Previous studies indicate that the inhibition of ERβ may have anti-tumoral potential against different malignant neoplasms [12], [15], [16], [17] including Medulloblastomas [8]. To further analyze this possibility, we have selected human medulloblastoma cell lines, Daoy, D283Med and D384Med, which express high levels of ERβ in the absence of ERα [9], and asked if the effectiveness of cisplatin treatment could be enhanced by the ER antagonist, ICI182,780 [18], [19]. Surprisingly, our initial morphological evaluation, depicted in Fig. 1A, show only limited nuclear damage (typical for cisplatin treatment; arrowhead), which was accompanied by mitotic figures (asterix), when the cultures of Daoy cells were exposed to cisplatin (1 µg/ml) in the presence of 10 µM ICI182,780. Further analyses based on cell membrane permeability (ViaCount) and apoptotic DNA damage (TUNEL) confirmed ICI182,780-mediate protection of Daoy cells from the cisplatin induced cytotoxicity (Fig. 1B). Quantitatively, an average cell viability increased from 47.8+/−8.4% to 67.9+/−5.1% when the cell were exposed to cisplatin or to cisplatin+ICI182,780, respectively (45% increase in cell survival). In the same culture conditions, the percentage of apoptotic cells (TUNEL positive) decreased from 15.4+/−2.1% in the presence of cisplatin to 5.5+/−0.6% in the presence of cisplatin+ICI182,780 (Fig. 1B, lower panel). In addition, results in Fig. 2A demonstrate that ICI182,780 used at concentrations ranging from 10 nM to 10 µM protected Daoy cells from cisplatin-induced cell death. In a similar manner, siRNA against ERβ counteracted cisplatin-induced cytotoxicity (last bar in Fig. 2A), further indicating that ERβ is involved in ICI182,780-mediated cell protection from cisplatin. Another two human medulloblastoma cell lines, D384Med and D283Med, tested in the same condition showed 44.3% (significant) and 21.1% (not significant) increase in cell viability, respectively (Fig. 2B). A similar trend in cell survival was also observed in two breast cancer cell lines BT20 and MCF7, which are both known to express ERβ [20]. However, effects of ICI182,780 counteracting cisplatin-induced cytotoxicity was less pronounced, most likely because these two breast-cancer cell lines are significantly less sensitive to the cisplatin treatment (Fig. 2B). Interestingly, we did not observed any major effects of ICI182,780 on cell survival when tested, in the absence of cisplatin, in exponentially growing Daoy cells (10%FBS) at concentrations ranging from 10 nM to 100 µM (Fig. 2C).

The analysis of cell cycle distribution demonstrated a gradual shift from G2/M arrest, which usually happens in cisplatin-treated cells [21], to G1 arrest when the cells treated with cisplatin were cultured in the presence of ICI182,780 (ICI; Fig. 3A). This transition in cisplatin-induced cell cycle arrest is already visible at 24 hours (not shown), and became much more apparent at 48 hours time point in which G2/M fraction decreased from 47.1% (cisplatin only) to 30.2% (cisplatin+ICI) and G1 fraction increased from 24.2% (cisplatin only) to 39.7% (cisplatin+ICI). Importantly, the continuous cell exposure to cisplatin and ICI182,780 for 72 hours resulted in two-fold lower level of SubG1 fraction, which represents the population of necrotic and apoptotic cells (decrease from 13.8% in cisplatin to 5.7% in cisplatin+ICI; Fig. 3A, lower panel). We have repeated evaluation of cell cycle distribution in Daoy, D384Med and in D283Med cells several times and the average data are presented in Fig. 3B. Again, all cell lines examined show an apparent shift from G2/M to G1 cell cycle arrest when the cisplatin treatment is accompanied by ICI182,780-mediated inhibition of ERβ.

If indeed this transition in cell cycle distribution is based on DNA damage/cell cycle checkpoint system, we should observe also a shift in the phosphorylation pattern between ATM/Chk2 and ATR/Chk1 [22]. Of note, the cisplatin treatment is expected to trigger G2/M arrest followed by elevated apoptosis [23]. The results in Fig. 4 demonstrate very low levels of phosphorylation of ATM, ATR, Chk1 and Chk2 in the absence of DNA damage (FBS and ICI). Following the treatment with cisplatin (Cis), over 4-fold increase in ATM/Chk2 phosphorylation and 1.4-fold increase of ATR/Chk1 phosphorylation were observed after 6 hours. The phosphorylation pattern between ATM/Chk2 and ATR/Chk1 was reversed when the cisplatin treated cells were compared to the cells treated with cisplatin + ICI182,780. Quantitatively, ATM/Chk2 phosphorylations decreased by an average of 2-fold and ATR/Chk1 phosphorylations increased by an average of 1.5-fold (Fig. 4B). These results demonstrate that the transition from G2/M to G1 arrest observed in the presence of ICI182,780 was indeed accompanied by the transition from ATM/Chk2 to ATR/Chk1 activation.

Since cellular responses to cisplatin and ICI182,780 are similar in all cell lines examined, we have selected Daoy cells to explore molecular basis of ICI182,780–induced resistance to cisplatin. In addition, effects of cisplatin and ICI182,780 were evaluated in cells replicating DNA (10%FBS), therefore the cisplatin treatment which primarily generates DNA-adducts and oxidative DNA damage [24], [25], [26] is also expected to cause DNA double strand breaks (DSBs) [27], [28], [29]. This happens when the replication forks are stalled on the cisplatin-induced primary DNA lesions [29], [30], [31]. We have used neutral comet assay to evaluate DSBs formation in Daoy cells treated with cisplatin [32]. The results in Fig. 5 show the average comet tail moment of 1.6+/−0.2 in control Daoy cells cultured in the presence of 10% FBS (FBS). The treatment with ICI182,780 (ICI) slightly increased this parameter to 1.9+/−0.5 (not significant). The average tail moment increased almost 4-fold (from 1.6+/−0.2 to 6.3+/−2) following cell exposure to 1 µg/ml of cisplatin (Cis). Importantly, a significant (*) 2.4-fold decrease in the tail moment (from 6.3+/−0.2 to 2.6+/−0.4) was observed when the Daoy cells were treated with cisplatin in the presence of ICI182,780 (Cis+ICI). This 2.4-fold decrease in the comet tail moment in the presence of ICI182,780 may suggest that either cisplatin generates less DNA damage, or that cisplatin-treated cells repair DSBs more effectively following the inhibition of ERβ. To address this question, we have utilized siRNA strategy against Rad51 – the major DNA repair protein involved in DSBs DNA repair during S-phase of the cell cycle [29], [33], [34]. The comparison between last two bars in Fig. 5 demonstrates that ICI182,780 is not able to rescue Rad51-deficient Daoy cells from cisplatin; note a significant increase (**) in comet tail moment from 2.6+/−0.4 to 4.5+/−0.6 (Fig. 5). Additionally, results in Fig. 6 show detectable changes in the phosphorylation pattern of histone H2AX (γH2AX - DNA damage response protein, which becomes phosphorylated within mega-basepare regions surrounding DNA strand breaks [28]). The number of γH2AX nuclear foci is relatively small in untreated exponentially growing Daoy cells (FBS), which increased dramatically in the presence of cisplatin (Fig. 6A; compare FBS and Cis). Despite of an apparent decrease in the DNA damage evaluated by the neutral comet assay (Fig. 5), the cells treated with cisplatin in the presence of ICI182780 (Cis+ICI) show an increase in γH2AX nuclear foci (evaluated by γH2AX/DAPI co-localization), which may imply more effective recruitment of DNA repair proteins, including Rad51 [35]. Of note, we have previously reported that ICI182,780–mediated inhibition of ERβ prevented translocation of IRS-1 to the nucleus and the binding between IRS-1 and Rad51 after DNA damage [9]. Indeed, results in Fig. 6A (lower panel) confirmed that only a small fraction of nuclear IRS-1 was detected in Daoy cells treated together with cisplatin and ICI182,780, which according to our previous observation is expected to increase the fraction of Rad51, which in the absence of nuclear IRS-1 can be recruited more effectively to the sites of DSBs, supporting HRR [9], [36]. The results in Fig. 6B show that cells in which cisplatin-induced DNA damage was accompanied by ICI182,780 treatment have significantly greater areas in which Rad51 co-localizes with the sites of DNA labeled by BrdU (de novo DNA replication). Quantitatively, the number of cells, in which 10 or more Rad51 nuclear foci co-localized with BrdU, increased almost 40% in the presence of ICI182,780 (Fig. 6B, histogram).

To evaluate if this significantly higher level of Rad51/BrdU co-localization correlates with increased HRR activity, we used previously generated in our lab Daoy/DRGFP cells [9], which stably express the HRR reporter cassette (DRGFP) [37]. Results in Fig. 7A demonstrate over 20-fold difference in HRR when the cisplatin treated Daoy/DRGFP cells were compared to Daoy/DRGFP cultured in the presence of cisplatin+ICI182,780. In particular, we have detected an average of 21+/−4 cells capable of repairing the DRGFP reporter cassette per 10,000 cells (n = 3); when the cisplatin treatment was accompanied by ICI182,780. In the absence of ICI182,780, we have detected only 1+/−1 cells capable of reconstituting the DRGFP per 10,000 cells (n = 3) (Fig. 7A; left panel). Note that in the absence of cisplatin (DRGFP control) the average level of HRR–mediated reconstitution of the functional GFP is about 3% in exponentially growing Daoy cells (10%FBS), which increased up to 5% in 10%FBS+ICI182,780 (Fig. 7A right panel, and [9]). Importantly, this ICI182,780-induced increase in HRR in cells treated with cisplatin correlated well with increased clonogenic growth of Daoy cells evaluated after the removal of cisplatin (Fig. 7B). In this experiment, we have used cisplatin at lower concentration (0.25 µg/ml) and analyzed its effects in the presence and absence of 10 µM ICI182,780. Following 24 hours, the cisplatin-containing culture medium was removed and the cells were re-pleated at 1,000; 3,000; and 10,000 cells/35 mm dish. The clonogenic growth was measured after 2 weeks of the continuous cell growth in the presence of 10%FBS. The results in Fig. 7B show that 24 hours of cell exposure to 0.25 µg/ml of cisplatin inhibited almost completely their future clonogenic growth. In contrast, Daoy cells treated with cisplatin in the presence of ICI182,780 formed an average of 10+/−3, 22+/−5 and 72+/−8 clones when plated at 1,000; 3,000; and 10,000 cells, respectively. Interestingly, in the absence of cisplatin, clonogenic growth of Daoy cells was significantly attenuated in cultures exposed to 10 µM ICI182,780 (Fig. 7C).

We have used three human medulloblastoma cell lines, Daoy, D384Med and D283Med. Daoy derive from a tumor in the posterior fossa of a 4 years-old boy (ATCC# HTB186), D283Med (ATCC#HTB-185), and D384Med [49] are metastatic medulloblastomas isolated from peritoneal ascites of children diagnosed with medulloblastoma. Daoy were maintained as monolayer cultures in Dulbecco's Modified Eagle Medium (DMEM) (GIBCO-BRL, Grand Island, NY) containing 10% fetal bovine serum (FBS), at 37°C in a 7% CO₂ atmosphere. D283Med and D384Med were cultured in suspension in DMEM supplemented with non-essential amino acids (GIBCO-BRL, Grand Island, NY), 2 mM L-glutamine, 1 mM sodium pyruvate, and 10% FBS. We have used MCF7 (ATCC# HTB-22) and BT-20 (ATCC# HTB-19) human breast cancer cell lines as a reference point in the experiment depicted in Fig. 2B. Exponentially growing cells were treated with cisplatain at 0.25 and 1.0 µg/ml in the presence or absence of ERβ antagonist, ICI182,780 (10 nM-100 µM; Tocris Bioscience, Ellisville, Mo) [9]. In some experiments, expression of Rad51 and ERβ was inhibited by utilizing ON-TARGETplus SMARTpool siRNA against human Rad51 - target sequences: CCAACGAUGUAAGAAUU; GCAGUGAUGUCCUGGAUAA; CUAAUCAGGUGGUAGCUCA; UAUCAUCGCCCAUGCAUCA (100 nM, Thermo Scientific); and human ERβ - target sequences: GGAAAUGCGUAGAAGGAAU; UUCAAUUUCGAGAGUUA; GCACGGCUCCAUAUACAUA; GAACCCACAGUCUCAGUGA (200 nM; Thermo Scientific) delivered to the cells by Oligofectamine transfection reagent (Invitrogen).

We have used GUAVA easyCyte 8HT and Calibur flow cytometers to detect and quantify these three cellular parameters. Briefly, the aliquots of 1×10⁶ cells/ml were fixed in 70% ethanol at −20°C, overnight. The cells were centrifuged at 1,600 rpm and the resulting pellets suspended in 1 ml of freshly prepared Propidium Iodide/RNaseA solution. Cell cycle distribution was evaluated using specialized software CellCycle included in GuavaSoft 1.1. In some experiments DNA replication was evaluated by BrdU pulse labeling (1 hour) using the DNA replication Assay (Millipore). Finally, cell death and cell survival were evaluated by two independent assay, TUNEL assay (Roche), which detects DNA damage associated with apoptosis, and cell membrane integrity by using ViaCount reagents, according to the manufacturer recommendations. Guava/Express plus and Guava/ViaCount software were used for data analyses.

Was utilized to detect DNA strand breaks in exponentially growing Daoy cells exposed to cisplatin in the presence and absence of ICI182,780. The cells treated with H2O2 (oxidative DNA damage) or neocarzinostatin (NCS; Sigma, Saint Louis, MO) were used as positive controls for the detection of secondary and primary DNA strand breaks (DSBs), respectively. The cells were subjected to single cell electrophoresis in neutral conditions [32] by utilizing SYBR green based kit from Trevigen and Automated Comet Assay System from Loats Associates Inc. The tail moment was calculated from 100 cells collected per single measurement by utilizing specialized comet software included in the Automated Comet Assay System (Loats Associates Inc., Westminster, MD).

To isolate protein extracts, monolayer cultures were treated with 400 µl of lysis buffer A [50 mM HEPES; pH 7.5; 150 mM NaCl; 1.5 mM MgCl₂; 1 mM EGTA; 10%glycerol; 1% TritonX-100; 1 mM phenylmethylsulfonyl fluoride (PMSF); 0.2 mM Na-orthovanadate and proteinase inhibitor cocktail] on ice for 5 minutes. Total proteins (50 µg) were separated on a 4–15% gradient SDS-PAGE (BioRad). The resulting blots were probed with following primary antibodies: anti-pSer1981 ATM mouse monoclonal antibody (Cell Signaling Technology Inc., Danvers, MA); anti-pSer428 ATR rabbit polyclonal antibody (Cell Signaling Inc.); anti-pSer317 Chk1 rabbit polyclonal (Cell Signaling Inc.), anti-pThr68 Chk2 rabbit polyclonal (Cell Signaling Inc.). Anti-Grb-2 antibody (Transduction Laboratories, Lexington, KY), was used to monitor equal loading conditions [33].