Abstract

Our long term objectives are to elucidate the questions of how Leishmania infect macrophages, and how these parasites subsequently differentiate, survive and multiply in these phagocytes. Understanding the cellular and molecular mechanisms of such host-parasite interactions in vitro is crucial for developing more effective chemo- and/or immuno-prophylaxis and therapy for leishmaniasis. Leishmania amazonensis molecules previously thought to be important in macrophage infection and thus proposed for investigation are: (1) the major surface glycoprotein/zinc proteinase (gp63); and (2) the 63 kb extrachromosomal DNA circles in tunicamycin (TM)-resistant variants. More emphasis has been placed on the molecular approaches. The gp63 gene of L. amazonensis was cloned and sequenced. Selected residues of gp63 were modified by site-specific mutagenesis of the genes from this and another species. Transfection of gp63-deficient variants with mutant genes allows the identification of catalytically and parasitically important residues. Two additional genes were identified in the 63 kb DNA circle by functional analysis after transfection of wildtype cells with deletion clones of this DNA. One was found to confer tunicamycin-resistance, apparently encoding N-acetylglucosamine-1- phosphate transferase (NAGTase). Using this gene as a selective marker, another gene immediately upstream was identified and found to overexpress a 36 kd protein, homologous to zeta-crystallin/NADPH quinone oxidoreductase (P36). It is proposed to continue the above-mentioned work in conjunction with the established in vitro transfection and macrophage infection systems as follows: (1) To optimize the efficiency of transfection for functional analysis of gp63 and other relevant molecules; (2) To further analyze the biological importance of catalytic, receptor-binding and other functional motifs of gp63 in leishmanial infection; (3) To further characterize the functional significance of posttranslational modifications in regulating gp63 expression by using N-glycosylation and GPI-anchor mutants; (4) Attempts to identify additional molecules of relevance by negative and positive phenotype selections; (5) To delineate """"""""avirulent"""""""" promastigote- derived axenic amastigotes as mutants defective in intracellular differentiation and/or replication. The results of these proposed studies will help our understanding not only Leishmania molecules in their infection of macrophages but also comparable molecules in other biological systems.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Allergy and Infectious Diseases (NIAID)
Type
Research Project (R01)
Project #
5R01AI020486-15
Application #
2671774
Study Section
Tropical Medicine and Parasitology Study Section (TMP)
Project Start
1983-04-01
Project End
2001-07-31
Budget Start
1998-08-01
Budget End
2001-07-31
Support Year
15
Fiscal Year
1998
Total Cost
Indirect Cost

  Institution

Name
Rosalind Franklin University
Department
Microbiology/Immun/Virology
Type
Schools of Medicine
DUNS #
069501252
City
North Chicago
State
IL
Country
United States
Zip Code
60064

  Publications

Dutta, Sujoy; Chang, Celia; Kolli, Bala Krishna et al. (2012) Delta-aminolevulinate-induced host-parasite porphyric disparity for selective photolysis of transgenic Leishmania in the phagolysosomes of mononuclear phagocytes: a potential novel platform for vaccine delivery. Eukaryot Cell 11:430-41
Mehta, Sanjay R; Zhang, Xing-Quan; Badaro, Roberto et al. (2010) Flow cytometric screening for anti-leishmanials in a human macrophage cell line. Exp Parasitol 126:617-20
Varela M, Ruben E; Munoz, Diana Lorena; Robledo, Sara M et al. (2009) Leishmania (Viannia) panamensis: an in vitro assay using the expression of GFP for screening of antileishmanial drug. Exp Parasitol 122:134-9
Mehta, Sanjay R; Huang, Robert; Yang, Meng et al. (2008) Real-time in vivo green fluorescent protein imaging of a murine leishmaniasis model as a new tool for Leishmania vaccine and drug discovery. Clin Vaccine Immunol 15:1764-70
Kolli, Bala Krishna; Kostal, Jan; Zaborina, Olga et al. (2008) Leishmania-released nucleoside diphosphate kinase prevents ATP-mediated cytolysis of macrophages. Mol Biochem Parasitol 158:163-75
Dutta, Sujoy; Furuyama, Kazumichi; Sassa, Shigeru et al. (2008) Leishmania spp.: delta-aminolevulinate-inducible neogenesis of porphyria by genetic complementation of incomplete heme biosynthesis pathway. Exp Parasitol 118:629-36
Dutta, Sujoy; Kolli, Bala Krishna; Tang, Aihua et al. (2008) Transgenic Leishmania model for delta-aminolevulinate-inducible monospecific uroporphyria: cytolytic phototoxicity initiated by singlet oxygen-mediated inactivation of proteins and its ablation by endosomal mobilization of cytosolic uroporphyrin. Eukaryot Cell 7:1146-57
Waki, Kayoko; Dutta, Sujoy; Ray, Debalina et al. (2007) Transmembrane molecules for phylogenetic analyses of pathogenic protists: Leishmania-specific informative sites in hydrophilic loops of trans- endoplasmic reticulum N-acetylglucosamine-1-phosphate transferase. Eukaryot Cell 6:198-210
Thiakaki, Maria; Kolli, Bala; Chang, Kwang-Poo et al. (2006) Down-regulation of gp63 level in Leishmania amazonensis promastigotes reduces their infectivity in BALB/c mice. Microbes Infect 8:1455-63
Dutta, Sujoy; Ray, Debalina; Kolli, Bala K et al. (2005) Photodynamic sensitization of Leishmania amazonensis in both extracellular and intracellular stages with aluminum phthalocyanine chloride for photolysis in vitro. Antimicrob Agents Chemother 49:4474-84

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