Leishmania amazonensis: early proteinase activities during promastigote–amastigote differentiation in vitro

Leishmania proteinase activity is known as parasite differentiation marker, and has been considered relevant for leishmanial survival and virulence. These properties suggest that Leishmania proteinases can be promising targets for development of anti-leishmania drugs. Here, we analyze the activities...

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Bibliographic Details
Published in:Experimental parasitology 2005, Vol.109 (1), p.38-48
Main Authors: Alves, C.R., Corte-Real, S., Bourguignon, S.C., Chaves, C.S., Saraiva, E.M.B.
Format: Article
Language:English
Subjects:
Amastigote-like
Animals
Biological and medical sciences
Cathepsin
Chromogenic Compounds - metabolism
Cysteine proteinases
Cytoplasmic Vesicles - enzymology
Flagella - enzymology
Fundamental and applied biological sciences. Psychology
Hot Temperature
Hydrogen-Ion Concentration
Hydrolysis
Immune Sera - immunology
Immunoblotting
Immunohistochemistry
Leishmania amazonensis
Leishmania mexicana - enzymology
Leishmania mexicana - growth & development
Leishmania mexicana - ultrastructure
Life cycle. Host-agent relationship. Pathogenesis
Peptide Hydrolases - metabolism
Proteinases
Protozoa
Protozoan Proteins - metabolism
Rabbits
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Summary:Leishmania proteinase activity is known as parasite differentiation marker, and has been considered relevant for leishmanial survival and virulence. These properties suggest that Leishmania proteinases can be promising targets for development of anti-leishmania drugs. Here, we analyze the activities of four proteinases during the early phase of the Leishmania amazonensis promastigotes differentiation into amastigotes induced by heat shock. We have examined activities of cysteine-, metallo-, serine-, and aspartic-proteinase by hydrolysis of specific chromogenic substrates at pH 5.0 and at the optimal pH for each enzyme. Our results show that metallo-, serine-, and aspartic-proteinases activities were down-regulated during the shock-induced transformation of promastigotes into amastigotes. In contrast, cysteine-proteinase activity increased concomitantly with the promastigote differentiation. Immunocytochemical localization using two anti-cysteine-proteinase monospecific rabbit antibodies detected the enzyme in several cell compartments of both parasite stages. Our results show different proteinase activity modulation and expression during the early phases of the shock-induced parasite transformation.
ISSN:0014-4894
1090-2449
DOI:10.1016/j.exppara.2004.10.005