L1 and HERV-W retrotransposons are hypomethylated in human ovarian carcinomas

Bulk ovarian tissue samples were surgically removed and placed in RNA later (Ambion, Austin, TX) in the operating room within 1 minute of removal from the patients. The pathological and clinical information of each sample is as follows: Sample #11 (Age 43), Adenocarcinoma (papillary serous, poorly differentiated, Stage IIc); Sample #18 (Age 34), Adenocarcinoma (endometroid, well differentiated, Stage IIb); Sample #19 (Age 57), Adenocarcinoma (papillary serous, poorly differentiated, Stage IIc); Sample #21 (Age 80), Malignant mixed mullerian; Sample #23 (Age 52), Adenocarcinoma (papillary serous, poorly differentiated, Stage IIa); Sample #29 (Age 66), Adenocarcinoma (papillary serous, poorly differentiated, Stage III); Sample #15 (Age 54), Serous borderline /low-malignancy potencial; Sample #31 (Age 40), Benign cystic masses; Sample #16 (Age 53), Normal ovary; Sample #89 (Age 53), Normal ovary. This study was approved by the Institutional Review Board of the University of Georgia and of Northside Hospital (Atlanta), from which the samples were obtained.

Genomic DNA was extracted by proteinase K digestion of 20–25 mg of bulk ovarian tissue and phenol-chlorophorm extraction. DNA was ethanol precipitated and re-suspended in water. Ten micrograms of genomic DNA were digested overnight at 37°C with 10 to 16 excess amount of either HpaII [methylation sensitive restriction enzyme] or MspI [not sensitive for methylation at internal cytosine]. These enzymes recognize the sequence CCGG, which is found in diverse positions in the promoter regions of these retroelements. Digested DNA was resolved on an agarose gel and transferred to a nylon membrane (Hybond N; Amersham-Biosciences, Piscataway, NJ) with NaOH. Membranes were prehybridized for 1 hour with 10 mg/ml of herring sperm DNA in Church buffer [0.5 M NaH₂PO₄, 7% SDS and 10 M EDTA] and hybridized overnight at 65°C in the same buffer with 100–200 ng of probe DNA labeled with [α-³²P]dCTP using a Nick Translation Kit (Roche, Indianapolis, IN). Filters were washed twice for 15 min in 2 × SSC and 0.1% SDS and then twice for 30 min in 1 × SSC and 0.1% SDS at 65°C and exposed to Phosphorimager screens (Molecular Dynamics, Sunnyvale, CA).

The HERV-W probe was designed in the LTR region, downstream of the putative TTAAAT box. PCR was performed on genomic DNA with forward primer HERVF 5'-CCACCACTGCTGTTTGCCAC-3 ' and reverse primer HERVR 5 '-GCCTCGTGTTCTCTGACCTGGGG-3', producing a 304 bp fragment. The LINE1 probe for the promoter region was designed according to Takai et al [18]. PCR was performed on genomic DNA with forward primer L1F 5'-CGGGTGATTTCTGCATTTCC-3' and reverse primer L1R 5'-GACATTTAAGTCTGCAGAGG-3', giving a product of 540 bp. PCR products were cloned into pCR2.1-TOPO and transformed into TOP10 E. coli cells (Invitrogen, Carlsbad, CA). Plasmids were extracted (Qiaprep Spin Miniprep Kit, Qiagen, Valencia, CA) and sequenced. Subsequent PCR reactions were performed on cloned plasmid DNA for both HERV-W and LINE1, and gel extracted PCR products were used as hybridization probes.

Total RNA was extracted using Trizol Reagent (Invitrogen, Carlsbad, CA) and 2–5 μg of total RNA were reverse transcribed into first-strand cDNA using the Thermoscript RT-PCR system (Invitrogen, Carlsbad, CA) in a final volume of 20 μl. The HERV-W primers used were: forward; 5'-TTGGCGGTATCACAACCTCT-3' reverse; 5'-GTGACGATTCCGGATTGA-3'; (product size:230 bp) based on the HERV-W sequence (GeneBank accession no. AC000064). The LINE-1 primers were: forward 5'-TCATAAAGCAAGTCCTCAGTGACC-3'; reverse 5 '-GGGGTGGAGAGTTCTGTAGATGTC-3' (product size:165 bp) based on the LINE-1 sequence (GeneBank accession no. M80343). Real-time monitoring of PCR reactions was performed using the DNA Engine Opticon 2 System (MJ Research, Waltham, MA) and the SYBR Green iQ dye (BioRad, Hercules, CA) [24]. For each reaction, the amount of a target and of an endogenous control (R ibosomal P rotein S27A) were determined using a calibration curve and the amount of target molecule was divided by the amount of endogenous reference to obtain a normalized target value [25]. RPS27A has been previously identified as a valid control gene in expression studies conducted among human malignant and control tissues [26]. In addition, we independently verified by microarray analyses that RPS27A expression levels are constant among the samples examined in this study (data not shown). Separate calibration (standard) curves for RPS27A, HERV-W and LINE-1 were constructed using serial dilutions of total cDNA from normal human ovarian tissue (purchased from Ambion, Austin, TX). Standards for HERV-W, LINE-1 and RPS27A were defined to contain an arbitrary starting concentration, and serial dilutions were used to construct the standard curve. Standard curve calibrations were included in each assay.