Leishmania mexicana: promastigotes and amastigotes secrete protein phosphatases and this correlates with the production of inflammatory cytokines in macrophages

Author:

ESCALONA-MONTAÑO A. R.,ORTIZ-LOZANO D. M.,ROJAS-BERNABÉ A.,WILKINS-RODRIGUEZ A. A.,TORRES-GUERRERO H.,MONDRAGÓN-FLORES R.,MONDRAGÓN-GONZALEZ R.,BECKER I.,GUTIÉRREZ-KOBEH L.,AGUIRRE-GARCIA M. M.

Abstract

SUMMARYPhosphatase activity ofLeishmaniaspp. has been shown to deregulate the signalling pathways of the host cell. We here show thatLeishmania mexicanapromastigotes and amastigotes secrete proteins with phosphatase activity to the culture medium, which was higher in the Promastigote Secretion Medium (PSM) as compared with the Amastigote Secretion Medium (ASM) and was not due to cell lysis, since parasite viability was not affected by the secretion process. The biochemical characterization showed that the phosphatase activity present in PSM was higher in dephosphorylating the peptide END (pY) INASL as compared with the peptide RRA (pT)VA. In contrast, the phosphatase activity in ASM showed little dephosphorylating capacity for both peptides. Inhibition assays demonstrated that the phosphatase activity of both PSM and ASM was sensible only to protein tyrosine phosphatases inhibitors. An antibody against a protein phosphatase 2C (PP2C) ofLeishmania majorcross-reacted with a 44·9 kDa molecule in different cellular fractions ofL. mexicanapromastigotes and amastigotes, however, in PSM and ASM, the antibody recognized a protein about 70 kDa. By electron microscopy, the PP2C was localized in the flagellar pocket of amastigotes. PSM and ASM induced the production of tumor necrosis factor alpha, IL-1β, IL-12p70 and IL-10 in human macrophages.

Publisher

Cambridge University Press (CUP)

Subject

Infectious Diseases,Animal Science and Zoology,Parasitology

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