The mutation G143A in the inhibitor binding site of cytochrome b confers a high level of resistance to fungicides targeting the bc 1 complex. The mutation, reported in many plant-pathogenic fungi, has not evolved in fungi that harbor an intron immediately after the codon for G143 in the cytochrome b gene, intron bi2. Using Saccharomyces cerevisiae as a model organism, we show here that a codon change from GGT to GCT, which replaces glycine 143 with alanine, hinders the splicing of bi2 by altering the exon/intron structure needed for efficient intron excision. This lowers the levels of cytochrome b and respiratory growth. We then investigated possible bypass mechanisms that would restore the respiratory fitness of a resistant mutant. Secondary mutations in the mitochondrial genome were found, including a point mutation in bi2 restoring the correct exon/intron structure and the deletion of intron bi2. We also found that overexpression of nuclear genes MRS2 and MRS3, encoding mitochondrial metal ion carriers, partially restores the respiratory growth of the G143A mutant. Interestingly, the MRS3 gene from the plant-pathogenic fungus Botrytis cinerea, overexpressed in an S. cerevisiae G143A mutant, had a similar compensatory effect. These bypass mechanisms identified in yeast could potentially arise in pathogenic fungi.The mitochondrial bc 1 complex is a membrane-bound multisubunit enzyme that catalyzes the transfer of electrons from ubiquinol to cytochrome c and couples this electron transfer to the vectorial translocation of protons across the inner mitochondrial membrane. Cytochrome b is the central membraneembedded subunit that forms the ubiquinol binding pockets called Q o and Q i .A number of quinol antagonists are known that inhibit bc 1 complex activity. These are either specific for the Q i site, such as antimycin, or for the Q o site, such as myxothiazol, stigmatellin, and the strobilurins. A range of Q o inhibitor compounds (Q o Is) have been developed as antimicrobial agents and are now widely used in agriculture to control fungal and oomycete plant pathogens. Unfortunately, acquired resistance has rapidly emerged in field populations of the plant pathogens. The cytochrome b mutation G143A plays a central role in the mechanism of resistance. The mutation has been reported in most Q o I-resistant pathogens (see http://www.frac.info/frac /index.htm and references within). G143A causes a high level of resistance (ÏŸ100Ï«) in pathogens, which are consequently controlled poorly or not at all by Q o Is. In the model organism Saccharomyces cerevisiae, G143A also dramatically increases resistance to myxothiazol (18,000Ï«) and azoxystrobin (4,000Ï«) (8). G143 is a highly conserved residue located in the Q o pocket, close to the inhibitor binding site. The replacement of glycine with alanine would prevent inhibitor binding through simple steric hindrance while the Q o site remains functional, as observed in the yeast model (8).The cytochrome b gene is encoded by the mitochondrial genome in all eukaryotes. In fungi, lar...