Genetic Vaccination against Murine Cysticercosis by Using a Plasmid Vector Carrying Taenia solium Paramyosin
http://www.100md.com
感染与免疫杂志 2005年第3期
Department of Immunology, Instituto de Investigaciones Biomedicas, Universidad Nacional Autonoma de Mexico, Mexico City, Mexico
Center for Biomedical Inventions, Department of Internal Medicine, University of Texas-Southwestern Medical Center, Dallas, Texas
ABSTRACT
A plasmid vector carrying the immunoprotective amino-terminal fragment of Taenia solium paramyosin (VW2-1) was designed for genetic vaccination studies. Mice that were genetically immunized with VW2-1 and challenged by intraperitoneal inoculation of Taenia crassiceps cysticerci showed 43 to 48% reductions in the parasite burden, values which were similar to values obtained previously when the recombinant protein was used.
TEXT
Human and porcine cysticercosis caused by Taenia solium is still prevalent in several countries of Latin America, Africa, and Asia (11). A strong effort is currently being directed toward the development of an effective vaccine against porcine cysticercosis. A number of strategies have been proposed, including the use of parasite crude extracts (9, 17), recombinant proteins (2, 3, 15), synthetic peptides (4), phage display (8), and genetic immunization (10, 18). Genetic vaccines are particularly appealing for applications in developing countries as they can be inexpensive to produce and store (5). In the present study, we evaluated the use of genetic immunization with the amino-terminal fragment of T. solium paramyosin (VW2-1), which was previously shown to be protective (15), as an alternative strategy for vaccination in the murine model of Taenia crassiceps cysticercosis.
A plasmid construct encoding a synthetic sequence for VW2-1 was designed for genetic immunization. The codon usage of the wild-type coding sequence for VW2-1 was adapted for mammalian cells (synVW2-1) by using procedures for gene synthesis (1). Briefly, a set of overlapping 60-mer oligonucleotides were assembled by PCR to construct synVW2-1, which was inserted into the pCMV plasmid vector (14). The construct was confirmed by DNA sequencing before large-scale purification with a QIAGEN Endofree Plasmid Giga kit (QIAGEN). A comparison of the wild-type and synthetic sequences of VW2-1 showed substantial changes in first (11.2%), second (4.85%), and third (52.6%) positions of codons. An extensive comparison of the outcomes of the immune responses elicited in mice genetically immunized with wild-type VW2-1 and with synVW2-1 consistently showed higher antibody and cellular immune responses with the synthetic gene (data not shown). The synthetic coding sequence is available from us upon request.
Vaccination assays were carried out by using 8- to 10-week-old female BALB/c mice that were bilaterally inoculated in the tibialis anterior muscle with pCMV-synVW2-1 or pCMV blank vector (100 μg of DNA per mouse in 100 μl of 0.9% saline). A third group contained nave mice. After 2 and 4 weeks, mice were boosted with identical doses of plasmid DNA.
In order to evaluate if the antibodies raised by genetic immunization were cross-reactive with paramyosins of T. solium and T. crassiceps, Western blot assays were carried out as described previously (16). Briefly, nitrocellulose membranes were blotted with recombinant full-length TPmy (recTPmy) and recombinant VW2-1 (recVW2-1) or with crude protein extracts from T. solium and T. crassiceps cysts (6). Membranes were reacted with pooled mouse sera that were collected 45 days after genetic immunization. Blots were developed by using a peroxidase-conjugated rabbit anti-mouse immunoglobulin G(H+L) (Zymed) secondary antibody, followed by diaminobenzidine (Sigma). A single 98-kDa protein, a size consistent with the expected size of paramyosins, was recognized in both crude extracts (Fig. 1). Moreover, recTPmy and recVW2-1 were also recognized by the sera from genetically immunized mice. These findings are consistent with the antigenic similarity between the two species of taeniids (12), as well as with the cross-reactivity of paramyosins from distant invertebrate sources (7).
The cellular immune response elicited in genetically immunized mice was characterized by proliferation assays and cytokine production by using spleen cells cultured in vitro as described previously (15). Briefly, a pool of spleen cells from each group, obtained 45 days after immunization, was cultured in the presence of 1 to 5 μg of recVW2-1 per ml for 72 h to a density of 5 x 105 cells per well. The responsiveness of spleen cells to concanavalin A was also checked by stimulation with 1 μg of concanavalin A per ml. Eighteen hours before harvesting, cells were pulsed with [methyl-3H]thymidine (1 μCi/well; NEN Life Science), and the amount of incorporated radioactive label was measured with a liquid scintillation counter (Betaplate, Turku, Finland). The results of proliferation studies showed that significant stimulation indices were obtained for spleen cells from mice that were immunized with pCMV-synVW2-1 (Table 1). Spleen cells from nave and immune animals showed similar responses to concanavalin A. The amounts of gamma interferon (IFN-) and interleukin-4 present in supernatants of spleen cells stimulated with recVW2-1 were determined by a sandwich enzyme-linked immunosorbent assay by using BD OptEIA cytokine kits (PharMingen). High levels of IFN- were detected in the supernatant of spleen cells from mice that were immunized with pCMV-synVW2-1 (Table 2). Assays with spleen cells from nave and pCMV-inoculated mice showed that there was almost no IFN- and interleukin-4 production. The cellular immune response elicited in genetically immunized mice is consistent with a Th1 profile that has previously been related to protection in the murine model of cysticercosis (13).
The effect of genetic immunization with plasmid pCMV-synVW2-1 on a challenge with T. crassiceps cysts was evaluated in the murine model of cysticercosis as described previously (15). Two weeks after the last boost, mice were intraperitoneally challenged with 10 T. crassiceps cysts in saline, and they were sacrificed 25 days later. The cysts from the peritoneal cavities were collected and counted by individual, ignoring the experimental design. Genetic immunization with synVW2-1 resulted in 43 to 48% reductions in the parasite load (Table 3); these values were close to the 52% obtained with the recombinant product (15). No statistically significant differences were observed between the pCMV blank vector and nave mouse groups.
Preliminary vaccination trials with pigs in which conventional or genetic immunization with recVW2-1 and synVW2-1 was used also produced about 50% reductions in the parasite load (data not shown). Recent vaccination trials with pigs in which the workers used a variety of strategies, including the use of oncosphere or metacestode crude antigens, synthetic peptides, recombinant proteins, phage display, and genetic immunization (2-4, 8-10, 17, 18), have resulted in claims of remarkably high levels of protection against T. solium cysticercosis. However, the intrinsic problems with carrying out experimental infection of pigs have meant that most groups have had to use small numbers of animals or low challenge doses in experiments. In the case of field trials under uncontrolled conditions, vaccines are required to show prophylactic as well as therapeutic properties. It appears that a multifunctional vaccine formulation that includes several protective antigens (oncosphere and metacestode) might be the way to produce a broad-spectrum vaccine to aid in the control of taeniosis/cysticercosis.
ACKNOWLEDGMENTS
This work was supported in part by grants from CONACYT (grant 41693-M to J.P.L. and P.O.-S) and DGAPA-UNAM (grant IN215702-3 to P.O.-S). C.F.S. was supported by scholarships from DGAPA-UNAM and SNI-CONACYT.
REFERENCES
1. Chambers, R. S., and S. A. Johnston. 2003. High-level generation of polyclonal antibodies by genetic immunization. Nat. Biotechnol. 21:1088-1092.
2. Flisser, A., C. G. Gauci, A. Zoli, J. Martinez-Ocana, A. Garza-Rodriguez, J. L. Dominguez-Alpizar, P. Maravilla, R. Rodriguez-Canul, G. Avila, L. Aguilar-Vega, C. Kyngdon, S. Geerts, and M. W. Lightowlers. 2004. Induction of protection against porcine cysticercosis by vaccination with recombinant oncosphere antigens. Infect. Immun. 72:5292-5297.
3. Guo, Y. J., S. H. Sun, Y. Zhang, Z. H. Chen, K. Y. Wang, L. Huang, S. Zhang, H. Y. Zhang, Q. M. Wang, D. Wu, and W. J. Zhu. 2004. Protection of pigs against Taenia solium cysticercosis using recombinant antigen or in combination with DNA vaccine. Vaccine 22:3841-3847.
4. Huerta, M., A. S. de Aluja, G. Fragoso, A. Toledo, N. Villalobos, M. Hernandez, G. Gevorkian, G. Acero, A. Diaz, I. Alvarez, R. Avila, C. Beltran, G. Garcia, J. J. Martinez, C. Larralde, and E. Sciutto. 2001. Synthetic peptide vaccine against Taenia solium pig cysticercosis: successful vaccination in a controlled field trial in rural Mexico. Vaccine 20:262-266.
5. Johnston, S. A., A. M. Talaat, and M. J. McGuire. 2002. Genetic immunization: what's in a name Arch. Med. Res. 33:325-329.
6. Laclette, J. P., A. Alagon, K. Willms, and A. Torre-Blanco. 1990. Purification of antigen B from Taenia solium cysticerci by affinity to mammalian collagen. J. Parasitol. 76:273-275.
7. Laclette, J. P., C. B. Shoemaker, D. Richter, L. Arcos, N. Pante, C. Cohen, D. Bing, and A. Nicholson-Weller. 1992. Paramyosin inhibits complement C1. J. Immunol. 148:124-128.
8. Manoutcharian, K., A. Diaz-Orea, G. Gevorkian, G. Fragoso, G. Acero, E. Gonzalez, A. De Aluja, N. Villalobos, E. Gomez-Conde, and E. Sciutto. 2004. Recombinant bacteriophage-based multiepitope vaccine against Taenia solium pig cysticercosis. Vet. Immunol. Immunopathol. 99:11-24.
9. Molinari, J. L., D. Rodriguez, P. Tato, R. Soto, F. Arechavaleta, and S. Solano. 1997. Field trial for reducing porcine Taenia solium cysticercosis in Mexico by systematic vaccination of pigs. Vet. Parasitol. 69:55-63.
10. Rosas, G., G. Fragoso, T. Garate, B. Hernández, P. Ferrero, M. Foster-Cuevas, R. M. Parkhouse, L. J. Harrison, S. L. Briones, L. M. González, and E. Sciutto. 2002. Protective immunity against Taenia crassiceps murine cysticercosis induced by DNA vaccination with a Taenia saginata tegument antigen. Microbes Infect. 4:1417-1426.
11. Sciutto, E., G. Fragoso, A. Fleury, J. P. Laclette, J. Sotelo, A. Aluja, L. Vargas, and C. Larralde. 2000. Taenia solium disease in humans and pigs: an ancient parasitosis disease rooted in developing countries and emerging as a major health problem of global dimensions. Microbes Infect. 2:1875-1890.
12. Sciutto, E., G. Fragoso, L. Trueba, D. Lemus, R. M. Montoya, M. L. Diaz, T. Govezensky, C. Lomeli, G. Tapia, and C. Larralde. 1990. Cysticercosis vaccine: cross protecting immunity with T. solium antigens against experimental murine T. crassiceps cysticercosis. Parasite Immunol. 6:687-696.
13. Terrazas, L. I., M. Cruz, M. Rodriguez-Sosa, R. Bojalil, F. Garcia-Tamayo, and C. Larralde. 1999. Th1-type cytokines improve resistance to murine cysticercosis caused by Taenia crassiceps. Parasitol. Res. 85:135-141.
14. Timares, L., A. Takashima, and S. A. Johnston. 1998. Quantitative analysis of the immunopotency of genetically transfected dendritic cells. Proc. Natl. Acad. Sci. USA 95:13147-13152.
15. Vázquez-Talavera, J., C. F. Solís, L. I. Terrazas, and J. P. Laclette. 2001. Characterization and protective potential of the immune response to Taenia solium paramyosin in a murine model of Cysticercosis. Infect. Immun. 69:5412-5416.
16. Vázquez-Talavera, J., C. F. Solís, E. Medina-Escutia, Z. Morales-Lopez, J. Proao, D. Correa, and J. P. Laclette. 2001. Human T and B cell epitope mapping of Taenia solium paramyosin. Parasite Immunol. 23:575-579.
17. Verastegui, M., R. H. Gilman, A. Gonzales, H. H. Garcia, C. Gavidia, N. Falcon, T. Bernal, Y. Arana, V. C. Tsang, and the Cysticercosis Working Group In Peru. 2002. Taenia solium oncosphere antigens induce immunity in pigs against experimental cysticercosis. Vet. Parasitol. 108:49-62.
18. Wang, Q. M., S. H. Sun, Z. L. Hu, D. Wu, and Z. C. Wang. 2003. Immune response and protection elicited by DNA immunisation against Taenia cysticercosis. Vaccine 21:1672-1680.(Carlos F. Solís, Pedro Os)
Center for Biomedical Inventions, Department of Internal Medicine, University of Texas-Southwestern Medical Center, Dallas, Texas
ABSTRACT
A plasmid vector carrying the immunoprotective amino-terminal fragment of Taenia solium paramyosin (VW2-1) was designed for genetic vaccination studies. Mice that were genetically immunized with VW2-1 and challenged by intraperitoneal inoculation of Taenia crassiceps cysticerci showed 43 to 48% reductions in the parasite burden, values which were similar to values obtained previously when the recombinant protein was used.
TEXT
Human and porcine cysticercosis caused by Taenia solium is still prevalent in several countries of Latin America, Africa, and Asia (11). A strong effort is currently being directed toward the development of an effective vaccine against porcine cysticercosis. A number of strategies have been proposed, including the use of parasite crude extracts (9, 17), recombinant proteins (2, 3, 15), synthetic peptides (4), phage display (8), and genetic immunization (10, 18). Genetic vaccines are particularly appealing for applications in developing countries as they can be inexpensive to produce and store (5). In the present study, we evaluated the use of genetic immunization with the amino-terminal fragment of T. solium paramyosin (VW2-1), which was previously shown to be protective (15), as an alternative strategy for vaccination in the murine model of Taenia crassiceps cysticercosis.
A plasmid construct encoding a synthetic sequence for VW2-1 was designed for genetic immunization. The codon usage of the wild-type coding sequence for VW2-1 was adapted for mammalian cells (synVW2-1) by using procedures for gene synthesis (1). Briefly, a set of overlapping 60-mer oligonucleotides were assembled by PCR to construct synVW2-1, which was inserted into the pCMV plasmid vector (14). The construct was confirmed by DNA sequencing before large-scale purification with a QIAGEN Endofree Plasmid Giga kit (QIAGEN). A comparison of the wild-type and synthetic sequences of VW2-1 showed substantial changes in first (11.2%), second (4.85%), and third (52.6%) positions of codons. An extensive comparison of the outcomes of the immune responses elicited in mice genetically immunized with wild-type VW2-1 and with synVW2-1 consistently showed higher antibody and cellular immune responses with the synthetic gene (data not shown). The synthetic coding sequence is available from us upon request.
Vaccination assays were carried out by using 8- to 10-week-old female BALB/c mice that were bilaterally inoculated in the tibialis anterior muscle with pCMV-synVW2-1 or pCMV blank vector (100 μg of DNA per mouse in 100 μl of 0.9% saline). A third group contained nave mice. After 2 and 4 weeks, mice were boosted with identical doses of plasmid DNA.
In order to evaluate if the antibodies raised by genetic immunization were cross-reactive with paramyosins of T. solium and T. crassiceps, Western blot assays were carried out as described previously (16). Briefly, nitrocellulose membranes were blotted with recombinant full-length TPmy (recTPmy) and recombinant VW2-1 (recVW2-1) or with crude protein extracts from T. solium and T. crassiceps cysts (6). Membranes were reacted with pooled mouse sera that were collected 45 days after genetic immunization. Blots were developed by using a peroxidase-conjugated rabbit anti-mouse immunoglobulin G(H+L) (Zymed) secondary antibody, followed by diaminobenzidine (Sigma). A single 98-kDa protein, a size consistent with the expected size of paramyosins, was recognized in both crude extracts (Fig. 1). Moreover, recTPmy and recVW2-1 were also recognized by the sera from genetically immunized mice. These findings are consistent with the antigenic similarity between the two species of taeniids (12), as well as with the cross-reactivity of paramyosins from distant invertebrate sources (7).
The cellular immune response elicited in genetically immunized mice was characterized by proliferation assays and cytokine production by using spleen cells cultured in vitro as described previously (15). Briefly, a pool of spleen cells from each group, obtained 45 days after immunization, was cultured in the presence of 1 to 5 μg of recVW2-1 per ml for 72 h to a density of 5 x 105 cells per well. The responsiveness of spleen cells to concanavalin A was also checked by stimulation with 1 μg of concanavalin A per ml. Eighteen hours before harvesting, cells were pulsed with [methyl-3H]thymidine (1 μCi/well; NEN Life Science), and the amount of incorporated radioactive label was measured with a liquid scintillation counter (Betaplate, Turku, Finland). The results of proliferation studies showed that significant stimulation indices were obtained for spleen cells from mice that were immunized with pCMV-synVW2-1 (Table 1). Spleen cells from nave and immune animals showed similar responses to concanavalin A. The amounts of gamma interferon (IFN-) and interleukin-4 present in supernatants of spleen cells stimulated with recVW2-1 were determined by a sandwich enzyme-linked immunosorbent assay by using BD OptEIA cytokine kits (PharMingen). High levels of IFN- were detected in the supernatant of spleen cells from mice that were immunized with pCMV-synVW2-1 (Table 2). Assays with spleen cells from nave and pCMV-inoculated mice showed that there was almost no IFN- and interleukin-4 production. The cellular immune response elicited in genetically immunized mice is consistent with a Th1 profile that has previously been related to protection in the murine model of cysticercosis (13).
The effect of genetic immunization with plasmid pCMV-synVW2-1 on a challenge with T. crassiceps cysts was evaluated in the murine model of cysticercosis as described previously (15). Two weeks after the last boost, mice were intraperitoneally challenged with 10 T. crassiceps cysts in saline, and they were sacrificed 25 days later. The cysts from the peritoneal cavities were collected and counted by individual, ignoring the experimental design. Genetic immunization with synVW2-1 resulted in 43 to 48% reductions in the parasite load (Table 3); these values were close to the 52% obtained with the recombinant product (15). No statistically significant differences were observed between the pCMV blank vector and nave mouse groups.
Preliminary vaccination trials with pigs in which conventional or genetic immunization with recVW2-1 and synVW2-1 was used also produced about 50% reductions in the parasite load (data not shown). Recent vaccination trials with pigs in which the workers used a variety of strategies, including the use of oncosphere or metacestode crude antigens, synthetic peptides, recombinant proteins, phage display, and genetic immunization (2-4, 8-10, 17, 18), have resulted in claims of remarkably high levels of protection against T. solium cysticercosis. However, the intrinsic problems with carrying out experimental infection of pigs have meant that most groups have had to use small numbers of animals or low challenge doses in experiments. In the case of field trials under uncontrolled conditions, vaccines are required to show prophylactic as well as therapeutic properties. It appears that a multifunctional vaccine formulation that includes several protective antigens (oncosphere and metacestode) might be the way to produce a broad-spectrum vaccine to aid in the control of taeniosis/cysticercosis.
ACKNOWLEDGMENTS
This work was supported in part by grants from CONACYT (grant 41693-M to J.P.L. and P.O.-S) and DGAPA-UNAM (grant IN215702-3 to P.O.-S). C.F.S. was supported by scholarships from DGAPA-UNAM and SNI-CONACYT.
REFERENCES
1. Chambers, R. S., and S. A. Johnston. 2003. High-level generation of polyclonal antibodies by genetic immunization. Nat. Biotechnol. 21:1088-1092.
2. Flisser, A., C. G. Gauci, A. Zoli, J. Martinez-Ocana, A. Garza-Rodriguez, J. L. Dominguez-Alpizar, P. Maravilla, R. Rodriguez-Canul, G. Avila, L. Aguilar-Vega, C. Kyngdon, S. Geerts, and M. W. Lightowlers. 2004. Induction of protection against porcine cysticercosis by vaccination with recombinant oncosphere antigens. Infect. Immun. 72:5292-5297.
3. Guo, Y. J., S. H. Sun, Y. Zhang, Z. H. Chen, K. Y. Wang, L. Huang, S. Zhang, H. Y. Zhang, Q. M. Wang, D. Wu, and W. J. Zhu. 2004. Protection of pigs against Taenia solium cysticercosis using recombinant antigen or in combination with DNA vaccine. Vaccine 22:3841-3847.
4. Huerta, M., A. S. de Aluja, G. Fragoso, A. Toledo, N. Villalobos, M. Hernandez, G. Gevorkian, G. Acero, A. Diaz, I. Alvarez, R. Avila, C. Beltran, G. Garcia, J. J. Martinez, C. Larralde, and E. Sciutto. 2001. Synthetic peptide vaccine against Taenia solium pig cysticercosis: successful vaccination in a controlled field trial in rural Mexico. Vaccine 20:262-266.
5. Johnston, S. A., A. M. Talaat, and M. J. McGuire. 2002. Genetic immunization: what's in a name Arch. Med. Res. 33:325-329.
6. Laclette, J. P., A. Alagon, K. Willms, and A. Torre-Blanco. 1990. Purification of antigen B from Taenia solium cysticerci by affinity to mammalian collagen. J. Parasitol. 76:273-275.
7. Laclette, J. P., C. B. Shoemaker, D. Richter, L. Arcos, N. Pante, C. Cohen, D. Bing, and A. Nicholson-Weller. 1992. Paramyosin inhibits complement C1. J. Immunol. 148:124-128.
8. Manoutcharian, K., A. Diaz-Orea, G. Gevorkian, G. Fragoso, G. Acero, E. Gonzalez, A. De Aluja, N. Villalobos, E. Gomez-Conde, and E. Sciutto. 2004. Recombinant bacteriophage-based multiepitope vaccine against Taenia solium pig cysticercosis. Vet. Immunol. Immunopathol. 99:11-24.
9. Molinari, J. L., D. Rodriguez, P. Tato, R. Soto, F. Arechavaleta, and S. Solano. 1997. Field trial for reducing porcine Taenia solium cysticercosis in Mexico by systematic vaccination of pigs. Vet. Parasitol. 69:55-63.
10. Rosas, G., G. Fragoso, T. Garate, B. Hernández, P. Ferrero, M. Foster-Cuevas, R. M. Parkhouse, L. J. Harrison, S. L. Briones, L. M. González, and E. Sciutto. 2002. Protective immunity against Taenia crassiceps murine cysticercosis induced by DNA vaccination with a Taenia saginata tegument antigen. Microbes Infect. 4:1417-1426.
11. Sciutto, E., G. Fragoso, A. Fleury, J. P. Laclette, J. Sotelo, A. Aluja, L. Vargas, and C. Larralde. 2000. Taenia solium disease in humans and pigs: an ancient parasitosis disease rooted in developing countries and emerging as a major health problem of global dimensions. Microbes Infect. 2:1875-1890.
12. Sciutto, E., G. Fragoso, L. Trueba, D. Lemus, R. M. Montoya, M. L. Diaz, T. Govezensky, C. Lomeli, G. Tapia, and C. Larralde. 1990. Cysticercosis vaccine: cross protecting immunity with T. solium antigens against experimental murine T. crassiceps cysticercosis. Parasite Immunol. 6:687-696.
13. Terrazas, L. I., M. Cruz, M. Rodriguez-Sosa, R. Bojalil, F. Garcia-Tamayo, and C. Larralde. 1999. Th1-type cytokines improve resistance to murine cysticercosis caused by Taenia crassiceps. Parasitol. Res. 85:135-141.
14. Timares, L., A. Takashima, and S. A. Johnston. 1998. Quantitative analysis of the immunopotency of genetically transfected dendritic cells. Proc. Natl. Acad. Sci. USA 95:13147-13152.
15. Vázquez-Talavera, J., C. F. Solís, L. I. Terrazas, and J. P. Laclette. 2001. Characterization and protective potential of the immune response to Taenia solium paramyosin in a murine model of Cysticercosis. Infect. Immun. 69:5412-5416.
16. Vázquez-Talavera, J., C. F. Solís, E. Medina-Escutia, Z. Morales-Lopez, J. Proao, D. Correa, and J. P. Laclette. 2001. Human T and B cell epitope mapping of Taenia solium paramyosin. Parasite Immunol. 23:575-579.
17. Verastegui, M., R. H. Gilman, A. Gonzales, H. H. Garcia, C. Gavidia, N. Falcon, T. Bernal, Y. Arana, V. C. Tsang, and the Cysticercosis Working Group In Peru. 2002. Taenia solium oncosphere antigens induce immunity in pigs against experimental cysticercosis. Vet. Parasitol. 108:49-62.
18. Wang, Q. M., S. H. Sun, Z. L. Hu, D. Wu, and Z. C. Wang. 2003. Immune response and protection elicited by DNA immunisation against Taenia cysticercosis. Vaccine 21:1672-1680.(Carlos F. Solís, Pedro Os)