6xHIS and Δcox15 with ScCOX156xHIS, as positive controls Using

6xHIS and Δcox15 with ScCOX15.6xHIS, as positive controls. Using two different expression vectors (see Materials and methods), the same phenotype suppression was observed, demonstrating that T. cruzi sequences are able to complement yeast respiratory deficiencies. To confirm these results, the oxygen consumption of WT, Δcox10, Δcox15 yeast strains and their corresponding transformants was measured (Fig. 2b). As expected, the knockout cells were impaired in O2 consumption due to their inability to produce heme A and consequently fully active CcO. The respiratory function was restored selleck chemicals with the expression of the corresponding T. cruzi COX10 and COX15

genes, as well as with the S. cerevisiae COX10 and COX15 genes. Taken together, these results demonstrate that TcCOX10 and TcCOX15 encode HOS and HAS enzymes that are functional in the yeast model. In order to verify the function of these proteins in heme A biosynthesis, the mitochondrial heme level was evaluated by differential absorption spectroscopy as described previously (Tzagoloff et al., 1975). The reduced minus oxidized spectra of mitochondrial cytochromes were recorded and are presented in Fig. 3a. The spectra of the knockout

cells only exhibited signals corresponding to heme b and heme c, and the heme a signal was absent, confirming the deficiency of its biosynthesis (Nobrega et al., 1990; Glerum et al., 1997). The spectrum recorded from the mitochondria of WT cells displayed bands corresponding to heme a, heme b

and heme c. The expression of TcCOX10 in Δcox10 and TcCOX15 in Δcox15 allowed the recovery of the heme a signal, reflecting the role in heme A synthesis of the TcCox10 and TcCox15 proteins NVP-BGJ398 datasheet as HOS and HAS enzymes, respectively. The protein levels of Cox10 and Cox15 were evaluated using Western blot analysis of yeast mitochondria. All these proteins (from S. cerevisiae and T. cruzi) were expressed as C-terminal his-tag fusion proteins (Fig. 3b). As expected, the proteins were detectable in the cells transformed with the plasmids expressing TcCOX10.6xHIS, GBA3 ScCOX10.6xHIS, TcCOX15.6xHIS and/or ScCOX15.6xHIS, and they were not detectable in the WT, Δcox10 or Δcox15 cells transformed with control vectors. The signals detected at around 38–45 kDa were consistent with the apparent molecular weight expected for TcCox10 and TcCox15 proteins based on their primary sequences (for TcCox10 388 aa, 42 kDa and for TcCox15 396 aa, 44 kDa, both molecular weights were estimated for the preprotein without the C-terminal tag, TriTrypDB, http://tritrypdb.org/tritrypdb/). In both cases, the band intensity of the T. cruzi proteins was always lower compared with the S. cerevisiae ones. Several factors could be involved in this observation: (1) the different mitochondrial targeting sequence [shorter in trypanosomatids (Hausler et al., 1997)] resulted in less efficient mitochondrial importation; (2) the lower stability of the T. cruzi proteins compared with the S.

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