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1. Plasmodium falciparum liver stage antigen-1 is cross-linked by tissue transglutaminase

Author

Doerig Christian, Holland Zoe JM, Piacentini Mauro, Di Giacomo Giuseppina, Rodolfo Carlo, Sacci John B, Nicoll William S, Hollingdale Michael R, and Lanar David E

Subjects
Arctic medicine. Tropical medicine, RC955-962, Infectious and parasitic diseases, RC109-216
Abstract

Abstract Background Plasmodium falciparum sporozoites injected by mosquitoes into the blood rapidly enter liver hepatocytes and undergo pre-erythrocytic developmental schizogony forming tens of thousands of merozoites per hepatocyte. Shortly after hepatocyte invasion, the parasite starts to produce Liver Stage Antigen-1 (LSA-1), which accumulates within the parasitophorous vacuole surrounding the mass of developing merozoites. The LSA-1 protein has been described as a flocculent mass, but its role in parasite development has not been determined. Methods Recombinant N-terminal, C-terminal or a construct containing both the N- and C- terminal regions flanking two 17 amino acid residue central repeat sequences (LSA-NRC) were subjected to in vitro modification by tissue transglutaminase-2 (TG2) to determine if cross-linking occurred. In addition, tissue sections of P. falciparum-infected human hepatocytes were probed with monoclonal antibodies to the isopeptide ε-(γ-glutamyl)lysine cross-bridge formed by TG2 enzymatic activity to determine if these antibodies co-localized with antibodies to LSA-1 in the growing liver schizonts. Results This study identified a substrate motif for (TG2) and a putative casein kinase 2 phosphorylation site within the central repeat region of LSA-1. The function of TG2 is the post-translational modification of proteins by the formation of a unique isopeptide ε-(γ-glutamyl)lysine cross-bridge between glutamine and lysine residues. When recombinant LSA-1 protein was crosslinked in vitro by purified TG2 in a calcium dependent reaction, a flocculent mass of protein was formed that was highly resistant to degradation. The cross-linking was not detectably affected by phosphorylation with plasmodial CK2 in vitro. Monoclonal antibodies specific to the very unique TG2 catalyzed ε- lysine cross-bridge co-localized with antibodies to LSA-1 in infected human hepatocytes providing visual evidence that LSA-1 was cross-linked in vivo. Conclusions While the role of LSA-1 is still unknown these results suggest that it becomes highly cross-linked which may aid in the protection of the parasite as it develops.

Published
2011
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2. Characterization of immunoglobulin G antibodies to Plasmodium falciparum sporozoite surface antigen MB2 in malaria exposed individuals

Author

John Chandy C, de la Vega Patricia, Sacci John B, Nguyen Thanh V, James Anthony A, and Kang Angray S

Subjects
Arctic medicine. Tropical medicine, RC955-962, Infectious and parasitic diseases, RC109-216
Abstract

Abstract Background MB2 protein is a sporozoite surface antigen on the human malaria parasite Plasmodium falciparum. MB2 was identified by screening a P. falciparum sporozoite cDNA expression library using immune sera from a protected donor immunized via the bites of P. falciparum-infected irradiated mosquitoes. It is not known whether natural exposure to P. falciparum also induces the anti-MB2 response and if this response differs from that in protected individuals immunized via the bites of P. falciparum infected irradiated mosquitoes. The anti-MB2 antibody response may be part of a robust protective response against the sporozoite. Methods Fragments of polypeptide regions of MB2 were constructed as recombinant fusions sandwiched between glutathione S-transferase and a hexa histidine tag for bacterial expression. The hexa histidine tag affinity purified proteins were used to immunize rabbits and the polyclonal sera evaluated in an in vitro inhibition of sporozoite invasion assay. The proteins were also used in immunoblots with sera from a limited number of donors immunized via the bites of P. falciparum infected irradiated mosquitoes and plasma and serum obtained from naturally exposed individuals in Kenya. Results Rabbit polyclonal antibodies targeting the non-repeat region of the basic domain of MB2 inhibited sporozoites entry into HepG2-A16 cells in vitro. Analysis of serum from five human volunteers that were immunized via the bites of P. falciparum infected irradiated mosquitoes that developed immunity and were completely protected against subsequent challenge with non-irradiated parasite also had detectable levels of antibody against MB2 basic domain. In contrast, in three volunteers not protected, anti-MB2 antibodies were below the level of detection. Sera from protected volunteers preferentially recognized a non-repeat region of the basic domain of MB2, whereas plasma from naturally-infected individuals also had antibodies that recognize regions of MB2 that contain a repeat motif in immunoblots. Sequence analysis of eleven field isolates and four laboratory strains showed that these antigenic regions of the basic domain of the MB2 gene are highly conserved in parasites obtained from different parts of the world. Moreover, anti-MB2 antibodies also were detected in the plasma of 83% of the individuals living in a malaria endemic area of Kenya (n = 41). Conclusion A preliminary analysis of the human humoral response against MB2 indicates that it may be an additional highly conserved target for immune intervention at the pre-erythrocytic stage of P. falciparum life cycle.

Published
2009
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3. Characterization of immunoglobulin G antibodies to Plasmodium falciparum sporozoite surface antigen MB2 in malaria exposed individuals

Author

Nguyen, Thanh V, Sacci, John B, de la Vega, Patricia, John, Chandy C, James, Anthony A, and Kang, Angray S

Abstract

Abstract Background MB2 protein is a sporozoite surface antigen on the human malaria parasite Plasmodium falciparum. MB2 was identified by screening a P. falciparum sporozoite cDNA expression library using immune sera from a protected donor immunized via the bites of P. falciparum-infected irradiated mosquitoes. It is not known whether natural exposure to P. falciparum also induces the anti-MB2 response and if this response differs from that in protected individuals immunized via the bites of P. falciparum infected irradiated mosquitoes. The anti-MB2 antibody response may be part of a robust protective response against the sporozoite. Methods Fragments of polypeptide regions of MB2 were constructed as recombinant fusions sandwiched between glutathione S-transferase and a hexa histidine tag for bacterial expression. The hexa histidine tag affinity purified proteins were used to immunize rabbits and the polyclonal sera evaluated in an in vitro inhibition of sporozoite invasion assay. The proteins were also used in immunoblots with sera from a limited number of donors immunized via the bites of P. falciparum infected irradiated mosquitoes and plasma and serum obtained from naturally exposed individuals in Kenya. Results Rabbit polyclonal antibodies targeting the non-repeat region of the basic domain of MB2 inhibited sporozoites entry into HepG2-A16 cells in vitro. Analysis of serum from five human volunteers that were immunized via the bites of P. falciparum infected irradiated mosquitoes that developed immunity and were completely protected against subsequent challenge with non-irradiated parasite also had detectable levels of antibody against MB2 basic domain. In contrast, in three volunteers not protected, anti-MB2 antibodies were below the level of detection. Sera from protected volunteers preferentially recognized a non-repeat region of the basic domain of MB2, whereas plasma from naturally-infected individuals also had antibodies that recognize regions of MB2 that contain a repeat motif in immunoblots. Sequence analysis of eleven field isolates and four laboratory strains showed that these antigenic regions of the basic domain of the MB2 gene are highly conserved in parasites obtained from different parts of the world. Moreover, anti-MB2 antibodies also were detected in the plasma of 83% of the individuals living in a malaria endemic area of Kenya (n = 41). Conclusion A preliminary analysis of the human humoral response against MB2 indicates that it may be an additional highly conserved target for immune intervention at the pre-erythrocytic stage of P. falciparum life cycle.

Published
2009

7. The development of a multivalent DNA vaccine for malaria

Author

Hedstrom, Richard C., Doolan, Denise L., Wang, Ruobing, Gardner, Malcolm J., Kumar, Anita, Sedegah, Martha, Gramzinski, Robert A., Sacci, John B., Jr., Charoenvit, Yupin, Weiss, Walter R., Margalith, Michal, Norman, Jon A., Hobart, Peter, Hoffman, Stephen L., and Raz, Eyal, editor

Published
1998
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8. Preerythrocytic, Live-Attenuated Plasmodium falciparum Vaccine Candidates by Design

Author

VanBuskirk, Kelley M., O'Neill, Matthew T., De La Vega, Patricia, Maier, Alexander G., Krzych, Urszula, Williams, Jack, Dowler, Megan G., Sacci,, John B., Kangwanrangsan, Niwat, Tsuboi, Takafumi, Kneteman, Norman M., Heppner,, Donald G., Murdock, Brant A., Mikolajczak, Sebastian A., Aly, Ahmed S. I., Cowman, Alan F., Kappe, Stefan H. I., and James, Anthony A.

Published
2009
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15. A proteomic view of the Plasmodium falciparum life cycle

Author

Florens, Laurence, Washburn, Michael P., Raine, J. Dale, Anthony, Robert M., Grainger, Munira, Haynes, J. David, Moch, J. Kathleen, Muster, Nemone, Sacci, John B., Tabb, David L., Witney, Adam A., Wolters, Dirk, Wu, Yimin, Gardner, Malcolm J., Holder, Anthony A., Sinden, Robert E., Yates, John R., and Carucci, Daniel J.

Published
2002
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17. Clinical trial in healthy malaria-naïve adults to evaluate the safety, tolerability, immunogenicity and efficacy of MuStDO5, a five-gene, sporozoite/hepatic stage Plasmodium falciparum DNA vaccine combined with escalating dose human GM-CSF DNA

Author

Richie, Thomas L., Charoenvit, Yupin, Wang, Ruobing, Epstein, Judith E., Hedstrom, Richard C., Kumar, Sanjai, Luke, Thomas C., Freilich, Daniel A., Aguiar, Joao C., Sacci, John B., Jr., Sedegah, Martha, Nosek, Ronald A., Jr., De La Vega, Patricia, Berzins, Mara P., Majam, Victoria F., Abot, Esteban N., Ganeshan, Harini, Richie, Nancy O., Banania, Jo Glenna, Baraceros, Maria Fe B., Geter, Tanya G., Mere, Robin, Bebris, Lolita, Limbach, Keith, Hickey, Bradley W., Lanar, David E., Ng, Jennifer, Shi, Meng, Hobart, Peter M., Norman, Jon A., Soisson, Lorraine A., Hollingdale, Michael R., Rogers, William O., Doolan, Denise L., and Hoffman, Stephen L.

Published
2012

18. Novel malaria antigen Plasmodium yoelii E140 induces antibody-mediated sterile protection in mice against malaria challenge

Author

Smith, Emily C., primary, Limbach, Keith J., additional, Rangel, Nonenipha, additional, Oda, Kyosuke, additional, Bolton, Jessica S., additional, Du, Mengyan, additional, Gowda, Kalpana, additional, Wang, Jianyang, additional, Moch, J. Kathleen, additional, Sonawane, Sharvari, additional, Velasco, Rachel, additional, Belmonte, Arnel, additional, Danner, Rebecca, additional, Lumsden, Joanne M., additional, Patterson, Noelle B., additional, Sedegah, Martha, additional, Hollingdale, Michael R., additional, Richie, Thomas L., additional, Sacci, John B., additional, Villasante, Eileen D., additional, and Aguiar, Joao C., additional

Published
2020
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19. The development of a multivalent DNA vaccine for malaria

Author

Hedstrom, Richard C., primary, Doolan, Denise L., additional, Wang, Ruobing, additional, Gardner, Malcolm J., additional, Kumar, Anita, additional, Sedegah, Martha, additional, Gramzinski, Robert A., additional, Sacci, John B., additional, Charoenvit, Yupin, additional, Weiss, Walter R., additional, Margalith, Michal, additional, Norman, Jon A., additional, Hobart, Peter, additional, and Hoffman, Stephen L., additional

Published
1998
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27. Mosquito bite immunization with radiation-attenuated Plasmodium falciparum sporozoites: safety, tolerability, protective efficacy and humoral immunogenicity

Author

Hickey, Bradley W., primary, Lumsden, Joanne M., additional, Reyes, Sharina, additional, Sedegah, Martha, additional, Hollingdale, Michael R., additional, Freilich, Daniel A., additional, Luke, Thomas C., additional, Charoenvit, Yupin, additional, Goh, Lucy M., additional, Berzins, Mara P., additional, Bebris, Lolita, additional, Sacci, John B., additional, De La Vega, Patricia, additional, Wang, Ruobing, additional, Ganeshan, Harini, additional, Abot, Esteban N., additional, Carucci, Daniel J., additional, Doolan, Denise L., additional, Brice, Gary T., additional, Kumar, Anita, additional, Aguiar, Joao, additional, Nutman, Thomas B., additional, Leitman, Susan F., additional, Hoffman, Stephen L., additional, Epstein, Judith E., additional, and Richie, Thomas L., additional

Published
2016
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29. Disruption of the Plasmodium falciparum liver-stage antigen-1 locus causes a differentiation defect in late liver-stage parasites

Author

Mikolajczak, Sebastian A., Sacci, John B., De La Vega, Patricia, Camargo, Nelly, VanBuskirk, Kelly, Krzych, Urszula, Cao, Jun, Jacobs-Lorena, Marcelo, Cowman, Alan F., and Kappe, Stefan H. I.

Subjects
Mice, Merozoites, Sporozoites, Plasmodium falciparum, Hepatocytes, Protozoan Proteins, Animals, Humans, Antigens, Protozoan, Mice, SCID, Article, Gene Deletion, Cell Line
Abstract

The malaria parasite Plasmodium falciparum infects humans and first targets the liver where liver-stage parasites undergo pre-erythrocytic replication. Liver-stage antigen-1 (LSA-1) is currently the only identified P. falciparum protein for which expression is restricted to liver stages. Yet, the importance of LSA-1 for liver-stage parasite development remains unknown. Here we deleted LSA-1 in the NF54 strain of P. falciparum and analysed the lsa-1(-) parasites throughout their life cycle. lsa-1(-) sporozoites had normal gliding motility and invasion into hepatocytes. Six days after infection of a hepatocytic cell line, lsa-1(-) parasites exhibited a moderate phenotype with an ~50% reduction of late liver-stage forms when compared with wild type. Strikingly, lsa-1(-) parasites growing in SCID/Alb-uPA mice with humanized livers showed a severe defect in late liver-stage differentiation and exo-erythrocytic merozoite formation 7 days after infection, a time point when wild-type parasites develop into mature merozoites. The lsa-1(-) parasites also showed aberrant liver-stage expression of key parasite proteins apical membrane antigen-1 and circumsporozoite protein. Our data show that LSA-1 plays a critical role during late liver-stage schizogony and is thus important in the parasite transition from the liver to blood. LSA-1 is the first P. falciparum protein identified to be required for this transitional stage of the parasite life cycle.

Published
2011

30. Discovery of Novel Plasmodium falciparum Pre-Erythrocytic Antigens for Vaccine Development

Author

Aguiar, Joao C., primary, Bolton, Jessica, additional, Wanga, Joyce, additional, Sacci, John B., additional, Iriko, Hideyuki, additional, Mazeika, Julie K., additional, Han, Eun-Taek, additional, Limbach, Keith, additional, Patterson, Noelle B., additional, Sedegah, Martha, additional, Cruz, Ann-Marie, additional, Tsuboi, Takafumi, additional, Hoffman, Stephen L., additional, Carucci, Daniel, additional, Hollingdale, Michael R., additional, Villasante, Eileen D., additional, and Richie, Thomas L., additional

Published
2015
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48. Inhibition of Liver-Stage Development Assay.

Author

Walker, John M., Doolan, Denise L., and Sacci, John B.

Abstract

In vitro infection of hepatocyte monolayer cultures with plasmodial sporozoites has become a valuable tool for the dissection of host-cell parasite interactions (1-4). This methodology has facilitated the study of how antibodies, cytokines, drugs, and immune effector cells can influence the infection of hepatocytes with plasmodial parasites. In vitro cultures have the advantage of allowing an investigator to isolate hepatocytes from nonparenchymal cells, thus avoiding any confounding of the results that might occur due to an interaction of the test conditions with nonparenchymal cells (kupffer cells, endothelial cells, lymphocytes, etc.). Several different types of inhibition of liverstage development assay (ILSDA) procedures can be utilized. They fall into two different categories: blocking entry of the parasite into the hepatocyte or inhibiting development of the liver stage schizont after infection. The first procedure is used to determine if immune sera can prevent the entry of parasites into the hepatocytes, while the other can be used to assess the capacity of sera, immune effector cells or drugs to affect the development of the intracellular liver stage parasite. Because these assays are assessing different aspects of the host-parasite relationship, the practical aspects of these tests are slightly different. [ABSTRACT FROM AUTHOR]

Published
2002
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