Abstract
Nuclear gene(s) have been shown to modulate the phenotypic expression of mitochondrial DNA mutations. We report here the identification and characterization of the yeast nuclear gene MTO2 encoding an evolutionarily conserved protein involved in mitochondrial tRNA modification. Interestingly, mto2 null mutants expressed a respiratory-deficient phenotype when coexisting with the C1409G mutation of mitochondrial 15 S rRNA at the very conservative site for human deafness-associated 12 S rRNA A1491G and C1409T mutations. Furthermore, the overall rate of mitochondrial translation was markedly reduced in a yeast mto2 strain in the wild type mitochondrial background, whereas mitochondrial protein synthesis was almost abolished in a yeast mto2 strain carrying the C1409G allele. The other interesting feature of mto2 mutants is the defective expression of mitochondrial genes, especially CYTB and COX1, but only when coexisting with the C1409G allele. These data strongly indicate that a product of MTO2 functionally interacts with the decoding region of 15 S rRNA, particularly at the site of the C1409G or A1491G mutation. In addition, we showed that yeast and human Mto2p localize in mitochondria. The isolated human MTO2 cDNA can partially restore the respiratory-deficient phenotype of yeast mto2 cells carrying the C1409G mutation. These functional conservations imply that human MTO2 may act as a modifier gene, modulating the phenotypic expression of the deafness-associated A1491G or C1409T mutation in mitochondrial 12 S rRNA.
Highlights
Interaction between the nuclear and mitochondrial genomes is necessary for controlling the phenotypic expression of mtDNA mutation(s)
We have identified and characterized yeast MTO2, a nuclear gene encoding a mitochondrial protein involved in tRNA modification
In E. coli, TrmU has been shown to be responsible for the biosynthesis of hypermodified 2-thiouridine (s2U) in the wobble position of tRNALys, tRNAGlu, and tRNAGln (21, 40 – 42). 2-Thiouridine modification was found in the wobble position of the yeast mitochondrial tRNAs [43]
Summary
Cloning of Yeast MTO2—The peptide sequence of the E. coli trmU sequence [30] was subjected to a BLAST search of the publicly available S. cerevisiae sequence databases (NCBI/GenbankTM/EMBL). This search led to the identification of one open reading frame encoding a protein (YDL033C, GenBankTM accession number Z71781) with a high degree of homology to E. coli TrmU. To obtain the full-length coding region of MTO2 DNA, PCR was performed using the high fidelity Pfu DNA polymerase (Promega) and total yeast genomic DNA isolated from W303–1B cells as a template, with primers 5Ј-AATTTTAAGAGCGCCGGG-3Ј (nucleotides (nt)1 143–163) and 5Ј-ACATGATTCAAGGGAAAAGACC-3Ј (nt 1713–1734) (GenBankTM accession number AY624369). W303–1B W1021–7C M12 M12–54 A18 W303⌬MTO1(PR) W303⌬MTO2(PS) W303⌬MTO2(o) W1021⌬MTO2(PS) W1021⌬MTO2(o) QY1
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