Abstract
Background/Aim: To determine whether Gramicidin S (GS)-nitroxide, JP4-039, esophageal radiation protection protected lung tumors in a transgenic model, LoxP-Stoop-LoxP Kristen Rat Sarcoma Viral oncogene (LSL-K-RAS) mice were administered intra-tracheal- Carbapenem-resistant Enterobacteriaceae (CRE) recombinase, bilateral lung tumors were confirmed at 11 weeks, then thoracic irradiation was delivered. Materials and Methods: Mice received single-fraction 15 Gy or 24 Gy to both lungs, in subgroups receiving intraesophageal administration 10 min before irradiation of JP4-039 (in F15 emulsion) tumor size reduction and survival were investigated. Mice were followed for survival, and reduction in tumor size. Results: There was no evidence of tumor radioprotection in mice receiving JP4-039/F15. Conclusion: Intraesophageal radioprotective small-molecule antioxidant therapy protects normal tissue but not tumor tissue in mice with transgenic lung tumors.
A major complication of clinical radiotherapy of lung cancer is damage to normal tissues in the surrounding target volume. In particular, radiotherapy of non-small cell lung carcinoma is associated with significant esophagitis, which may be dose-limiting, and can result in esophageal stricture in survivors. Animal models of lung cancer have facilitated the search for new radioprotector drugs (1-5). Local administration of both manganese superoxide dismutase-plasmid liposome (MnSOD-PL) gene therapy (6-28) and the small molecule GS-nitroxide conjugate JP4-039 (29-33) has been demonstrated to selectively protect the esophagus with no significant tumor radioprotection in orthotopic tumor models (16, 18, 20, 34). Intraesophageal administration of MnSOD-PL in mice with orthotopic Lewis lung carcinomas at the carina has been shown to reduce irradiation-induced esophagitis with no significant reduction in survival due to increase in tumor size (20, 34). In other experiments, single or multiple administrations of MnSOD-PL to the oral cavity during head and neck irradiation of mice with orthotopic squamous cell carcinoma in the floor of the mouth demonstrated no significant tumor radioprotection (16, 35). Recently, a small molecule GS-nitroxide has been reported to provide significant local tissue radioprotection when administered in a novel F15 lipid emulsion (32). Fluorochrome-labeled JP4-039-BODIPY has been demonstrated to target mitochondria of cells in vitro (4), supporting its proposed mechanism of action (33).
In the present studies, we tested the effect of intraesophageal administration of JP4-039/F15 in a model of transgenic lung carcinoma. LSL-K-RAS mice were administered intraesophageal CRE-recombinase, which has been shown to induce multi-focal bilateral lung tumors in the subsequent 11-15 weeks (36). Mice with established bilateral tumors received single-fraction whole-lung irradiation with the goal of providing tumor size reduction and long-term local control. In subgroups of mice that received intraesophageal administration of JP4-039/F15, we compared tumor size reduction by irradiation and survival. We sought to determine whether the known esophageal radioprotection mediated by JP4-039 (32) would also provide tumor radioprotection, and lead to more rapid death from faster tumor growth.
Materials and Methods
LSL-K-RAS transgenic tumor model. LSL-K-RAS mice and control LSL mice (3, 37-40) were obtained from McGarry Houghton (36) and housed four per cage according to the University of Pittsburgh Institutional Animal Care and Use Committee (IACUC) regulations. Mice were fed standard laboratory chow. At ages of six to eight weeks, male and female mice were administered intratracheal CRE-recombinase according to published methods (36). Mice were followed for 11-14 weeks and at serial time points, representative animals were examined for the appearance of bilateral lung tumors. At the time when lung tumors of measurable size in all mice were detected, subgroups of 8 mice were randomized to receive radioprotective esophageal therapy prior to whole-lung irradiation.
Administration of JP4-039 in F15 emulsion. The GS-nitroxide conjugate, JP4-039 (33), in F15 liposome emulsion (100 μl containing 400 μg drug/mouse) was administered orally prior to irradiation as published elsewhere (32).
Mouse lung irradiation. Adult mice with bilateral CRE-recombinase-induced tumors, received single fraction 15 Gy or 24 Gy total-lung irradiation according to published methods (7). The head, neck, and lower body were shielded so that only the lung received irradiation (32). Mice were treated on a 6 MV linear accelerator (Varian Corporation, Palo Alto, CA, USA) according to published methods (32). Mice were followed-up for survival. When animals became moribund or lethargic, they were sacrificed.
Lung histopathology and evaluation of tumor size. Mice dying of extension of lung cancer, radiation-associated morbidity, or at the end of the experiment at day 110 were sacrificed. The lungs were expanded with Optimal Cutting Temperature (OCT), excised, frozen, sectioned and hematoxylin and eosin (H&E)-stained lung sections were examined for the percentage of lung containing tumor. Histopathological evaluation of both lungs was carried out in serial sections from each animal. Ten sections of each lung were analyzed and the percentage of lung replaced by tumor was calculated. Histopathological findings of acute or late radiation toxicity in the lungs were documented as published (34).
Statistics. Kaplan–Meier survival curves were plotted for each of the four treatment groups (namely, unirradiated control group; 19 Gy upper body irradiation only; F15 intraesophageal administration prior to irradiation; and intraesophageal JP4-039/F15 prior to irradiation). Comparison between any two groups was carried with the two-sided log-rank test. In the tumor growth study, sections of each lung were analyzed descriptively, where the percentage of lung replaced by tumor was calculated.
Results
CRE-recombinase induced bilateral lung cancers in LSL-K-RAS mice. Mice treated with CRE-recombinase intra-nasal injection as described in the methods and as published elsewhere (36) were followed for 11-17 weeks and at serial times examined for the presence of bilateral lung cancer. Figure 1A shows the histological appearance of representative bilateral lung tumors in mice receiving intra-nasal CRE-recombinase. Lung tumors were evaluated histopathologically and diagnosed as either adenomas or squamous cell carcinomas. These results confirm and extend those of previous publications using the CRE-recombinase model for induction of bilateral transgenic lung cancer (3, 36-40).
Intraesophageal absorption of JP4-039/F15 provides esophageal radiation protection with no detectable tumor protection. Mice receiving intraesophageal JP4-039/F15 were irradiated to 15 Gy to the thoracic cavity. One group of control mice received 15 Gy irradiation with no prior JP4-039/F15. Another control group received F15-alone intraesophageal administration with no irradiation. As shown in Figure 1B at seven days after 15 Gy thoracic irradiation, tumor size was reduced by irradiation with no tumor protective effects (size increase) by JP4-039/F15.
In a second experiment, we observed mice for 110 days. As shown in Figure 2, a higher lung irradiation dose of 24 Gy resulted in a longer survival of mice to 50 days. There were no early deaths. Subgroups of animals receiving intraesophageal F15 emulsion alone prior to 24 Gy showed no deaths until 60 days. Those receiving JP4-039/F15 prior to irradiation showed no deaths until 50 days. The results demonstrated no significant decrease in survival in mice receiving intraesophageal radioprotective JP4-039/F15.
The survival curve of mice with lung tumors not receiving irradiation demonstrated no late deaths from lung cancer after day 10, suggesting tumor regression in a sub-population of tumor-bearing mice (Figure 2).
Histological evidence of spontaneous tumor regression in mice surviving beyond 10 days. Surviving LSL-K-RAS mice that had been injected with CRE-recombinase were analyzed at day 110 for histopathological evaluation of lung tissue. Mice dying at earlier time points were also analyzed. The gross appearance of the lungs from five representative mice at 110 days showed no evidence of tumor (Figure 3). Two sections from each of the representative mice are shown in Figure 3. Two mice (Figure 3 A and B) showed normal lung architecture, while others (Figure 3 C and E) showed some peri-alveolar bronchial infiltrates of inflammatory cells. H&E-stained frozen sections were examined for evidence of tumor (adenoma or adenocarcinomas). No tumors were observed in any of 690 lung sections examined in all dying mice or those sacrificed after day 10. All observed lesions of inflammatory infiltrates were within normal limits for LSL mice at 110 days of age. Inflammatory foci (infiltrates) were observed around some airways (Figure 3 C-E) and vessels were considered normal and unrelated to any tumor or disease.
The survival of non-irradiated control tumor-bearing mice beyond 10 days after detection of bilateral lung tumors suggested spontaneous resolution of these CRE-recombinase-induced lung cancers. Histopathological evaluation was carried-out in mice in all groups. There were no differences in lung morphology detected in the JP4-039/F15- or F15-treated groups when compared to the irradiated control group.
Discussion
The present results confirm and extend prior reports demonstrating the effect of esophageal radioprotection by swallowed JP4-039/F15 (32), now in another (LSL) mouse strain. In previous studies, C57BL/6NHsd mice received total-lung irradiation preceded by intraesophageal JP4-039/F15. There was a significant decrease in irradiation-induced esophagitis with higher doses of irradiation using JP4-039/F15 and decrease in early death with no significant morbidity of other tissues. Furthermore, there was no evidence of drug uptake in organs outside the oral cavity/esophagus, confirming and extending other publications demonstrating the safety of a local administration of radioprotective GS-nitroxide conjugates (32).
A new finding of the present experiments was the long-term survival of 70% of control non-irradiated mice with bilateral CRE-recombinase-induced tumors. Prior publications indicated that some of the tumors in CRE-recombinase-treated mice are not squamous cell carcinomas, but represent adenomas or benign lung tumors (3, 37-41). In the present studies, careful histological evaluation of lungs in long-term surviving mice demonstrated no evidence of tumors, not only in irradiated or JP4-039/F15 treated then irradiated groups, but also in control unirradiated groups. These results are consistent with the interpretation that some bilateral lung tumors in LSL-K-RAS, CRE-recombinase induced K-RAS transgenic mice are benign tumors and not associated with progression, invasion, or metastasis. The results suggest caution in using this CRE-recombinase-induced transgenic lung cancer model for studies of the therapy of aggressive rather than limited-stage lung cancers and suggest the need for use of another model, which includes a mutant p53 allele (41).
There has been controversy over the use of orthotopic tumors in mice for cancer therapy experiments rather than mice with transgenic cancer. Orthotopic tumor models have been criticized as unrealistic and not representative of true lung cancer in that they have been established by transplantation of documented tumor cell lines, including those removed from chemical carcinogen- or virally-induced established lung cancer (16, 18, 20, 34). In particular, the Lewis lung carcinoma model, which has been a mainstay of orthotopic tumor experiments for lung cancer, has been shown to produce locally invasive and metastatic lung cancer (34), but suffers as a model system as it is not representative of spontaneous lung cancer. Other models of orthotopic head and neck cancer have also been utilized for studies of normal tissue radioprotection (16), and similar criticism has been levied at the use of orthotopic squamous cell transplantation of established tumor cell lines in the floor of the mouth as a representative model system for head and neck cancer.
An alternative to the use of orthotopic tumor models is the transgenic tumor model. The LSL-K-RAS and C57BL/6-K-RAS models have been used as being representative of spontaneous true transgenic tumors and have been suggested as being more valuable (36), reproducible, and efficient for studies of tumor biology. Several transgenic models of lung carcinoma have included the hepatocyte growth factor (HGF) transgenic model (40) or spontaneous lung tumors arising in specific mouse strains.
In the present studies, we tested the LSL-K-RAS model as a system in which to document the effectiveness of radioprotective small-molecule therapy for the esophagus in a setting of true spontaneous tumors. The present results demonstrate the reproducible induction of bilateral transgenic lung tumors in LSL-K-RAS mice treated with intratracheal CRE-recombinase. However, 70% of these tumors spontaneously regressed in non-irradiated, non-drug-treated mice in the control group. Upon histopathological examination, no lung carcinomas were detected 110 days past the time-point when tumors were originally induced. In contrast, in orthotopic tumor-bearing mice, all would have died from progressive or metastatic cancer by this time point (16, 18, 20, 34). Further studies are required to identify an appropriate transgenic mouse model for high frequency detectable and reproducibly fatal lung carcinomas.
At present, orthotopic tumor models of localized yet progressive and fatal lung cancer may be more appropriate for evaluating the safety of intraesophageal radioprotective therapies in a setting in which all control non-irradiated mice would be expected to die of progressive lung cancer.
Acknowledgements
This manuscript is supported by the following grants: NIH R01-CA119927-11 and NIH/NIAID 1U19A168021-06. This project used the UPCI animal facility that is supported in part by award P30CA047904.
- Received January 17, 2014.
- Revision received February 27, 2014.
- Accepted March 4, 2014.
- Copyright © 2014 International Institute of Anticancer Research (Dr. John G. Delinassios), All rights reserved