Biochemical, biophysical and cellular studies of selenophosphate synthetase from Naegleria gruberi

The target microorganism of the present study belongs to the Naegleria genus. This genus includes free life amoebas widely distributed around the world that, in order to survive in bad temperature and pH environments, developed an adaptive strategy consisting of cells differentiation to flagellate and cystic form. The biosynthesis and incorporation of selenocysteine amino acid (Sec, U) in N. gruberi has been described and, because of the co-translational incorporation of this amino acid in response to a UGA codon during the reading step, this process has several specific factors which make it a target for molecular studies. Among the identified genes, we can highlight the one which encodes the selenophosphate synthetase that is involved in the catalytic conversion of selenite and adenosine triphosphate into selenium phosphate, a necessary step to the Sec synthesis that uses selenide and ATP to produce selenophosphate. SPS from N.gruberi is encoded with an methyltransferase N-terminal fused with the typical SPS C-terminal domain, an open read frame that contains 2211 nucleotides encoding 737 amino acids. This discovery has motivated the initial aims of this project, based on the cellular investigation of SPS2, native on the three different form lifes of N. gruberi, through immunoenzymatic assays, besides a study with the recombinant protein to clarify the biochemistry and biophysics features of NgSPS2. The results indicated that the protein do not keep both domains fused after the translation process, suggesting that they need to be separated to perform their biological function. The investigation of the N. gruberi culture revealed that the cells become less sensitive to stress agent in the presence of selenium, which seems to be correlated with the increasing activity of the selenoprotein synthesis. The biochemistry characterization of the NgSPS2 C-terminal domain, using size exclusion chromatography and electrophoresis under non-denaturing conditions revealed the predominance of dimers in solution according with the typical homologous SPS oligomeric state. The crystallization tests have not resulted in crystal growth; however, the limited proteolysis may be an alternative to optimize the crystallization process. These studies may enlarge the knowledge about the biosynthesis of Sec. in N. gruberi. (AU)