Evidence for CRK3 participation in the cell division cycle of Trypanosoma cruzi

Santori, MI; Laria, S; Gomez, EB; Espinosa, I; Galanti N.; Tellez-Inon, MT

Abstract

Trypanosoma cruzi CRK3 gene encodes a Cdc2p related protein kinase (CRK). To establish if it has a role in the regulation of the parasite cell cycle we studied CRK3 expression and activity throughout three life cycle stages. CRK3 from epimastigote soluble extracts interacted with p13suc1-beads. Endogenous CRK3 phosphorylated histone H1 and this activity was inhibited by specific CDK inhibitors: Olomoucine, Flavopiridol and Roscovitine. Flavopiridol partially inhibited the growth of T. cruzi epimastigotes at 50 nM, the lowest concentration used, but even with the highest (5 ?M), cell growth was not completely arrested. CRK3 from Flavopiridol-inhibited epimastigote extracts exhibited a dose dependent inhibition of histone H1 phosphorylation. T. cruzi p13suc1-binding CRK displayed the same inhibition profile. This suggests that CRK3 is the enzyme responsible for the majority of the kinase activity associated with p13suc1. CRK3 activity of hydroxyurea (HU) synchronized epimastigotes peaked in G2/M boundary while the kinase activity associated to p13suc1-beads increased at the same time point but remained high until late G2/M. In addition, CRK3 expression was constant during the cell cycle. This is a common pattern of CDK activity regulation. Taken together, these results support the idea that CRK3 is involved in control of the cell cycle in T. cruzi. © 2002 Elsevier Science B.V. All rights reserved.

Más información

Título según WOS: Evidence for CRK3 participation in the cell division cycle of Trypanosoma cruzi
Título según SCOPUS: Evidence for CRK3 participation in the cell division cycle of Trypanosoma cruzi
Título de la Revista: MOLECULAR AND BIOCHEMICAL PARASITOLOGY
Volumen: 121
Número: 2
Editorial: Elsevier
Fecha de publicación: 2002
Página de inicio: 225
Página final: 232
Idioma: English
URL: http://linkinghub.elsevier.com/retrieve/pii/S0166685102000397
DOI:

10.1016/S0166-6851(02)00039-7

Notas: ISI, SCOPUS