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hages and dendritic cells of their mammalian hosts. In eukaryotic cells protein phosphorylation is a major mechanism of signal transduction, and involved in regulation of many different cellular processes including differentiation, cell division, and host-pathogen responses. Previously it was demonstrated that protein kinases, including casein kinase 1 and casein kinase 2, are released/secreted by promastigotes of several Leishmania species. Constitutive or induced release of CK1 and CK2 from promastigotes could be modulated by temperature and pH, two important environmental cues for leishmanial differentiation from promastigotes to amastigotes and visa versa. Modification of temperature and acidic pH, have been utilized for axenic amastigote propagation in vitro and studies on parasite differentiation. Enzymes belonging to the CK1 family are found in all eukaryotes from protozoa to humans where they phosphorylate a wide range of protein substrates involved in various processes including: cell cycle, receptor signaling, transport, apoptosis, transcription, and DNA repair. Several CK1 isoforms have been characterized in yeast, and at least six isoforms have been identified in humans. The catalytic domains of CK1 isoforms are highly conserved, but the N-terminal and C-terminal non-catalytic domains differ significantly in both length and primary amino acid sequence. CK1 isoforms tend to be constitutively expressed, and characterized by an acidophilic target phosphorylation sites. These sites are frequently adjacent serine/ threonine residues phosphorylated by other protein kinases allowing CK1 to act in hierarchical manner and further modulated activity of other protein kinases. Secreted Casein Kinase 1.4 Analysis of the TriTryp kinome identified multiple CK1 isoforms in L. major, Trypanosoma cruzi and T. brucei , of which four are conserved among trypanosomatids. CK1 1685439 isoform two, present in all three trypanosomatids, Apigenin site appears to be essential for parasite growth. Knockdown of ck1.2 expression in T. brucei bloodstream forms results in major morphological changes and death, while protein kinase inhibitors inhibiting Leishmania promastigote growth were shown to bind and inhibit leishmanial CK1.2 . CK1 isoforms in other organisms have been localized to specific subcellular environments including the nucleus, cytosol, and plasma membrane. Recently analysis of the Leishmania secretome using conditioned culture medium showed that CK1.2 is released by promastigotes, and appears to be associated with exosomes released by the parasites. Expression of L. major CK1.2 in mammalian cells stimulated the phosphorylationdependent degradation of the IFNAR1 chain of the IFN type I receptor and attenuation of IFN-a/b signaling, suggesting that secreted CK1s may also play a role as parasite virulence factors. Further analysis of the TriTryp kinome identified a CK1 isoform unique to Leishmania that appears to have a secretion signal sequence. Here we report on the cloning, expression and molecular characterization of CK1 isoform 4 from L. donovani. Over expression in L. donovani demonstrates that isoform 4 is secreted by the parasite, and plays 11414653 a role in parasite growth and survival. These results encourage further investigations of leishmanial CK1.4 as a potential chemotherapeutic target. submitted to NCBI GeneBank. Predicted protein sequence alignment and motif analysis was carried out using ClustalW2 and motif scan, respectively. Blast analysis using both th

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Author: Interleukin Related