Human cervical carcinoma (HeLa S3) cells (24) were grown in Dulbecco’s modified Eagle’s medium (DMEM; Nacarai, Tokyo, Japan), supplemented with 10% fetal bovine serum (FBS) (Sanko Pure Chemicals, Tokyo, Japan) and penicillin-streptomycin at 37°C in a humidified atmosphere with 5% CO₂.

The ON-TARGETplus SMARTpool siRNAs used for knockdown of the human PARG gene were purchased from Thermo Fisher Scientific Inc. (Lafayette, CO, USA). They were introduced into HeLa S3 cells with DharmaFECT Transfection reagent following the manufacturer’s protocol (Thermo Fisher Scientific). In brief, 2 μM siRNA (50 μl) were added to serum-free DMEM (50 μl) in one tube, and DharmaFECT1 (1.5 μl) was added to 98.5 μl of serum-free medium in the other tube. They were gently mixed and incubated for 5 min at room temperature, and were then combined, mixed and further incubated for 20 min at room temperature. Subsequently, complete medium (800 μl) was added and cells were cultivated with the medium in a 35-mm culture dish.

An MTS assay was performed according to the manufacturer’s instructions. In brief, mock- or siRNA-transfected cells were cultured in microtiter plate wells. MTS solution (20 μl) (Promega, Madison, WI, USA) was added to each well (containing 100 μl of cell culture) and incubated for 3 h in a 37°C, 5% CO₂-humidified incubator. Then, the absorbance at 492 nm was measured by a microtiter plate reader (Thermo Electron Corp., Vantaa, Finland) and normalized by the absorbance at 630 nm.

RT-qPCR was carried out as previously described (24). First-strand cDNAs were synthesized with ReverTra Ace (Toyobo Corp., Tokyo, Japan), random primers (Takara, Kyoto, Japan) and total RNAs were extracted from HeLa S3 cells. A primer pair to amplify the human GAPDH cDNAs was previously reported (24), and those for amplifying the PARP1 and PARG cDNAs were: hPARP1S514, 5′-GCAGAGTATGCCAAGTCCAACAG-3′ and hPARP1AS813, 5′-ATCCACCTCATCGCCTTTTC-3′; and hPARG-S, 5′-ATGTGTAAGTGGCAAAATGAAGGG-3′ and hPARG-A952, 5′-CTTCTCTGGCCTGTTCATCTTC-3′, respectively. Real-time PCR analysis was carried out using the Mx3000P Real-Time QPCR system (Stratagene, La Jolla, CA, USA) as previously described (24). For PCR amplification, cDNAs were amplified using SYBR-Green real-time PCR Master Mix (Toyobo) and 0.3 μM of each primer pair. Amplification of the PARP1 cDNA was carried out, starting with an initial step for 1 min at 94°C, followed by 42 cycles (94°C 30 sec, 55°C 30 sec and 72°C 1 min). The conditions for amplification of the PARG and GAPDH cDNAs were 1 min at 94°C, followed by 42 cycles (94°C 15 sec, 55°C 10 sec, and 72°C 15 sec).

Western blotting was carried out as previously described (24,25) with antibodies against PARP1 (Santa Cruz Biotechnology, Santa Cruz, CA, USA) and PAR (Calbiochem, Darmstadt, Germany) followed by the addition of horseradish peroxidase (HRP)-conjugated secondary antibody (Calbiochem). Signal intensities were quantified with a LAS4000 system and Multi Gauge Software (Fuji Film, Tokyo, Japan).

Luc reporter plasmids carrying 75-bp of the human PARG promoter regions were designated pKBST-Δ6 (21). The 5′-flanking regions of the human PARP1 gene were obtained by PCR with PrimeStar Taq polymerase (Takara) and the template genomic DNA from HeLa S3 cells as previously described (26). The sense and antisense primers used for PCR were: hPARP1-2660, 5′-TCGGTACCGGGTCCTCCAAAGAGCTAC-3′; and AhPARP1-2895, 5′-ATCTCGAGCCGCCACCGAACACGC CGC-3′, respectively. The amplified DNA fragments were digested with KpnI and XhoI and ligated into the MCS of the pGL4-basic (pGL4.10[luc2]), vector (Promega) to make pGL4-PARP1. Deletion derivatives, pGL4-PARP1Δ1 and pGL4-PARP1Δ2, were generated by PCR with pGL4-PARP1 as the template and primer sets: hPARP1-2851, 5′-TCGGTA CCGCCAGGCATCAGCAATCTA-3′ and AhPARP1-2895; and hPARP1-2660 and AhPARP1-2851, 5′-ATCTCGAGTA GATTGCTGATGCCTGGC-3′, respectively. The nucleotide sequences of the PCR products were determined by a DNA Sequencing system (Applied Biosystems, Foster City, CA, USA) with Rv (5′-TAGCAAAATAGGCTGTCCCC-3′) and GL (5′-CTTTATGTTTTTGGCGTCTTCC-3′) primers.

Plasmid DNAs were transfected into HeLa S3 cells by the DEAE-dextran method (24–26). After a further 24 h of incubation, cells were collected and lysed with 100 μl of 1X cell culture lysis reagent, mixed and centrifuged at 12,000 × g for 5 sec. The supernatant was stored at −80°C. The Dual Luciferase assay was performed with the Dual Luciferase assay system (Promega), as previously described (21).

In order to suppress PARG gene expression, ON-TARGETplus SMARTpool siRNAs (PARG-siRNA) were transfected into HeLa S3 cells with DharmaFECT 1 reagent. The relative amounts of PARG transcripts were reduced by PARG-siRNA treatment (Fig. 1A). In 100 nM of PARG-siRNA-treated cells, the PARG gene expression level decreased to approximately half of that in the mock-transfected cells. Since this treatment did not affect viability of cells compared with the mock-transfected cells (data not shown), further experiments were performed with 100 nM of PARG-siRNA.

As the PARG gene encodes the main poly(ADP-ribose) degrading enzyme, the level of poly(ADP-ribosyl)ated proteins was assumed to increase following the introduction of PARG-siRNA into HeLa S3 cells. Western blotting revealed that the amounts of poly(ADP-ribose) decreased in the PARG-siRNA-transfected HeLa S3 cells (Fig. 1B). In addition, the decrease of poly(ADP-ribose) in the whole-cell extracts was accompanied by a decrease in PARP1 protein levels (Fig. 1C), suggesting that the PARG-siRNA diminished poly(ADP-ribose) and the PARP1 protein.

To examine whether the decrease in PARP1 protein level is caused by changes in gene expression and promoter activity, RT-qPCR analyses and transient transfection experiments were performed. As shown in Fig. 2A, the relative PARP1 gene expression of PARG-siRNA-transfected cells was 60% that of the control (mock) cells. In addition, the transient transfection and Luc reporter assay indicated that the PARP1 promoter activity decreased in the PARG-siRNA-transfected cells compared to the control cells (Fig. 2B). We also tested whether the 75-bp core promoter of the PARG gene (21) responds to PARG-siRNA treatment (Fig. 2B, bars 5 and 6), but only a 10% decrease was observed. To limit the PARG-siRNA responsive element(s), we constructed two deletion plasmids that contained −187 to +6 and −13 to +50 bp of the human PARP1 promoter (Fig. 2C). The results showed that the 193-bp fragment, which contains the GC-box/Sp1, NF-κB/c-Rel, GATA-1 and GATA-2 binding sequences, responded to the PARG-siRNA. The promoter activity obtained from pGL4-PARP1Δ2-transfected cells was lower than that of the pGL4-basic vector-transfected cells, indicating that the 63-bp sequence from −13 to +50 is not essential for transcription of the PARP1 gene. These results suggest that the transfection of PARG-siRNA leads to suppression of PARP1 gene expression through the 193-bp sequence of the PARP1 promoter region.

It has been demonstrated that poly(ADP-ribose) metabolism is associated with cell death or apoptosis (13–15). To examine the effects of MNNG and STS on PARP1 in HeLa S3 cells, western blot analysis was performed (Fig. 3). The treatment with STS (0.1–0.3 μM) induced cleavage of PARP1, suggesting that caspases were activated and cells underwent apoptosis. Although the relative amount of PARP1 was diminished to 50%, cleaved forms of PARP1 were not detected by the treatment with 30 μM of MNNG (Fig. 3).

Subsequently, the effect of MNNG and STS on cell viability was analyzed following the transfection of PARG-siRNA. Although 40 μM of MNNG treatment caused severe damage to the cells, transfection of PARG-siRNA did not further increase cell death (Fig. 4A). On the other hand, PARG-siRNA strongly impaired cell viability when cells were treated with 0.3 and 0.4 μM of STS (Fig. 4B). These results suggest that PARG-siRNA treatment enhances cell death in conditions that cause PARP1 cleavage.