Detecting Ozone-Induced Changes in Cellular Redox Balance via GSH/GSSG-Glo™ Assay

Introduction

Epidemiological studies reveal an association between lung disease and ozone exposure. Steadily increasing levels of ambient ozone in urban areas correlate with increasing incidences of acute respiratory distress syndrome (ARDS), asthma and lung cancers, and patients with these diseases experience more serious symptoms on days with higher ambient ozone levels^{(1) (2) (3)} . Additional studies have shown that ozone exposure induces acute and chronic pulmonary inflammation, both of which are postulated to be part of the pathogenic process of chronic obstructive pulmonary diseases (COPD), ARDS, asthma and idiopathic pulmonary fibrosis (IPF)⁽⁴⁾ . The effect of environmental stressors, like ozone, on physiological responses has been outlined in whole organism studies. Ozone exposure in the lungs can cause lipid and protein peroxidation in the epithelial lining fluid and on the cell surface, increase reactive oxidative species (ROS) in the cell and induce DNA damage and cell death^{(1) (5) (6) (7)} . In addition, whole organism studies document increased production of glutathione post-ozone exposure. Upregulated expression of this antioxidant is hypothesized to minimize the harmful effects of the strong oxidant and to restore redox homeostasis^{(8) (9) (10)} . Consequently, the effect of ozonation on cellular health can be deduced by monitoring total glutathione and the ratio of glutathione in reduced (GSH) and oxidized (GSSG) forms. Whole animal studies have strengths in that the experimental system contains the variety of interactions seen in the body. However, these models can confound analysis due to the interaction of oxidants with nontarget cell types. Cell culture studies allow interactions and reactions specific to critical target cell types to be investigated more thoroughly. Type II alveolar cells are the site of gas exchange and integral to lung function, but their responses to ozonation have not been fully characterized. To model the effects of environmental oxidants on these cells in culture, we examined the effect of ozone on redox homeostasis in rat type II pneumocytes (L2 cells).

Results

L2 cells were seeded at 10⁴ cells/well, exposed for 1 hour to 3.5L/minute CO₂ + 350ppb O₃ (hazardous level of O₃ as defined by the EPA) then allowed to recover for 24 hours. As a measure of cellular health and the redox state of the cells, total glutathione and GSSG levels were determined using the GSH/GSSG-Glo™ Assay (Cat.# V6611). Changes in the levels of total glutathione detected are consistent with previous whole animal studies, suggesting that alveolar cells use glutathione to mitigate the effect of ozone exposure⁽¹¹⁾ . Our data differ from the whole animal reports in that a) only a single cell type is being analyzed under controlled conditions, b) pneumocytes, not bronchial or tracheal cells, are the focus and c) ozone exposure is within environmentally relevant levels. We found that L2 cells exposed to 350ppb O₃ had a small but statistically significant increase in total glutathione (Figure 1, Panel A; p<0.0001). Further analyses show that O₃ exposure resulted in a twofold increase in the concentration of oxidized glutathione (Figure 1, Panel B) such that the ratio of total to oxidized glutathione decreased by 50% in the presence of 350ppb ozone (Figure 1, Panel C).

Figure 1. O₃ exposure increases absolute and relative levels of glutathione and GSSG.

10⁴ cells were seeded in DMEM + 10% FBS in white-walled 96-well plates (Costar) and allowed to attach for 48 hours at 5% CO₂/air, 37°C. Ozone was generated from O₂ via Ozone Gas Generator (Pacific Ozone Technology) and diluted with 5% CO₂/air. Before exposure, medium was exchanged for HBSS, and cells were exposed to 37°C, 3.5L/minute 5% CO₂/air + 350ppb O₃ for 1 hour, then allowed to recover for 24 hours in fresh medium. Total glutathione (Panel A), GSSG levels (Panel B) and the oxidative ratio (total glutathione/GSSG; Panel C) were determined using the GSH/GSSG-Glo™ Assay with luminescence measured by the FLx800™ Multidetection Microplate Reader (BioTek). Graphs represent the mean ± S.E.M, n = 30 (Panel A: p<0.0001; Panel B: p<0.0001).

A priori, we developed two hypotheses to describe alveolar cells’ potential responses to oxidative stress. In the first, ozone exposure causes an increase in cellular antioxidants, and thus the total amount of glutathione increases. Because there is usually 100 times more GSH than GSSG in the cells, ozonation would either not affect or would cause a slight increase in the relative ratio of GSH:GSSG. The second hypothesis also relies on the GSH:GSSG ratio, stating that because there is an excess of GSH, ozone exposure does not change the absolute amount of glutathione, just the percentage in the oxidized form. Our data suggest that rat type II pneumocytes respond using a combination of the two strategies. Exposure to hazardous levels of ozone causes both a small increase (+7%) in total cytoplasmic glutathione levels and a large increase (215%) in oxidized glutathione. The significance and scale of these changes are important to note. Studies in the literature often report only total glutathione levels (and use the unfortunate shorthand of calling it GSH rather than total glutathione), which masks potentially important data about the GSH:GSSG balance. Because the GSH/GSSG-Glo™ Assay detects total and oxidized glutathione, more information is gathered from each experiment and a more complete model developed.

In ozone exposure studies, experimental conditions are achieved by exposing cells to different gas environments in different physical locations. Because of this, the different gas treatments that comprise a single experiment cannot be performed in adjacent wells of a 96-well plate. It is critical, therefore, that the biochemical analyses performed are flexible and include internal controls so that data can be compared between cells treated at different times, as well as during different runs. The GSH/GSSG-Glo™ Assay provides a straight-forward approach to examining cellular redox state that works well with this type of experimental design.

Additional advantages of the GSH/GSSG-Glo™ Assay are that all steps occur in the cell culture wells, reducing stress that might occur during scraping or trypsinization to release cells and sample loss during manipulations. The luminescent signal is proportional to the amount of glutathione within the sample and stable for 3 hours, allowing flexibility in data collection schemes. Also, unlike other assays available, all of the reagents needed to measure GSSG and total glutathione are included and the assay determines GSSG levels directly in the well, without additional deproteination steps, extractions or HLPC separation.

The rapid and simple protocol allows increased flexibility in the biochemical analyses that can be performed during a single ozone exposure setup. In fact, the GSH/GSSG-Glo™ Assay can be performed using the same cell population in parallel wells during the 1.5-hour incubation period within the ApoTox-Glo™ Assay, an assay that assesses cell viability, cytotoxicity and apoptosis events in the same cell population by measuring a protease activity specific to live cells, a protease activity that is released from cells that have lost membrane integrity and caspase-3/7 activity. This approach provides additional time savings and confidence in the data trends across biochemical assays since the cells used were all plated, exposed and processed at the same time.

Conclusion

By exposing L2 cells to 350ppb O₃ and characterizing changes using the GSH/GSSG-Glo™ Assay, we determined that type II alveolar cells' response to oxidative stress includes changes in the total amount and oxidative state of cytoplasmic glutathione. Our findings indicate that full characterization of alveolar cells’ redox homeostasis mechanisms will require attention to absolute and relative concentrations of the components involved. The GSH/GSSG-Glo™ Assay determines total and oxidized glutathione levels, is exceedingly easy to use and can be performed in cell-culture-treated 96-well plates, making it an ideal choice for experiments requiring technically difficult exposure parameters and where high-throughput or multiplexing would augment analysis.