Standard molecular procedures were performed as described by Ausubel et al.
(1995). The bifunctional yeast – E. coli vector YCpLac33 ( Gietz and Sugino, 1988) was used as template for amplification of ycf1::URA3 disruption cassette. The pmr1Δycf1Δ double mutant was obtained by disruption of the YCF1 gene by homologous recombination with the ycf1::URA3 cassette. The latter was amplified with Platinum® high fidelity Taq DNA polymerase (Invitrogen) and the primers described in Table 2. Then, the disruption cassette was purified with the PureLink™ gel extraction kit (Invitrogen) and employed for transformation of the pmr1Δ strain. The disruption was confirmed by PCR and restriction analyses performed with phenol–chloroform purified genomic DNA from potential yeast transformant colonies selected in SC medium lacking Osimertinib in vivo uracil. Yeast strains were growth in SC medium at 30 °C until the stationary phase, then harvested by centrifugation (1 min/15,000 × g) and washed twice with distilled water. For survival assays, 1.2 × 107 cells/mL were treated in SC medium supplemented or not with CdCl2 (50 μM, 100 μM, 200 μM or 400 μM) and incubated for 4 h in an orbital shaker (120 rpm) at 30 °C. After the treatments, cells were washed and diluted to 1.2 × 103 cells/mL. Aliquots of buy Galunisertib 100 μL were plated in SC solid medium
and incubated at 30 °C for 2–3 d to determine cell viability. The yeast strains were treated with 50 μM CdCl2 as
described in section 2.3. At 1 h intervals, Y-27632 chemical structure 10 mL aliquots were collected. Then, 1 mL of these samples was used for survival determination and the remaining 9 mL was centrifuged and subjected to atomic absorption using a 3100 Atomic Absorption Spectrometer (PerkinElmer) for quantification of residual Cd2+ concentration in the supernatant. Cd2+ content was estimated by determining the difference in metal concentration between control medium without biomass and test medium containing biomass (Gomes et al., 2002). The results were normalized with respect to the number of surviving cells at each time point, and are expressed as micrograms of Cd2+ absorbed by 107 surviving cells. The strains were treated as described in Section 2.3. After 4 h, cells were harvested for total RNA extraction using RNeasy Mini Kit (Qiagen) according to the manufacturer’s instructions. About 200–300 ng of total RNA previously treated with DNAse I amplification grade (Promega) were subjected to first strand cDNA synthesis using the poly-T antisense primer, and the M-MLV reverse transcriptase (Promega). PCR was carried out with Platinum Taq DNA polymerase (Invitrogen) and the specific primers described in Table 2. The reactions were performed with 20 ng of first strand cDNA, except for PMC1, for which 10 ng was used. The ACT1 gene was employed as a constitutive control.