated by autoantibodies (reviewed inreference 36). Interestingly, in most cases, several differentviruses have been proposed as etiologic agents of the same disease.Experimental data have suggested that viruses trigger an autoimmunehumoral response by distinct mechanisms, including polyclonalB-lymphocyte activation, antigenic mimicry, modification of self-antigen,production of anti-idiotypic antibodies, or enhancement of majorhistocompatibility complex molecule expression on potential antigen-presentingcells (4, 9, 11, 15, 20, 25, 31, 37). However,although it has been conclusively shown in several models thatautoantibody secretion was triggered by infection, the actualpathogenicity of these antibodies has not always been demonstrated.Similarly, other stimuli, like immunization of mice with rat redblood cells, may lead to autoantibody production without developmentof the corresponding disease, in this case, hemolytic anemia (8,24, 34). Therefore, it may be that mere autoantibody secretionis not sufficient to trigger an autoimmune disease and that theimmune environment of the host plays an important role in thepathogenicity of suchautoantibodies.

Viruses have also been shown to variably affect macrophage functions, including cytokine production and the ability to presentantigens (6, 16). Since it is known that some autoantibody-mediateddiseases involve phagocytosis by macrophages, we postulated thatmodulation of this cellular function may explain the inductionof such clinical diseases observed in the course of viral infections.To test this hypothesis, we used an experimental model of anemiainduced by administration of antierythrocyte monoclonal antibodies(29). Our results indicate that a viral infection with lactatedehydrogenase-elevating virus (LDV) may trigger a dramatic hemolyticdisease by enhancing the pathogenicity of autoantibodies. If confirmedwith other models, this observation may indicate how differentviruses can trigger similar clinical autoimmune diseases and openthe way to novel therapeuticapproaches.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Mice. Female BALB/c mice were bred at the Ludwig Institute for Cancer Research by G. Warnier and used when 6 to 8 weeksold.

Antibody. Immunoglobulin G1 (IgG1) 31-9D and IgG2a 34-3C anti-mouse erythrocyte monoclonal antibodies have been derived from NZB mice(29) and were purified from cell supernatants by two successiveprecipitations with ammoniumsulfate.

Viruses. The Riley strain of LDV, from the American Type Culture Collection, was grown in NMRI mice and titrated by injection of serialdilutions into groups of mice (7). Approximately 2 × 10⁷ 50% infective doses were injected intraperitoneally in 0.5 mlof saline into recipientanimals.

Hematocrit. Mice were bled by retro-orbital puncture after appropriate anesthesia. Hematocrit was measured after centrifugation of heparinizedblood in a Hettich-Haematokrit centrifuge (Hettich, Tuttlingen,Germany).

In vitro erythrophagocytosis. The ability of macrophages to phagocytose sensitized red cells was measured as described previously (28). Briefly, normalmouse red cells were sensitized by incubation of 500 µl of packederythrocytes with 50 µg of monoclonal antibody in 10 ml of phosphate-bufferedsaline with 2% bovine serum albumin for 2 h at room temperature.Macrophages were derived from total peritoneal cells by adhesionon a tissue culture petri dish for 3 h. They were then incubatedfor 3 h with 20 µl of washed sensitized red cells in 2 ml of supplementedDulbecco's medium containing 10% fetal calf serum, washed withphosphate-buffered saline, and stained with o-toluidine. Phagocytosiswas expressed as the percentage of cells having internalized atleast fiveerythrocytes.

Analysis of liver sections. Liver sections fixed in Bouin solution and embedded in paraffin were analyzed after staining withhematoxylin.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Effect of LDV infection on in vivo autoantibody-induced anemia. BALB/c mice were infected with LDV after inoculation of antierythrocyte monoclonal antibody. Two different antierythrocyteantibodies were used, both derived from NZB mice (29). Injectionof both antibodies leads to in vivo anemia in normal uninfectedmice, although by distinct pathways. Whereas IgG2a 34-3C triggerserythrophagocytosis (28, 29), erythrocyte destruction inducedby IgG1 31-9D is mediated by cell sequestration in the spleenand liver (29). As shown in Fig. 1 for a typical experimentof six performed, the 34-3C monoclonal autoantibody alone inducedonly moderate lethality (2 out of 10 mice in this experiment died,while in other experiments, all of the mice in this experimentalgroup survived). No further modifications of survival were observedat later times (not shown). In sharp contrast, all animals diedwhen they were infected with LDV after receiving the 34-3C antibody.This effect of LDV infection on autoantibody pathogenicity wasnot observed with the 31-9D antibody, since all mice, infectedor uninfected, survived the administration of this antierythrocytemonoclonal antibody. This indicated also that LDV by itself didnot induce the death of infected mice.

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FIG. 1. Effect of LDV infection on survival after antierythrocyte autoantibody inoculation. Survival was determined every day in groups of 10 BALB/c mice that received 4 mg of antierythrocyte autoantibody 34-3C or 31-9D, followed 1 day later by LDV infection. Control animals were untreated or received autoantibody 34-3C or 31-9D only.

To determine whether this increase of lethality in LDV-infected mice was related to an enhancement of antierythrocyte autoantibodypathogenicity, we measured hematocrit at different times after34-3C antibody administration (Fig. 2 shows typical results offive experiments performed). In uninfected mice, 34-3C triggereda moderate anemia that reached a maximum 4 days after autoantibodyadministration and resolved 2 days later. In contrast, infectedmice that received the 34-3C antibody developed a dramatic anemia4 days later, with hematocrits dropping to about 20 to 25% ofnormal values (Fig. 2). Although other causes may be consideredas well, this almost complete destruction of red blood cells islikely to have contributed to the death at day 6 after autoantibodyinjection of all of the animals that simultaneously received the34-3C antierythrocyte autoantibody and the virus. Whereas LDV-inducedlethality required the administration of at least 1 mg of antierythrocyteantibody, enhancement of autoantibody pathogenicity by viral infectionwas observed with as little as 100 µg of 34-3C. Indeed, whilein a typical experiment, the latter dose of antibody triggeredonly a minimal hematocrit drop, from 49.8 ± 0.4 to 43.1 ± 1.3,in uninfected animals in 4 days, it induced a much more importantdecrease in LDV-infected mice, from 49.9 ± 0.5 to 34.3 ± 2.3.

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FIG. 2. Enhancement of 34-3C antierythrocyte autoantibody-induced anemia by LDV infection. Hematocrit was measured at different times after injection of 2 mg of antierythrocyte autoantibody in groups of four or five uninfected BALB/c mice or in animals also infected with LDV. Controls were uninfected animals that received no antibody. Results are expressed as mean ± standard errors.

This effect of LDV infection on autoantibody pathogenicity was transient, as shown in Fig. 3. Five out of six animals thatreceived LDV 1 day before or 1 day after antierythrocyte autoantibodyadministration either had a hematocrit below 10.5 at day 4 afterthis antibody injection or were dead. In contrast, animals thathad been infected 4 days before 34-3C inoculation developed amoderate anemia, similar to that of uninfected mice.

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FIG. 3. Kinetics of LDV-induced enhancement of anemia. Hematocrit was determined 4 days after injection of 2 mg of the 34-3C antibody into BALB/c mice. LDV infection was performed at different times before or after 34-3C inoculation, as shown. Control mice were uninfected. Mice with a hematocrit of 0 were dead.

The pattern of anemia triggered by the administration of the 31-9D autoantibody in uninfected mice was not different fromthat following 34-3C inoculation, although variations were observedfrom one experiment to another. However, in contrast to what hadbeen observed with the 34-3C antibody, the 31-9D-mediated anemiawas only slightly modified by LDV infection (data notshown).

Enhancement of in vitro and in vivo erythrophagocytosis by macrophages after LDV infection. Because it has been previously demonstrated that 34-3C-mediated anemia, but not 31-9D-mediated anemia, involves phagocytosisof autoantibody-sensitized red cells by macrophages (29), itwas postulated that the effect of LDV on the disease triggeredby the 34-3C antibody could be related to an increase in the abilityof macrophages from infected animals to ingest autoantibody-coatedcells. To test this hypothesis, peritoneal macrophages were derivedfrom normal and infected BALB/c mice and their ability to ingestnormal red cells or erythrocytes sensitized with either the 34-3Cor the 31-9D autoantibody was measured in vitro. As shown in Fig.4 (results of a typical experiment of six performed), no significanterythrophagocytosis was observed with normal red cells, neitherwith macrophages from control mice nor with cells from LDV-infectedanimals. In contrast, LDV infection strongly increased the abilityof macrophages to ingest 34-3C-coated red cells, which were alreadysignificantly phagocytosed by macrophages from normal animals.Internalization of 31-9D-sensitized erythrocytes by macrophagesfrom uninfected mice was marginal and only moderately increasedafter LDV infection.

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FIG. 4. In vitro erythrophagocytosis by macrophages from LDV-infected mice. Macrophages from groups of four control BALB/c mice or from four animals infected for 4 days with LDV were pooled, and their ability to phagocytose either normal red cells or erythrocytes sensitized with the 34-3C or 31-9D monoclonal antibody was measured in vitro as described in Materials and Methods.

That LDV could enhance erythrophagocytosis was confirmed by ex vivo analysis of liver sections. As shown in Fig. 5 for typicalmice, 4 days after concomitant administration of 34-3C autoantibodyand infection with LDV, numerous macrophages that had ingestedlarge numbers of erythrocytes could be detected. In contrast,only a few phagocytosed red cells were observed in liver sectionsfrom mice that received the autoantibody alone and none were seenin control infected or uninfected animals.

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FIG. 5. In vivo erythrophagocytosis in LDV-infected mice. Liver sections were prepared from control mice (a) and from mice 4 days after administration of 2 mg of the 34-3C antibody alone (b), LDV alone (c), or the 34-3C antibody and LDV (d). Cells that have phagocytosed large numbers of erythrocytes are shown by white arrows. The experiment was performed twice with three mice per group. Original magnification, ×460.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Using an experimental model of autoimmune hemolytic anemia induced by the administration of monoclonal autoantibodies reactingwith erythrocyte antigens, we have shown in this work that a viruscould enhance the pathogenicity of these autoantibodies, leadingto the development of overt disease and even death of the infectedanimals. In contrast to most mechanisms that have been proposedso far to explain how a virus can trigger an autoimmune disease,in this case, the virus does not induce the autoimmune responseitself $---$ e.g., autoantibody production $---$ but modifies the immune environmentof the infected host, which results in increased pathogenicityof pre-existing autoantibodies. Therefore, disease developmentrequires at least two distinct steps: first, initiation of theanti-self reaction, mimicked here by passive autoantibody administration,and then enhancement of the pathogenicity of this autoimmune response.This could correspond to the actual progression of some humanautoimmune diseases which may often be enhanced by viral infections.Such a mechanism may also explain why different viruses can beinvolved in the development of a particular disease, since, contraryto the production of autoantibodies, the modulation of the hostenvironment is not antigen specific but can most probably be explainedby responses elicited similarly by different infectious agents,like cytokine secretion. Indeed, we observed a similar enhancementof antierythrocyte autoantibody pathogenicity after infectionwith mouse hepatitis virus (not shown), which supports thishypothesis.

The mechanism by which LDV increases antierythrocyte autoantibody pathogenicity appears to be, at least mainly, enhancementof macrophage phagocytic function. Indeed, LDV could increasethe anemia induced by the 34-3C antibody, which has been shownto trigger erythrophagocytosis (29), but only slightly modifiedthe disease initiated by the 31-9D antibody, which involves adifferent pathogenic pathway. In addition, in vitro analysis ofmacrophage phagocytic function indicated that the ability to ingest34-3C-coated, but not uncoated or 31-9D-coated, red cells wasstrongly enhanced in mice infected with the virus (Fig. 4). Finally,ex vivo analysis of liver sections showed the phagocytosis ofnumerous red cells in mice that had received both the 34-3C antibodyand the virus but not in control animals (Fig. 5). Although manyviral infections result in a decrease in macrophage functions,including phagocytosis, some viruses, such as herpes simplex virus(2), Coxsackie virus (22), or Newcastle disease virus (19),have been shown to enhance the ability of these cells to incorporatevarious targets. Whereas contradictory results have been reportedafter LDV infection (17, 18, 32), another nidovirus, mousehepatitis virus, can also increase macrophage-mediated phagocytosis(33).

Enhancement of the phagocytic activity of a particular macrophage most probably does not require infection of this cell, althoughthis remains to be demonstrated. Our results (Fig. 4) suggestthat after LDV infection, the frequency of macrophages with increasedphagocytic activity (more than 25%) is higher than the frequencyof macrophages from adult mice reported to be infected by thisvirus (5 to 15%; 26). In addition, whereas the phagocytic activityis fully increased 4 days after LDV inoculation (Fig. 4), it hasbeen previously shown that as soon as 3 days postinfection, mostinfected cells have been killed by the virus (1). Quite possibly,production of cytokines, such as gamma interferon or granulocyte-macrophagecolony-stimulating factor, in the course of infection can activatemacrophages enough to enhance their ability to ingest antibody-coatedtargets. Indeed, the latter cytokine has been reported to dramaticallyenhance in vivo 34-3C antierythrocyte pathogenicity (3). Onthe other hand, gamma interferon which is secreted after infectionwith many viruses, including both LDV and mouse hepatitis virus(27, 30, and unpublished results), has been shown to promotephagocytosis by macrophages (10). Interestingly, this effectof gamma interferon has been proposed to explain enhanced phagocyticactivity after Newcastle disease virus or vesicular stomatitisvirus infection (13, 14). The possibility that the virus-mediatedincrease in autoantibody pathogenicity reported here is linkedto an enhancement of macrophage expression of Fc $gamma$ receptors, moleculesthat are involved in 34-3C-induced anemia (5, 21) and areupregulated by interferons and granulocyte-macrophage colony-stimulatingfactor (12, 23, 35), is currently underinvestigation.

This observation that the pathogenicity of autoantibodies depends on their microenvironment, including the microbiologicalstatus of the host, may open the way to new therapeutic approachesto autoimmune diseases. For example, targeting of macrophage activationin addition to the autoimmune response itself may prove valuablefor patients with autoantibody-mediated diseases. A more completeelucidation of the mechanisms leading to macrophage activationmay therefore provide interesting information on the pathogenesisof autoimmune diseases and on possible alternative ways to treatthem.

	ACKNOWLEDGMENTS

We are indebted to J. Van Snick and P. Monteyne for critical reading of the manuscript and to T. Briet, M.-D. Gonzales, andJ. Van Broeck for expert technicalassistance.

This work was supported by the Fonds National de la Recherche Scientifique (FNRS); the Fonds de la Recherche ScientifiqueMédicale (FRSM); the Loterie Nationale; the Fonds de DéveloppementScientifique (UCL); the Opération Télévie; the State-PrimeMinister's Office-S.S.T.C. (interuniversity attraction poles,grant 44), the "Actions de recherche concertées" from the Communautéfrançaise de Belgique-Direction de la Recherche scientifique(concerted actions, grant 99/04-239), Belgium; and the Swiss NationalFoundation for Scientific Research. J.-P.C. is a research directorwith theFNRS.

	FOOTNOTES

^* Corresponding author. Mailing address: Unit of Experimental Medicine, UCL MEXP 7430, Av. Hippocrate 74, B-1200 Bruxelles,Belgium. Phone: 32 2 764 7437. Fax: 32 2 764 7430. E-mail: coutelier{at}mexp.ucl.ac.be.

Present address: Service d'hématologie et d'immunologie, CHU de Yopougon, Abidjan 21, Côte d'Ivoire.

Present address: 4845 Jalhay,Belgium.

^§ Present address: Department of Microbiology, University of Illinois, Chicago, IL60612.

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Top
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Results
Discussion
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	Articles by Coutelier, J.-P.

1.	Anderson, G. W., R. R. R. Rowland, G. A. Palmer, C. Even, and P. G. W. Plagemann. 1995. Lactate dehydrogenase-elevating virus replication persists in liver, spleen, lymph node, and testis tissues and results in accumulation of viral RNA in germinal centers, concomitant with polyclonal activation of B cells. J. Virol. 69:5177-5185[Abstract].
2.	Armerding, D., P. Mayer, M. Scriba, A. Hren, and H. Rossiter. 1981. In vivo modulation of macrophage functions by herpes simplex virus type 2 in resistant and sensitive inbred mouse strains. Immunobiology 160:217-227[Medline].
3.	Berney, T., T. Shibata, R. Merino, Y. Chicheportiche, V. Kindler, P. Vassalli, and S. Izui. 1992. Murine autoimmune hemolytic anemia resulting from Fc $gamma$ receptor-mediated erythrophagocytosis: protection by erythropoietin but not by interleukin-3, and aggravation by granulocyte-macrophage colony stimulating factor. Blood 79:2960-2964[Abstract/Free Full Text].
4.	Cafruny, W. A., and D. E. Hovinen. 1988. Infection of mice with lactate dehydrogenase-elevating virus leads to stimulation of autoantibodies. J. Gen. Virol. 69:723-729[Abstract/Free Full Text].
5.	Clynes, R., and J. V. Ravetch. 1995. Cytotoxic antibodies trigger inflammation through Fc receptors. Immunity 3:21-26[CrossRef][Medline].
6.	Coutelier, J.-P., J. Van Broeck, and S. F. Wolf. 1995. Interleukin-12 gene expression after viral infection in the mouse. J. Virol. 69:1955-1958[Abstract].
7.	Coutelier, J.-P., and J. Van Snick. 1985. Isotypically restricted activation of B lymphocytes by lactic dehydrogenase virus. Eur. J. Immunol. 15:250-255[Medline].
8.	Cox, K. O., and A. Howles. 1981. Induction and regulation of autoimmune hemolytic anemia in mice. Immunol. Rev. 55:31-53[CrossRef][Medline].
9.	Cunningham, M. W., S. M. Antone, J. M. Gulizia, B. M. McManus, V. A. Fischetti, and C. J. Gauntt. 1992. Cytotoxic and viral neutralizing antibodies crossreact with streptococcal M protein, enteroviruses, and human cardiac myosin. Proc. Natl. Acad. Sci. USA 89:1320-1324[Abstract/Free Full Text].
10.	Donahoe, R. M., and K. Y. Huang. 1976. Interferon preparations enhance phagocytosis in vivo. Infect. Immun. 13:1250-1257[Abstract/Free Full Text].
11.	Eaton, M. D. 1980. Autoimmunity induced by syngeneic splenocyte membranes carrying irreversibly adsorbed paramyxovirus. Infect. Immun. 27:855-861[Abstract/Free Full Text].
12.	Fertsch, D., and S. N. Vogel. 1984. Recombinant interferons increase macrophage Fc receptor capacity. J. Immunol. 132:2436-2439[Abstract].
13.	Hamburg, S. I., G. H. Cassell, and M. Rabinovitch. 1980. Relationship between enhanced macrophage phagocytic activity and the induction of interferon by Newcastle disease virus in mice. J. Immunol. 124:1360-1364[Abstract].
14.	Hamburg, S. I., R. E. Manejias, and M. Rabinovitch. 1978. Macrophage activation: increased ingestion of IgG-coated erythrocytes after administration of interferon inducers to mice. J. Exp. Med. 147:593-598[Abstract/Free Full Text].
15.	Haspel, M. V., T. Onodera, B. S. Prabhakar, M. Horita, H. Suzuki, and A. L. Notkins. 1983. Virus-induced autoimmunity: monoclonal antibodies that react with endocrine tissues. Science 220:304-306[Abstract/Free Full Text].
16.	Isakov, N., M. Feldman, and S. Segal. 1982. Acute infection of mice with lactic dehydrogenase virus (LDV) impairs the antigen-presenting capacity of their macrophages. Cell. Immunol. 66:317-322[CrossRef][Medline].
17.	Isakov, N., M. Feldman, and S. Segal. 1982. Lactic dehydrogenase virus (LDV) impairs the antigen-presenting capacity of macrophages yet fails to affect their phagocytic activity. Immunobiology 162:15-27[Medline].
18.	Lussenhop, N., B. Holmes, W. A. Cafruny, and P. G. W. Plagemann. 1982. Acute infection of mice with lactate dehydrogenase-elevating virus enhances Fc and complement receptor activity of peritoneal macrophages. J. Gen. Virol. 61:25-32[Abstract/Free Full Text].
19.	Manejias, R. E., S. I. Hamburg, and M. Rabinovitch. 1978. Serum interferon and phagocytic activity of macrophages in recombinant inbred mice inoculated with Newcastle disease virus. Cell. Immunol. 38:209-213[CrossRef][Medline].
20.	Massa, P. T., R. Dörries, and V. ter Meulen. 1986. Viral particles induce Ia antigen expression on astrocytes. Nature (London) 320:543-546[CrossRef][Medline].
21.	Meyer, D., C. Schiller, J. Westermann, S. Izui, W. L. W. Hazenbos, J. S. Verbeek, R. E. Schmidt, and J. E. Gessner. 1998. Fc $gamma$ RIII (CD16)-deficient mice show IgG isotype-dependent protection to experimental autoimmune hemolytic anemia. Blood 92:3997-4002[Abstract/Free Full Text].
22.	Modalsli, K., G. Bukholm, and M. Degre. 1990. Coxsackie B1 virus infection enhances the bacterial invasiveness, the phagocytosis and the membrane permeability in HEp-2 cells. APMIS 98:489-495[Medline].
23.	Morrissey, P. J., L. Bressler, K. Charrier, and A. Alpert. 1988. Response of resident murine peritoneal macrophages to in vivo administration of granulocyte-macrophage colony-stimulating factor. J. Immunol. 140:1910-1915[Abstract/Free Full Text].
24.	Naysmith, J. D., M. G. Ortega-Pierres, and C. J. Elson. 1981. Rat erythrocyte-induced anti-erythrocyte autoantibody production and control in normal mice. Immunol. Rev. 55:55-87[CrossRef][Medline].
25.	Nepom, J. T., H. L. Weiner, M. A. Dichter, M. Tardieu, D. R. Spriggs, C. F. Gramm, M. L. Powers, B. N. Fields, and M. I. Greene. 1982. Identification of a hemagglutinin-specific idiotype associated with reovirus recognition shared by lymphoid and neural cells. J. Exp. Med. 155:155-167[Abstract/Free Full Text].
26.	Onyekaba, C. O., J. T. Harty, and P. G. W. Plagemann. 1989. Extensive cytocidal replication of lactate dehydrogenase-elevating virus in cultured peritoneal macrophages from 1-2-week-old mice. Virus Res. 14:327-338[CrossRef][Medline].
27.	Plagemann, P. G. W., R. R. R. Rowland, C. Even, and K. S. Faaberg. 1995. Lactate dehydrogenase-elevating virus: an ideal persistent virus? Springer Semin. Immunopathol. 17:167-186[Medline].
28.	Pottier, Y., I. Pierard, A. Barclay, P. L. Masson, and J.-P. Coutelier. 1996. The mode of action of treatment by IgG of haemolytic anaemia induced by an anti-erythrocyte monoclonal antibody. Clin. Exp. Immunol. 106:103-107[CrossRef][Medline].
29.	Shibata, T., T. Berney, L. Reininger, Y. Chicheportiche, S. Ozaki, T. Shirai, and S. Izui. 1990. Monoclonal anti-erythrocyte autoantibodies derived from NZB mice cause autoimmune hemolytic anemia by two distinct pathogenic mechanisms. Int. Immunol. 2:1133-1141[Abstract/Free Full Text].
30.	Smith, A. L., S. W. Barthold, M. S. de Souza, and K. Bottomly. 1991. The role of gamma interferon in infection of susceptible mice with murine coronavirus, MHV-JHM. Arch. Virol. 121:89-100[CrossRef][Medline].
31.	Srinivasappa, J., J. Saegusa, B. S. Prabhakar, M. K. Gentry, M. J. Buchmeier, T. J. Wiktor, H. Koprowski, M. B. A. Oldstone, and A. L. Notkins. 1986. Molecular mimicry: frequency of reactivity of monoclonal antiviral antibodies with normal tissues. J. Virol. 57:397-401[Abstract/Free Full Text].
32.	Stevenson, M. M., J. C. Rees, and M. S. Meltzer. 1980. Macrophage function in tumor-bearing mice: evidence for lactic dehydrogenase-elevating virus-associated changes. J. Immunol. 124:2892-2899[Medline].
33.	Tamura, T., A. Sakaguchi, C. Kai, and K. Fujiwara. 1980. Enhanced phagocytic activity of macrophages in mouse hepatitis virus-infected nude mice. Microbiol. Immunol. 24:243-247[Medline].
34.	Verdonck, E., C. J. Pfau, M.-D. Gonzalez, P. L. Masson, and J.-P. Coutelier. 1994. Influence of viral infection on anti-erythrocyte autoantibody response after immunization of mice with rat red blood cells. Autoimmunity 17:73-81[Medline].
35.	Vogel, S. N., D. S. Finbloom, K. E. English, D. L. Rosenstreich, and S. G. Langreth. 1983. Interferon-induced enhancement of macrophage Fc receptor expression: $beta$ -interferon treatment of C3H/HeJ macrophages results in increased numbers and density of Fc receptors. J. Immunol. 130:1210-1214[Abstract].
36.	von Herrath, M., and M. B. A. Oldstone. 1996. Virus-induced autoimmune disease. Curr. Opin. Immunol. 8:878-885[CrossRef][Medline].
37.	Yamada, M., A. Zurbriggen, and R. Fujinami. 1990. Monoclonal antibody to Theiler's murine encephalomyelitis virus defines a determinant on myelin and oligodendrocytes, and augments demyelination in experimental allergic encephalomyelitis. J. Exp. Med. 171:1893-1907[Abstract/Free Full Text].