(A) Ty1 structure and transcription. Ty1 structure consists of two direct long terminal repeats (LTR, symbolized by black triangles) and two open reading frames, TYA and TYB, analogs of the retroviral gag and pol genes. Ty1 transcription regulatory sequences are located within the first kilobase of the retrotransposon. Dotted arrows indicate Ty1 mRNA and Ty1-AS RNA. LTR-lacZ and TYA-lacZ fusions are indicated by bent arrows under the box. (B) Functional classes of genes differentially expressed in adenine-deprived bas1Δ cells relative to adenine-supplied bas1Δ cells. The number of genes whose expression was up- or down-regulated (in parentheses) by at least a factor of 2.5 is indicated for each class. (C) Northern-blot analysis of Ty1, Ty2 and Ty3 mRNA levels in wild-type (FYBL1-23D) and bas1Δ (LV426) cells grown in SDc minimum medium supplemented or not with adenine. For each sample, ∼15 µg of RNA were loaded onto the gel. The sizes of the mRNA molecules are 5.6 kb (Ty1 and Ty2), 5.1 kb (Ty3) and 1.3 kb (ACT1). Ratios were determined on a Molecular Dynamics Phosphorimager with ImageQuant software and set as 1 for wild-type (WT) cells grown with adenine. (D) Northern-blot analysis of Ty1 mRNA in WT (FYBL1-23D), bas1Δ (LV426) pho2Δ (LV1010) and bas1Δ pho2Δ (LV1012) cells grown with and without adenine. PHO84, which is activated by PHO2 served as a positive control (). Growth conditions, the northern-blot experimental procedure and mRNA quantifications are described in the legend of (C).

(A) Intracellular purine derivative contents from the WT (FYBL1-23D), bas1Δ (LV426) and pho2Δ (LV1010) strains. Cells were grown in SDc medium to mid-log phase, metabolites were extracted and intracellular nucleotide concentrations were determined by HPLC. (B) Schematic representation of de novo purine pathway in S. cerevisiae. Ade, adenine; Hypox, hypoxanthine; Gua, guanine ; IMP, inosine 5′-monophosphate; PRPP, 5-phosphoribosyl-1-pyrophosphate. (C) β-Galactosidase activity of a TYA-lacZ fusion at Ty1-ML1 in WT (LV33 Ty1(ML1)-lacZ) and bas1Δ (LV436) cells grown in SDc minimum medium supplemented or not with adenine, hypoxanthine or guanine. β-Galactosidase specific activities are expressed in nanomoles of 2-nitrophenyl β-d-galactopyranoside hydrolyzed per minute per milligram of protein. Data represent the average and standard error of three independent cultures. Intracellular concentrations of ATP and GTP were determined by HPLC as in A and are indicated for each culture below the bars.

(A) β-Galactosidase activity of TYA-lacZ fusions at Ty1-ML1, Ty1-OR and Ty1-ML2 in bas1Δ cells (LV436, LV658 and LV500, respectively) and bas1Δ tye7Δ cells (LV1213, LV1287 and LV1285, respectively). Growth conditions and data representations are described in the legend of C. Exact averages of β-galactosidase specific activities are given above the bars. AF, activation factor (No adenine versus + adenine). (B) Northern-blot analysis of Ty1, Ty2 and Ty3 mRNA levels in WT (FYBL1-23D), bas1Δ (LV426) and bas1Δ tye7Δ (LV1234) cells. Growth conditions, northern-blot experimental procedure and mRNA quantifications are described in the legend of C. (C) Growth assay of WT cells carrying a his3Δ4 allele (LV69, row 1) and WT (LV150, row 3), ste12Δ (LV993, row 2), bas1Δ (LV922, row 4), ste12Δ bas1Δ (LV926, row 5), tye7Δ (LV1370, row 6), bas1Δ tye7Δ (LV1372, row 7) and ste12Δ bas1Δ tye7Δ (LV1374, row 8) cells, carrying a Ty1-his3Δ4 allele. Cells were spotted onto plates in a series of 10-fold dilutions of 1 A₆₀₀ of overnight precultures. All plates were incubated at 30°C for four days. Rows are numbered for clarity.

(A) Coordinates and sequences of potential Tye7 binding sites in Ty1 and Ty2 (E-box I to III). Coordinates are given relative to the numbering of Ty1-H3 () and YLRWTy2-1 (). ENO1 E-box () and Tye7p consensus binding site () are indicated. (B) Chromatin immunoprecipitation (ChIP) analysis of Tye7 occupancy at the Ty1 promoter in bas1Δ (LV1058) and bas1Δ TYE7-MYC (LV1368) strain. Signals are expressed as ratios of ChIP/Total DNA and are set as 1 for untagged TYE7 bas1Δ cells grown with adenine. Data represent the average and standard error of two independent real-time PCR amplifications. (C) β-Galactosidase activity of LTR-lacZ and TYA-lacZ fusions at Ty1-DR3 in bas1Δ cells (LV1013 and LV722, respectively) and bas1Δ tye7Δ cells (LV1320 and LV1341, respectively). Growth conditions and data representations are described in the legend of C. Exact averages of β-galactosidase specific activities are given above the bars. AF, activation factor (versus adenine).

(A) Northern-blot analysis of RNA extracted from WT (FYBL1-23D), bas1Δ (LV426), tye7Δ (LV1232) and bas1Δ tye7Δ (LV1234) cells. L, M and S stand for large, medium and short Ty1-AS RNA species, respectively. (B) Northern-blot analysis of Ty1 mRNA and Ty1-AS RNA levels in WT (FYBL1-23D) and spt3Δ (LV940) cells transformed with pPL297 (TETop-Myc-TYE7, URA3, CEN) or the empty vector p2717. Growth conditions, northern-blot experimental procedure and mRNA quantifications are described in the legend of C.