Changes in mitochondrial stability during the progression of the Barrett’s esophagus disease sequence

Four esophageal cell lines were used; HET1A, QH, Go and OE33 cells representing the normal squamous epithelium-SIM-high grade dysplasia (HGD)-esophageal adenocarcinoma (EAC) sequence, respectively. HET1A cells were obtained from American Type Culture Collection (ATCC) (LGC Standards, Middlesex, UK), and maintained in antibiotic-free bronchial epithelial cell basal media (BEBM) enhanced with hormonal cocktail BEGM® SingleQuots®. QH and Go cells were obtained from ATCC and cultured in BEBM enhanced with BEGM® SingleQuots® and supplemented with 10 % foetal calf serum (FCS) (Lonza, MD, USA) and 1 % penicillin/streptomycin (Lonza). OE33 esophageal adenocarcinoma cells were sourced from the European Collection of Cell Cultures (Sailsbury, UK) and maintained in Roswell Park Memorial Institute (RPMI) 1640 medium (Lonza) supplemented with 10 % FCS and 1 % penicillin/streptomycin. All cell lines were maintained at 37 °C.

All research was carried out in accordance with the Declaration of Helsinki, with all patients providing informed written consent, and approval for this study was granted by the St James’s Hospital and Adelaide, Meath and National Children’s Hospital Institutional Review Board. In vivo patient samples were snap frozen in liquid nitrogen and stored at −80 °C for RMC assay experiments. Patients with histologically confirmed SIM and Barrett’s-associated EAC were recruited while in attendance of Barrett’s esophagus surveillance endoscopy or esophagectomy at the National Esophageal and Gastric Centre at St. James’s Hospital, Dublin. In-vitro, HET1A, QH, Go and OE33 cells, of similar cell passage number were grown to 70–80 % confluence in 25 cm² flasks to isolate DNA for the RMC assay. In order to examine mitochondrial instability, random mitochondrial point mutations and deletions were quantified using detailed methods previously published by our group [18]. This RMC assay allows the quantification of point mutations and deletions in the mitochondrial genome at single molecule resolution. All tissues were analyzed in a blinded fashion. All PCR products were sequenced by the High-Throughput Sequencing Facility at the University of Washington.

To further examine mitochondrial biology, ROS levels were examined in vitro. Cells were seeded in 96 well plates at density 2500 to 8000 cells/well, depending on the cell line. Seeding at different concentrations was necessary to compensate for different growth rates between different cell lines, in order to ensure the same degree of confluence at the initiation of functional experiments. Following 24 h, ROS levels were assessed. Cells were incubated with 5 μM 2, 7-dichlorofluorescein diacetate (Sigma-Aldrich) using our previously published protocols [18]. Following 40 min incubation, the ROS probe was removed, cells were analyzed using the Spectra Max Gemini System at excitation 485 nm and emission 538 nm. Mean fluorescence values for each cell line were obtained from at least three independent experiments. Crystal violet assays were performed at the same time to allow for normalization of ROS levels to cell number in each cell line. Following 24 h, the media was decanted. Cells were washed with PBS, fixed with 1 % gluteraldehyde (Sigma-Aldrich) for 20 min, 1 % gluteraldehyde was discarded and 0.1 % crystal violet solution was added for 30 min and removed by washing with water. Plates were blotted on tissue paper and allowed to air dry on the bench overnight. Once dry, the cells were resuspended in 1 % Triton X100 (Sigma-Aldrich) and incubated on a shaker for 15 min. The absorbance was read at 550 nm using a Perkin Elmer Wallac 1420 Victor2 plate reader.

Cytoglobin (CYGB), a gene linked with oxidative stress [19], was assessed in samples from patients representing the Barrett’s disease sequence; normal squamous epithelium (n = 6), SIM (n = 30), low-grade dysplasia (LGD) (n = 6), HGD (n = 12) and EAC (n = 8). Expression of this gene was used as a proxy marker for oxidative or cellular stress, with increased ROS levels associated with an increase in CYGB gene expression, in order to scavenge excess ROS [20‐22]. The purpose of this experiment was to allow us to perform an in-vivo cellular stress assessment to complement our in-vitro ROS analysis. All cases were prospectively recruited at our national referral centre. Following each biopsy for standard histological examination, a matched biopsy for RNA extraction was immediately taken directly adjacent. Matched biopsies were placed in RNAlater preservative solution (Invitrogen) and transferred to the laboratory. Normal control samples were taken from individuals attending for upper GI endoscopy with no evidence of gastro-esophageal reflux or other inflammatory aetiology. If the esophagus was macroscopically normal at endoscopy, biopsies were taken and stored as above. Only samples which demonstrated normal squamous mucosa were used in further analysis. Cancer samples were taken from individuals undergoing assessment for a new diagnosis of EAC arising in a setting of Barrett’s esophagus. All cancer cases were chemotherapy and radiotherapy naïve. All histological examination was carried out by GI pathologists. All samples were placed immediately in RNAlater at the time of endoscopy. Samples were transferred to a 4 °C fridge overnight. The following day all samples were transferred to a −20 °C freezer for storage pending the results of histological examination of matched tissues. Following histological examination of matched biopsies, samples were selected for analysis across the different histological groups.

Patient material was homogenized using a Tissue-Lyser for 5 mins at a frequency of 25 pulses per second and RNA was extracted using the Qiagen Rneasy Mini Kit (Qiagen). RNA quantity and quality was determined spectrophotometrically using a Nanodrop 1000 spectrophotometer (NanoDrop, Technologies, Wilmington, DE) and quality assessment of all samples was performed on the Agilent 2100 bioanalyzer platform (Agilent technologies, Santa Clara, CA), using the RNA Nano 6000 kit. High quality total RNA was reverse transcribed to cDNA using random hexamer oligodeoxyribonucleotides that prime mRNA for cDNA synthesis. Quantitative PCR was used to quantify cytoglobin mRNA expression (ABI Biosystems) in samples relative to the 18S ribosomal RNA endogenous control and analyzed using SDS 2.3 and SDS RQ Manager 1.2 relative quantification software. Analysis of gene expression data was performed using the 2^ΔΔCt relative quantification method using the change in the expression of a target gene relative to the expression of a reference sample in the study.

Data were analyzed with SPSS (PASW [Predictive Analytics Software] version 18) (IBM, Armonk, New York, USA) and Graph Pad Prism (Graph Pad Prism, San Diego, CA) software. Differences between HET1A, QH, Go and OE33 cell lines were calculated using unpaired Student’s t-tests and Kruskal Wallis tests. In-vitro results were reported as mean and variation was expressed as standard deviation (SD). In-vivo and ex-vivo: differences between continuous variables, for matched patient groups were calculated using Wilcoxon signed-rank tests, while in unmatched patient groups the Mann–Whitney U test was used. Patient data were reported as mean and variation was expressed as standard error of the mean (SEM = SD divided by the square root of the sample size). Statistical significance was defined as p ≤ 0.05.