Deletion of SET1 enhances the termination defect of nrd1 and nab3 mutants. (A, top) Schematic representation of the SNR13 region. SNR13 is upstream of the infrequently transcribed TRS31 gene. The probe used for hybridization is indicated by the horizontal bar below the schematic. (Bottom) Total RNA (5 μg) from WT (BY4741), set1Δ (YSB2253), nrd1(1-164Δ) (YSB2094), nrd1(1-164Δ) set1Δ (YSB2153), nrd1(151-214Δ) (YSB2086), and nrd1(151-214Δ) set1Δ (YSB2152) strains was analyzed by Northern blot using the SNR13 probe. The positions of mature full-length snR13 and stable snR13-TRS31 read-through RNAs are marked on the left. The bottom shows methylene blue staining of 25S and 18S rRNAs as a loading control. Transcripts were quantitated with a phosphorimager. snR13 read-through transcripts were calculated as a percentage of full-length snR13. These numbers were divided by the value for the nrd1(151-214Δ) strain to give the “fold over nrd1(151-214Δ)” values listed below each lane. (B) Effect of set1Δ on the snR13 read-through transcript levels in nrd1(1-164Δ) and nrd1(151-214Δ) mutants quantified as the ratio of the nrd1 set1 double mutant to the nrd1 mutant alone using values from at least four Northern blot experiments. Error bars show standard deviations. (C) RT-PCR of snR13 read-through (26 cycles, using primers downstream of the normal termination site) and total (full-length plus read-through) transcripts (20 cycles, using primers within the mature snR13) were performed on RNA from three independent cultures of nab3-11 (YF1471) and nab3-11 set1Δ (YSB2559) strains grown at the semipermissive temperature of 30°C. Quantitation by phosphorimager analysis is expressed by dividing the read-through by the total signal. Because these ratios were not corrected for numbers of PCR cycles, they are a relative, not absolute, measure of the read-through. This experiment was repeated by using RT-qPCR, which gave similar results (see Fig. S1B in the supplemental material). (D, top) Schematic representation of the rDNA region. 35S rRNA genes are interspersed with nontranscribed spacer 1 (NTS1), the 5S rRNA gene (black arrow), and nontranscribed spacer 2 (NTS2). The position of the probe used to detect the NTS1 CUT is shown below the diagram as a black line. (Bottom) RNA samples as in panel A were analyzed by Northern blotting using the NTS1 CUT probe. Levels of the NTS1 CUT were normalized to the methylene blue 25S rRNA signal. These values for each strain were then divided by the value of the nrd1(151-214Δ) strain to give the “fold over nrd1(151-214Δ)” values that are listed below each lane.