Plasmid DNA and protein vaccination of mice to the outer surface protein A of <i>Borrelia burgdorferi</i> leads to induction of T helper cells with specificity for a major epitope and augmentation of protective IgG antibodies <i>in vivo</i>

Zhong, Weimin; Wiesmüller, Karl‐Heinz; Kramer, Michael D.; Wallich, Reinhard; Simon, Markus M.

doi:10.1002/eji.1830261130

Cited by 24 publications

(7 citation statements)

References 58 publications

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“…Direct gene transfer into mouse muscle or skin leads to expression of an immunogenic protein encoded by the injected plasmid and has created a novel technology of immunization designated as nucleic acid or DNA vaccination [1,2]. In experimental animal models injection of a plasmid coding for a single antigenic protein confers protection against viral, protozoal, and more recently, intracellular bacterial infections including influenza virus [3], Plasmodium yoelii [4], Mycobacterium tuberculosis [5,6] and Borrelia burgdorferi [7,8]. Whether DNA vaccination protects against enteropathogenic extracellular bacteria, however, has not yet been investigated.…”

Section: Introductionmentioning

confidence: 99%

DNA immunization confers systemic, but not mucosal, protection against enteroinvasive bacteria

et al. 1999

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Naked plasmid DNA (pRc/Y-hsp60) with a cytomegalovirus promoter and a sequence encoding Yersinia enterocolitica 60-kDa heat shock protein (Y-HSP60) was used for vaccination. After intramuscular injection of pRc/Y-hsp60, Y-hsp60 mRNA could be detected by reverse transcription-PCR in muscle, liver and spleen. A single immunization with pRc/Y-hsp60 induced significant Y-HSP60-specific T cell responses after 1 week. IFN-gamma production by spleen cells upon stimulation with Y-HSP60 was strictly dependent on the presence of CD4+ T cells, indicating the generation of a Th1 response upon DNA immunization. DNA immunization in addition induced strong Y-HSP60-specific IgG2a, weak IgG1, but not IgA antibodies. Immunization of BALB/c and C57BL/6 mice with pRc/Y-hsp60 conferred protection against disseminated Y. enterocolitica infection in spleen, but not at the site of mucosal entry, the Peyer's patches. Furthermore, pRc/Y-hsp60 vaccination did not induce cross-protection against related pathogens. Vaccination of beta2-microglobulin- and H2-I-Abeta-deficient mice was not protective, suggesting that both CD4+ and CD8+ T cells are required for protective immunity induced by DNA vaccination.

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Section: Introductionmentioning

confidence: 99%

DNA immunization confers systemic, but not mucosal, protection against enteroinvasive bacteria

et al. 1999

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“…In this line, we and others have shown that vaccination with ospA-containing plasmids elicited Ab responses able to prevent subsequent infection (12,20,35). Similarly, immunization of mice with OspC-encoding DNA vaccines resulted in the production of specific Ab in mice, however, with unknown protective potential (28).…”

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confidence: 73%

DNA Vaccines Expressing a Fusion Product of Outer Surface Proteins A and C fromBorrelia burgdorferiInduce Protective Antibodies Suitable for Prophylaxis but Not for Resolution of Lyme Disease

et al. 2001

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DNA vaccines encoding the outer surface protein A (OspA) ofBorrelia burgdorferi have been shown to induce protective humoral responses capable of preventing but not curing infection in mice. Subsequent studies showed that an established infection or disease could be resolved by passive transfer of antibodies to OspC. In the present study, DNA vaccines encoding either the OspC antigen alone or fused to OspA and under the transcriptional control of the human elongation factor 1α promoter were evaluated for their protective and/or curative potential. In contrast to ospA-containing plasmids, none of the six constructs with ospC alone were immunogenic in vivo, independent of whether they contained promoter or leader sequences from ospA and/or ospC, or alternatively, the signal sequence of the human tissue plasminogen activator. Solely, a DNA vaccine encoding an OspA-OspC fusion product led to expression of the respective polypeptide chain in transfected cells in vitro and to the induction of OspA- and OspC-specific antibodies in vivo. Immune sera raised against the OspA-OspC fusion product conveyed full protection against subsequent infection, most probably via OspA-specific antibodies, but were unable to resolve infection.

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“…Hence, T cells seem to be responsible for development of destructive arthritis as opposed to conferring protection from disease [31]. Attempts to map dominant T-helper-cell epitopes of OspA in humans with a variety of HLA.DR alleles [28], as well as in H-2 k mice [32,33], have been reported. Although several T cell epitopes of OspA have been identified [28], the number of patients tested to date is too small to draw conclusions regarding dominant epitopes for particular class II MHC alleles.…”

Section: Review Articlementioning

confidence: 99%

“…Although several T cell epitopes of OspA have been identified [28], the number of patients tested to date is too small to draw conclusions regarding dominant epitopes for particular class II MHC alleles. In the H-2 k mouse, a single, C-terminal peptide is able to prime the animal for a protective anti-OspA antibody response [32,33]. Despite intensive investigations by many research groups, we still do not understand the cellular and molecular mechanisms which lead to antibiotic treatment-resistant Lyme arthritis in certain individuals.…”

Section: Review Articlementioning

confidence: 99%

Cellular and molecular aspects of Lyme arthritis

Gross¹,

Huber²

2000

CMLS, Cell. Mol. Life Sci.

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Lyme disease is a multisystem illness initiated upon infection with the spirochete Borrelia burgdorferi. Whereas the majority of patients who develop Lyme arthritis may be successfully treated with antibiotic therapy, about 10% go on to develop arthritis which persists for months to years, despite antibiotic therapy. Development of what we have termed treatment-resistant Lyme arthritis has previously been associated with both the presence of particular major histocompatibility complex class II alleles and immunoreactivity to the spriochetal outer surface protein A (OspA). Recently, we showed that patients with treatment-resistant Lyme arthritis, but not patients with other forms of arthritis, generate synovial fluid T cell responses to an immunodominant epitope of OspA and a highly homologous region of the human-lymphocyte-function-associated antigen-1alphaL chain. Identification of a bacterial antigen capable of propagating an autoimmune response against a self-antigen provides a model of molecular mimicry in the pathogenesis of treatment-resistant Lyme arthritis.

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Plasmid DNA and protein vaccination of mice to the outer surface protein A of Borrelia burgdorferi leads to induction of T helper cells with specificity for a major epitope and augmentation of protective IgG antibodies in vivo

Cited by 24 publications

References 58 publications

DNA immunization confers systemic, but not mucosal, protection against enteroinvasive bacteria

DNA immunization confers systemic, but not mucosal, protection against enteroinvasive bacteria

DNA Vaccines Expressing a Fusion Product of Outer Surface Proteins A and C fromBorrelia burgdorferiInduce Protective Antibodies Suitable for Prophylaxis but Not for Resolution of Lyme Disease

Cellular and molecular aspects of Lyme arthritis

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