Air Force Research Laboratory, Directed Energy Bioeffects Division, Brooks AFB, TX, 78235,
1 US Army Institute of Surgical Research, Fort Sam Houston, TX, 78234,
2 Veridian Engineering Inc., San Antonio, TX, 78216,
3 Department of Carcinogenesis, University of Texas M.D. Anderson Cancer Center, Science Park, Smithville, TX 78957 and
4 Department of Biology, Trinity University, San Antonio, TX, 78212, USA
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Abstract |
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Abbreviations: ANOVA, analysis of variance; BrdUrd, 5-bromodeoxyuridine; DMBA, dimethylbenz[a]anthracene; ID, interior diameter; IR, infra-red; MMW, millimeter wavelength; ODC, ornithine decarboxylase; PBS, phosphate-buffered saline; RFR, radio frequency radiation; TPA, 12-O-tetradecanoylphorbol-13-acetate.
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Introduction |
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As stated above, only three studies have investigated carcinogenic effects of RFR in models of skin cancer. In two of these studies (performed in the same laboratory), exposure to 2450 MHz RFR, either prior to or during initiation and promotion with 3,4-benzopyrene, accelerated the development of skin cancer and, consequently, decreased animal survival time (9,19). It was also noted, however, that the same acceleration of skin cancer development and reduction in survival occurred in animals exposed to chronic confinement stress in the absence of RFR exposure, suggesting that the hypothesized RFR effect could possibly be due to a non-specific stress reaction (9). In the third study, chronic exposure to 2450 MHz RFR did not alter tumor development in a mouse model of melanoma (18).
Recently, hardware systems capable of generating RFR of millimeter wavelength (MMW) (30300 GHz) have been developed and are increasingly being used for a number of applications, such as satellite communications, military radar, non-lethal weapons, high speed data communications, automotive anti-collision devices, weapons detection and medical devices. To date, no study has investigated possible carcinogenic effects of MMW frequencies. The depth of penetration of 94 GHz RFR has been calculated to be ~0.3 mm (2124), suggesting that all of the MMW energy absorption in animals and humans will occur in the skin. It is therefore most likely that, if any long-term carcinogenic effects exist, they would be observed in the skin. If such effects exist, it is also probable that MMW exposure would promote rather than initiate carcinogenesis. Hence, the goal of this study was to determine whether a single or repeated exposure to 94 GHz RFR serves as either a promoter or a co-promoter in the development of skin cancer.
To investigate this question, we used a two-stage model of carcinogenesis that utilizes SENCAR mice initiated with dimethylbenz[a]anthracene (DMBA) and promoted by repetitive application of 12-O-tetradecanoylphorbol 13-acetate (TPA) to elicit skin papillomas (25). A papilloma is a benign epithelial neoplasm consisting of villous or arborescent outgrowths of fibrovascular stroma covered by neoplastic cells; although benign, papillomas are premalignant lesions that will progress to malignant squamous cell carcinomas with extended observation times (25,26). The SENCAR mouse model has been extensively used to study carcinogenic effects of 60 Hz magnetic fields (2732) and is therefore an established model for the study of potential effects of non-ionizing radiation on skin carcinogenesis.
Because MMW exposure at the levels investigated herein produce hyperthermia, it was necessary to delineate whether any effects noted were specific to MMW exposure or if they were simply a result of the hyperthermia attendant on MMW exposure. In order to examine this question, the biological effect of MMW exposure was compared with comparable thermal levels of infra-red (IR) exposure, which has a penetration depth similar to that of 94 GHz RFR (21,23). Conflicting reports appear in the literature, suggesting that hyperthermia treatment (via a water bath) can either serve as an anti-promoter (33,34) or as a promoter (35), depending on the treatment regimen.
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Materials and methods |
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Animal housing facility
Each room in the animal housing facility was equipped with independent temperature, humidity, ventilation and light controls. Room temperature was maintained at 24 ± 1°C, with relative humidity at 50 ± 5%. Air flow rate was constant at 18 exchanges/h. A time controlled lighting system provided a 12 h light/12 h dark cycle (lights on at 0600). During most of the experiments the illumination level was no greater than 279.86 lux at any cage level. During the initiation phase of each experiment (see below) `light covers' were utilized to allow an illumination level of no greater than 161.46 lux at any cage level and 43.06 lux at 1.0 m above the floor. Throughout all experiments the location of each animal cage on the racks was systematically changed weekly to ensure that the environmental conditions, including illumination levels, were similar for all mice. The experimental rooms (used for chemical application and MMW/IR exposures) were adjacent to the animal housing facility to minimize stress and environmental contamination during transport of the animals.
Animal husbandry
Animals were housed in groups of up to 7 per cage in Plexiglas cages (41x21x20 cm) with stainless steel wire covers and were allowed ad libitum access to food and water. The mice were provided with Lab Diet 5015 mouse diet (PMI International, Brentwood, MO) that contained only 4.5% of its calories as fat. Corncob bedding (1/8 inch; Green Pet Products, Conrad, IA) was used throughout each study and clean cages and fresh water were supplied to the animals twice a week. During the experimental period all animals were visually inspected twice daily (MondayFriday); once between 0730 and 0830 and again between 1530 and 1630. On weekends animals were inspected once daily.
Papilloma initiation
At 7 weeks of age all animals were anesthetized with Metofane (methoxyflurane, catalog no. 55685; Pitman-Moore, Mundelein, IL), permanently marked for identification using a toe clip method (36) and the dorsoscapular region of the back (~2.5x4 cm) was shaved using multiple electric shavers to avoid overheating of the skin. On the following day mice were examined and excluded from the experimental groups (see below) if: (i) dermal abrasions, nicks or cuts occurred during shaving; (ii) general health or skin problems were evident; (iii) hair re-growth occurred within 24 h of shaving; (iv) mice were outside the weight range.
Two days following shaving and toe clipping, animals were initiated by treatment with a topical application of DMBA (catalog no. 1176775; Fisher Scientific, Houston, TX). The DMBA was mixed on the day of initiation and applied at a dose of 10 nmol in 200 µl of acetone to the shaved dorsoscapular region of the back. DMBA initiation occurred under subdued lighting conditions within the laboratory, as DMBA is light sensitive. Following DMBA initiation, mice were housed in disposable cages (4 mice/cage, 25x13x12 cm; Lab Products, Seaford, DE) with filter tops for 2 weeks in order to eliminate residual DMBA that might have been transferred to the cages or bedding. During these 2 weeks food and water were provided ad libitum and clean cages were supplied twice weekly. These initiated animals were maintained under low intensity yellow light conditions (yellow filter no. 4VC50; Grainger, San Antonio, TX). Following this `wash-out' period animals were returned to conventional Plexiglas cages and treatment of animals was continued according to the experimental design (see below). We arbitrarily designated week 1 as the first full week after the last day of the DMBA `wash-out' period.
When appropriate to the experimental design, control animals were included that were not initiated with DMBA. These control animals received only an application of 200 µl of the vehicle (acetone). Dosing of animals with acetone was performed under identical environmental conditions (i.e. subdued lighting) to those used for DMBA dosing. Following this vehicle dosing animals were housed and handled exactly as the DMBA-treated animals.
Papilloma promotion protocol
Animals received a specified dose of TPA (catalog no. 445004; Alexis Biochemicals, San Diego, CA), administered in 200 µl of acetone, applied to the dorsoscapular region of the back. All TPA promotion occurred twice a week between the hours of 0800 and 1200. Control animals received 200 µl of acetone (TPA vehicle).
The TPA stock solution (838 µg/ml TPA) was mixed at the beginning of each experimental series and was stored in an amber colored glass bottle at 20°C. TPA was diluted in acetone from the stock solution on each day of application.
Exposure systems and dosimetry MMW exposure system
Animals were exposed in the far field to 94 GHz RFR (continuous wave) (Applied Electromagnetics, Marietta, GA). A dielectric lens was placed 88 cm from the conical transmitter horn (24 mm i.d.) to increase the power density and focus the beam (37). Since the resulting field was parallel to the floor, a 45° aluminum reflector was placed 120 cm from the lens to aim the MMW field towards the animal's dorsal surface. The animal was located 60 cm below the aluminum reflector. In preliminary experiments IR thermography (FLIR Systems, Portland, OR) was used to determine the increase in skin temperature elicited by MMW or IR exposure at various power densities; the power densities chosen for use in the actual experiments were those required to elicit an increase in skin temperature of 1315 and 45°C in Experiments 1 and 2, respectively. In addition, IR thermography was performed during Experiment 2 at the beginning of the co-promotional phase (week 1) and at the end of the co-promotional phase (after week 12) to ensure that the increases in skin temperature produced by either MMW or IR exposure were consistent throughout the experiment.
IR exposure equipment
Two 250 W IR heat lamps (1100 nm peak spectral irradiance, catalog no. 250R40/10; Osram Sylvania Products, St Mary's, PA) were mounted 30 cm above the exposure area. The combined field intensity emitted from both lamps was adjusted using a Via-Stat Power Transformer (Superior Electric Co., Bristol, CN). Field intensity of both lamps was calibrated with a radiometer (Molectron Detector, Portland, OR) located at the center of the exposure area.
Restrainers
Each animal was exposed or sham exposed in a custom-designed Styrofoam restrainer that ensured correct placement of the animal during exposures to MMW and IR (38). A rectangular region (2.25x3 cm) was removed from the top part of the restrainer to permit exposure of only the dorsoscapular region of the mouse. Each restrainer held only one animal and each animal was exposed individually.
Experiment 1 (single exposure)
The goal of this experiment was to determine whether a single dose of MMW exposure (1.0 W/cm2 for 10 s) was sufficient to promote skin cancer in DMBA-initiated SENCAR mice. All animals in this experiment were initiated with DMBA. Following the end of the DMBA `wash-out' period, animals with a body weight that varied more than 20% from the mean of the entire colony were excluded from the experimental groups. All remaining animals were randomly assigned to one of the three experimental groups (MMW, IR and sham, n = 55/group) using body weight as a blocking variable to ensure that there were no statistical differences in initial group mean body weights.
In a pilot study IR thermography was used to determine the rise in skin temperature elicited by MMW exposure (1.0 W/cm2 for 10 s). The IR exposure parameters required to elicit the same increase in skin temperature (1315°C) were determined and subsequently used throughout the experiment.
During the experiment each mouse was anesthetized (Metofane), placed in a restrainer and the dorsoscapular region of the back was exposed once to MMW (1.0 W/cm2 for 10 s) or IR (1.5 W/cm2 for 10 s) or was sham exposed (placed in a restrainer for 10 s without irradiation). After exposure all animals were returned to their home cages and allowed to regain consciousness.
In addition to the three experimental groups, a positive control group (n = 27) was included to ensure the success of chemical initiation by DMBA. This positive control group was initiated at the same time as the experimental animals, using the same mixture of DMBA, however, this group was not exposed to MMW or IR, but received promotion by TPA (3.4 nmol in 200 µl acetone) twice weekly for 23 weeks.
For the duration of the experiment (23 weeks) each animal was weighed, visually inspected and palpated once each week for papilloma formation. The individuals performing the visual inspection and palpation of the animals were blind as to the animals assigned to each experimental group. At the end of the 23 week period mice were killed by CO2 inhalation. Five animals were randomly chosen from each group for necropsy. Any other animals displaying irregularities of the skin (i.e. lesions that appeared to be abnormal papillomas) were also selected for necropsy and examined via histopathology.
Experiment 2 (repeated exposure)
The goal of this experiment was to determine if repeated MMW exposure (2 exposures/week for 12 weeks, 333 mW/cm2) was sufficient to promote or co-promote skin cancer in DMBA-initiated SENCAR mice.
A pilot study was performed in order to determine the optimal dose of TPA to be used as the co-promoter. In this pilot study all animals were toe clipped and shaved as described above. Before DMBA initiation took place animals were separated into three experimental groups (n = 35/group) using body weight as a blocking variable. Groups 1 and 2 were initiated with DMBA (10 nmol in 200 µl acetone) while group 3 was treated with vehicle (acetone). Beginning 2 weeks following DMBA initiation and continuing for 16 weeks, group 1 received 0.85 nmol TPA and groups 2 and 3 received 1.7 nmol TPA. As described in the promotion protocol, all animals received TPA twice weekly on Tuesday and Friday between the hours of 0800 and 1200. All dosing with TPA was performed according to experimental group, starting with group 1 (receiving 0.85 nmol TPA) and progressing to groups 2 and 3 (1.7 nmol TPA).
For the duration of the pilot study (16 weeks) experimental animals were weighed, visually inspected and palpated for papilloma formation once each week by individuals who were blind as to the animals assigned to each experimental group. At the end of the 16 week period mice were killed by CO2 inhalation and animals were chosen for necropsy as described above.
The pilot study identified the TPA dose (0.85 nmol) to be used in the repeated exposure experiment (see Figure 1). This concentration of TPA reduced the possibility of a `ceiling effect' occurring. New animals were shaved and toe clipped and then separated into eight groups (n = 50/group) using body weight as a blocking variable (see Table I
). All groups except groups 3 and 8 were initiated with DMBA (10 nmol in 200 µl acetone); groups 3 and 8 served as control groups and were treated with 200 µl of acetone during the initiation phase.
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Before each exposure on Monday and Tuesday animals were weighed, visually inspected, and palpated. During each exposure animals were conscious and individually restrained and the dorsoscapular region of the back was either sham exposed (placed in a restrainer without irradiation for 10 s) or exposed to MMW (333 mW/cm2 for 10 s) or IR (600 mW/cm2 for 10 s). As before, the IR exposure parameters were chosen in order to match the increase in skin temperature (45°C) produced by the MMW exposure.
Following exposure animals were removed from the restrainer and immediately treated with either TPA or acetone. Application of the promoter or vehicle was performed after exposure to prevent any possible alteration in energy absorption due to the presence of fluid on the exposed region of the back. Animals were then returned to their home cages.
At the end of 12 weeks exposure of animals to MMW, IR or sham conditions was discontinued, however, TPA application continued until termination of the experiment at 23 weeks. Throughout the 23 week experimental period evaluators, blind as to which animals were assigned to each experimental group, counted and measured papillomas. At the end of the 23 week period mice were killed by CO2 inhalation and necropsied as described in Experiment 1.
Experiment 3
This experiment determined whether the repeated MMW exposure conditions used in Experiment 2 would induce alterations in well-accepted short-term biomarkers of carcinogenesis (27). Phase 1 of this experiment examined epidermal thickness and incorporation of 5-bromodeoxyuridine (BrdUrd) into DNA, whereas Phase 2 examined epidermal ornithine decarboxylase (ODC) activity. ODC is a key enzyme in the biosynthesis of polyamines that promote cell proliferation and the transition of many mammalian tissues from a relatively quiescent state to a rapidly proliferating population of cells is accompanied by large increases in ODC levels (39). All animals were shaved and toe clipped as described previously. Before DMBA initiation took place animals were separated into eight experimental groups using body weight as a blocking variable. Experimental groups and animal treatments were identical to those in Experiment 2 (see Table I).
Epidermal thickness and BrdUrd incorporation
Collection of skin samples. Four animals per experimental group were killed by CO2 inhalation at the end of 1, 2 and 5 weeks of treatment. Animals were killed 48 h after the most recent TPA treatment (0.85 nmol). One hour before death BrdUrd (Ccatalog no. B5002; Sigma, St Louis, MO) was dissolved in Dulbecco's 1x phosphate-buffered saline (PBS) at a concentration of 20 mg/ml. Thirty minutes before death animals were injected i.p. with BrdUrd at a dose of 100 µg BrdUrd/g body wt. Immediately following death a depilatory (Nair) was applied to the dorsoscapular region of the back (for 3060 s) and the hair was removed by gently scrubbing the back under cold water. Skin from the entire dorsoscapular area of the back was carefully excised and placed in 10% formalin. The excised skin was cut parallel to its long axis to yield two halves. One of these halves was cut parallel to its long axis into four 1 mm wide strips, each of which was fixed in 10% formalin for 12 h and then paraffin embedded. Paraffin blocks were sliced into 5 µm thick sections and the resulting slices were mounted on glass microscope slides.
Epidermal thickness: Skin sections were stained with hematoxylin and eosin. Epidermal thickness was evaluated using light microscopy by a board-certified veterinary pathologist who was blind as to the animals assigned to each experimental group. Epidermal thickness across the length of the strip that had been adjacent to the midline axis (i.e. the region above the spine) was evaluated on a scale from 0 to 4 according to the following criteria: 0, normal epithelium, ~13 cell layers thick with a thin stratum corneum; 1, minimal hyperplasia, epithelium ~46 cell layers thick; 2, minimal to mild hyperplasia, variable amounts of hyperplasia across the specimen, areas fitting each description present; 3, mild hyperplasia, epithelium ~79 cell layers thick or epithelial layer composed of ~46 hypertrophic cells; 4, moderate hyperplasia, epithelial layer ~1015 cell layers thick.
BrdUrd incorporation: BrdUrd incorporation into DNA was detected using immunohistochemical techniques (40). Staining consisted of deparaffinizing the skin sections and then incubating sections in a 0.05% protease (P5380, Type 8; Sigma) solution for 20 min followed by a wash with 0.01 M PBS/albumin. Sections were incubated in a 1:1500 dilution of BrdUrd primary antibody (33281A; BD PharMingen, San Diego, CA) for 12 h at 4°C. Sections were then rinsed in 0.01 M PBS/albumin and incubated in biotinylated secondary antibody (mouse IgG, PK-4002; Vector Laboratories, Burlingame, CA) for 30 min at room temperature. After rinsing with 0.01 M PBS/albumin, sections were incubated in the Vectastain ABC mixture from the above PK-4002 kit for 30 min at room temperature. After rinsing with 0.01 M PBS, sections were stained with a 0.1% 3,3'-diaminobenzidine tetrahydrochloride (D5637; Sigma)/0.02% hydrogen peroxide solution for 23 min. Slides were soaked in 70% and 95% alcohol and 100% 2-propanol for 2 min each. Sections were then rinsed in AmeriClear (C4200-1; Baxter Scientific, McGaw Park, IL) and coverslipped using Permount (SP15-100; Fisher Scientific, Fair Lawn, NJ).
Using light microscopy, random interfollicular fields were selected for scoring of BrdUrd-labeled nuclei. A total of 500 basal cells (labeled and unlabeled) adjacent to the basement membrane were evaluated and the labeling index was expressed as percent labeled cells. The microscopist was blind as to which animals belonged in each experimental group.
Epidermal ODC activity
Four animals per experimental group were killed by CO2 inhalation at the end of weeks 1, 2 and 5 of treatment. To serve as positive controls, additional mice were killed at 1 and 10 weeks of promotion with TPA (3.4 nmol). All animals were killed 6 h after the most recent TPA or acetone treatment. Immediately following death a depilatory (Nair) was applied to the dorsoscapular region of the back (for 3060 s) and the hair was removed by gently scrubbing the back under cold water. The backs of the mice were kept on ice until the skin samples were collected. Skin from this dorsoscapular area of the back was carefully harvested and spread on a chilled glass plate. The epidermal layer was removed by scraping the skin with a razor blade. Scrapings from each mouse was placed directly into 0.5 ml of homogenizing buffer, quick frozen with liquid nitrogen and stored at 70°C.
To achieve detectable ODC activity levels, epidermal samples from two mice within a treatment group were mixed together to form a single assay sample. This resulted in two assay samples within each treatment group. Epidermal tissue samples were placed in homogenizing buffer (25 mM sodium phosphate buffer, 5 mM dithiothreitol, 0.05 mM EDTA, 0.1 mM pyridoxal 5'-phosphate). Samples were homogenized on ice using a Polytron homogenizer (PT 10/35) set on a high setting (15 s on/15 s off/15 s on, to minimize sample heating). The cell lysates were centrifuged at 12 000xfor 30 min at 4°C. The clear lysates were transferred into fresh pre-chilled tubes. Total protein in 2 µl aliquots of each sample was measured by the bicinchonic acid method following the manufacturer's protocol (Pierce Chemical Co., Rockford, IL).
Samples were incubated in an assay mixture containing 35 mM sodium phosphate buffer, pH 7.2, 0.2 mM pyridoxal 5'-phosphate, 4 mM dithiothreitol, 1 mM EDTA and 0.4 mM L-ornithine (0.5 µCi [l-14C]DL-ornithine hydrochloride). Samples were incubated at 37°C for 1 h in 15 ml Erlenmayer flasks equipped with rubber stoppers and center well assemblies. A 2:1 (v/v) mixture of ethanolamine and methoxyethanol (200 µl) was added to the center well assembly. After the incubation period the reaction was stopped by addition of 0.5 ml of 2 M citric acid. The flasks were further incubated for 1 h to ensure complete absorption of 14CO2 by the ethanolamine and methoxyethanol mixture. Finally, the center well containing the ethanolamine/methoxyethanol mixture was carefully transferred to a vial containing 10 ml of toluene-based scintillation fluid and 2 ml of ethanol. Radioactivity was measured in a Beckman LS6000 SC liquid scintillation counter with >95% efficiency. The ODC enzyme activity was expressed as pmol 14CO2 released/h/mg protein.
Statistics
Based on data from the published literature (27), the power calculations for Experiment 1 showed that with 50 animals/group there would be a 90% power to detect a significant change (P 0.05) if the number of animals developing papillomas (tumor incidence) in each group differed by more than 8 (16%). Based on the TPA data from DiGiovanni et al. (27), power calculations for Experiment 2 showed that with 50 animals/group the smallest change required in tumor incidence to produce significance was 28%.
In Experiments 1 and 2 statistical analyses of tumor incidence at 16 and 23 weeks of promotion were performed using the 2 test (41). For multiplicity data mean number of tumors per mouse was calculated for each treatment group at each week of promotion. MannWhitney U-tests were used to compare treatment groups at 16 and 23 weeks of promotion. All analyses were performed using Statistica (StatSoft, Tulsa, OK). Statistical significance was considered to be P
0.05.
In Experiment 3 the epidermal thickness and BruUrd-labeled cells were each evaluated using analysis of variance (ANOVA) with a NewmanKeuls post hoc test. The assay for epidermal ODC activity required the pooling of epidermal cells resulting in two assay samples per treatment group. Thus, there was no within statistical cell error term.
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Results |
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There was little ODC activity in the animals receiving vehicle (acetone) rather than TPA (see Figure 4C). Furthermore, there were no substantial differences among those animals that were sham exposed or exposed to MMW or IR. TPA promotion increased epidermal ODC activity gradually over the 5 week period. In these TPA-treated groups there were no substantial differences among animals sham exposed or exposed to MMW or IR.
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Discussion |
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To our knowledge, the present study is the first to investigate potential carcinogenic effects at frequencies in the MMW range. The experiments presented herein address two potential scenarios of accidental overexposure. The first is a single, accidental overexposure to a relatively high power density of MMW (Experiment 1). A single MMW exposure did not alter either tumor incidence or multiplicity in DMBA-initiated SENCAR mice, providing strong evidence that, under the conditions of the experiment, a single high dose of MMW is insufficient to promote tumor formation in previously initiated skin. This finding is not surprising, since even known promoting agents must be applied repeatedly to produce an increase in tumorigenesis in initiated skin (25). The second exposure scenario is that of repeated exposure to lower levels of MMW (Experiment 2). Again, MMW exposure (twice a week for 12 weeks) did not alter tumor incidence or multiplicity in DMBA-initiated mice, either alone or when MMW exposure was combined with treatment with a known chemical promoter (TPA). Thus, there was no evidence that MMW exposure under these experimental conditions served as either a promoter or a co-promoter in a well-accepted animal model of skin carcinogenesis (25).
This conclusion was further buttressed by the results from the assays of early biomarkers of tumor-promoting activity. Epidermal hyperplasia-associated effects were assessed using three different procedures: epidermal thickness (27), BrdUrd labeling index of epidermal cells (27,42) and epidermal ODC activity (39,43,44). Not surprisingly, all of these indices of epidermal hyperplasia were increased by promotion with TPA, as in previous studies (27,39,4244). Exposure to MMW alone did not alter any of these early biomarkers and MMW exposure did not affect the increases in these indices of epidermal hyperplasia that were associated with chemical promotion by TPA. These results are consistent with the tumor multiplicity and incidence data and provide further support for the conclusion that MMW exposure does not promote tumorigenesis.
A number of similarities have been noted between skin cancer in humans and chemically induced skin cancer in SENCAR mice. As examples, the development of skin cancer in both species is associated with alterations in the tumor suppressor gene p53 (45), loss of heterozygosity at specific chromosomal loci (46), altered cyclin kinase inhibitor activity (47,48) and increased clusterin protein expression during photodynamic therapy (49). Furthermore, skin tumorigenesis is inhibited by retinoids (50) and prevented by drugs that inhibit epidermal lipid peroxidation (51). Thus, the SENCAR mouse skin cancer model used in the present experiments is an appropriate model for extrapolation to questions concerning human skin cancer.
In a two-stage skin tumorigenesis protocol using DMBA-initiated SENCAR mice, Mitchel and colleagues demonstrated that hyperthermic treatment (44°C for 30 min in a water bath) could serve as a co-promoter if applied near the time of initiation (35), but as an anti-promoter if applied near the time of chemical promotion (33,34). Furthermore, although hyperthermia alone is not carcinogenic, hyperthermia may enhance the development of tumors induced by ionizing radiation (52,53). Based on this information, we included IR exposure in our experimental design to control for any non-specific effects of hyperthermia alone and to ensure that any carcinogenic effects of MMW exposure would be a product of the RFR energy rather than this potential confounding variable. The hyperthermia response to MMW or IR exposure did not alter tumor development under either experimental paradigm, despite the fact that hyperthermic exposure occurred in close time proximity to the application of TPA; additionally, neither MMW nor IR exposure significantly altered any of the early markers of tumorigenesis. The finding that hyperthermia did not serve as an anti-promotor in our experiments may be due to the relatively short exposure duration (10 s) as compared to the 30 min used by Mitchel and colleagues (33,34).
In summary, neither a single exposure to relatively high levels of 94 GHz RFR nor repeated exposure to lower doses of 94 GHz RFR altered either tumor incidence or multiplicity in DMBA-initiated SENCAR mice. Furthermore, repeated MMW exposures did not act synergistically with a known chemical promoter (TPA) to alter tumor incidence or multiplicity. Finally, repeated MMW exposure failed to alter epidermal thickness, the labeling (BrdUrd) index of epidermal cells or epidermal ODC activity, indices that are used as early markers of tumor-promoting activity. We therefore conclude that MMW exposure under these experimental conditions does not promote or co-promote tumorigenesis in this well-established animal model of skin carcinogenesis.
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Notes |
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Acknowledgments |
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The Animal Care and Use Committee at Brooks AFB approved the experimental protocols. The animals involved in this study were procured, maintained and used in accordance with the Federal Animal Welfare Act and the Guide for the Care and Use of Laboratory Animals, prepared by the Institute of Laboratory Animal ResourcesNational Research Council. The views, opinions and/or findings contained in this report are those of the authors and should not be construed as official Department of the Air Force, Department of the Army, Department of Defense or US Government position, policy or decision unless so designated by other documentation. Trade names of materials and/or products of commercial or non-government organizations are cited as needed for precision. These citations do not constitute official endorsement or approval of the use of such commercial materials and/or products. Approved for public release; distribution unlimited.
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References |
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