Article ID Journal Published Year Pages File Type
9140064 Molecular and Biochemical Parasitology 2005 13 Pages PDF
Abstract
Previous affinity chromatography experiments have described the unexpected binding of an isoform of casein kinase I (CK1) from Leishmania mexicana, Trypanosoma cruzi, Plasmodium falciparum and Toxoplasma gondii to an immobilized cyclin-dependent kinase (CDK) inhibitor (purvalanol B). In order to further evaluate CK1 as a potential anti-parasitic target, two T. gondii CK1 genes were cloned by PCR using primers derived from a putative CK1 gene fragment identified from a T. gondii EST database. The genes are predicted to encode a smaller polypeptide of 38 kDa (TgCK1α) and larger 49 kDa isoform bearing a C-terminal extension (TgCK1β). Enzymatically active recombinant FLAG-epitope tagged TgCK1α and TgCK1β enzymes were immuno-precipitated from transiently transfected T. gondii parasites. While TgCK1α expression was found to be cytosolic, TgCK1β was expressed predominantly at the plasma membrane. Deletion mapping showed that the C-terminal domain of TgCK1β confers this membrane-association. Recombinant TgCK1α and TgCK1β isoforms were also expressed in E. coli and biochemically characterized. A 38 kDa native CK1 activity was partially purified from T. gondii tachyzoites by ion-exchange and hydrophobic interaction chromatography with biochemical and serological properties closely resembling those of recombinant TgCK1α. In contrast, we were not able to identify a native CK1 activity corresponding to the larger TgCK1β 49 kDa isoform in tachyzoite lysates. Purvalanol B and the related compound aminopurvalanol A selectively inhibit TgCK1α, confirming the existence of potentially exploitable structural differences between host and parasite CK1 enzymes. Since the more cell-permeable aminopurvalanol also inhibits parasite growth, these results provide further impetus to investigate inhibitors of CK1 as anti-parasitic agents.
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