Use of a Small Animal Radiation Research Platform (SARRP) facilitates analysis of systemic versus targeted radiation effects in the mouse ovary

We have previously demonstrated that a single dose of 1 Gy TBI is sufficient to cause a significant reduction in ovarian follicles 2 weeks post-exposure in adult female CD1 mice, whereas a lower dose of 0.1 Gy is not [37]. Consequently, we exposed mice to a single dose of 1 Gy radiation but varied the field (Fig. 1a-c). We used the SAARP to generate three experimental cohorts of mice: one that received TBI, one that received targeted ionizing radiation to both ovaries, and one that received targeted radiation to a single ovary while the contralateral ovary was spared (Fig. 1a). Comparison of ovaries from mice that received TBI to those that were exposed to a targeted radiation field containing both ovaries allowed us to investigate systemic damage relative to targeted damage. In addition, by comparing targeted ovaries to contralateral non-targeted ovaries within individual animals, we were able to assess off-target effects in a paired organ system. For all cohorts, ovaries were harvested 2 weeks post-exposure. Importantly, we did not observe significant differences in animal weight among the cohorts at the time of tissue harvest (Fig. 1d). This consistency in weight in addition to the absence of animal lethality, suggests that the exposures to 1 Gy did not cause acute toxicity at this time point. We also did not observe any difference in the total number of serial sections obtained per ovary, suggesting that radiation exposure did not cause dramatic changes in ovarian size (Fig. 1e).

To examine the ovarian effects of systemic versus targeted radiation, we compared the ovaries from the animals that received TBI and targeted radiation to both ovaries (T2) to each other and to the Sham controls (Fig. 1). Ovarian histological sections were used to evaluate tissue appearance and to perform quantitative analysis of healthy follicles. Analysis of histological sections revealed that ovaries from all cohorts, irrespective of radiation exposure, had morphologically normal antral follicles and corpora lutea providing evidence of both follicle growth and estrous cyclicity (Fig. 2a-c). Whereas primordial and primary follicles were clearly visible in ovarian sections from the Sham cohort, they were not visible in the irradiated cohorts (Fig. 2d-f). In fact, in ovarian sections from both the TBI and T2 cohorts, only remnants of small follicles were visible, and these were not included in the follicle counts (Fig. 2e and f). To quantify these differences between the experimental groups and the Sham control, we classified and counted healthy follicles according to previously established morphological criteria (Fig. 3a) [38]. When examining all follicle classes together, both TBI and T2 cohorts showed a significant decrease in total counts relative to the Sham cohort (343.5 ± 92.0 follicles, 1761.0 ± 2620.3 follicles, and 6689.2 ± 2289.6 follicles, respectively; Additional file 1). We were particularly interested in primordial follicles, since they dictate the ovarian reserve and reproductive lifespan of an individual. Thus, we examined the number of primordial follicles in each experimental cohort separately from growing follicles. Within the Sham cohort, there was an average of 17.8 ± 2.0 primordial follicles per section (Fig. 3b) and 9.9 ± 1.4 growing follicles per section (Fig. 3c). Exposure to radiation significantly reduced the amount of average primordial follicles to 0.1 ± 0.1 follicles per section in the TBI cohort and 3.6 ± 6.6 follicles per section in the T2 cohort (Fig. 3b). Exposure to radiation also reduced the number of growing follicles to an average of 1.3 ± 0.3 growing follicles per section in the TBI cohort and an average of 4.7 ± 7.5 follicles per section in the T2 cohort (Fig. 3c). However, this reduction was only significant when comparing the TBI to the Sham cohort (Fig. 3c). If we further examined growing follicles on a class-specific basis, we observed that there were significantly fewer primary and secondary follicles in both the TBI and T2 cohorts relative to the Sham controls, but there were no differences in the number of antral follicles across cohorts, suggesting that the largest follicles are not sensitive to radiation-induced damage (Additional file 2).

Because we kept the ovaries from each individual animal separate for processing, we were able to further analyze the data to see if there were any differences in follicle counts depending on the animal or the respective ovary (Fig. 4, Additional file 3). In the Sham cohort, both primordial and growing follicle counts were similar across mice (Fig. 4a and b). The follicle counts between left and right ovaries were similar in two of the three mice, but in one mouse, the right ovary had significantly more follicles per section than the left (18.6 ± 6.9 and 14.5 ± 9.4 primordial follicles per section, respectively, and 12.5 ± 5.0 and 9.6 ± 6.7 growing follicles per section, respectively). In the TBI cohort, follicle counts were similarly low across all mice, and no differences were seen between the left and right ovaries in both primordial and growing follicle counts (Fig. 4c and d). In the T2 cohort, three of the five mice exhibited a near loss of all primordial and growing follicles in response to radiation, but two mice still had follicles present (Fig. 4e and f). In fact, one of the animals (mouse C) had follicle counts that were similar to those in the Sham cohort (Fig. 4a and c). Thus, the observation that mice in the T2 cohort had a less pronounced reduction in follicle numbers compared to the TBI cohort was primarily due to the response of two animals rather than a global phenomenon across the cohort (Fig. 3b-c and Fig. 4c-f). Specifically, mouse C and E still had primordial follicles present (Fig. 4e). Also in mice from the T2 cohort, all the right and left ovaries had similar numbers of follicles except for one mouse in which the right ovary had more follicles than the left (4.3 ± 2. and 0.0 ± 0.3 primordial follicles per section, respectively; Fig. 4e and 3.5 ± 2.7 and 1.1 ± 1.1 growing follicles per section, respectively, Fig. 4f).

To examine potential off-target effects of radiation damage to the ovary, we used the SAARP to deliver precise radiation to one ovary while sparing the contralateral ovary for each mouse (Fig. 1a; T1 cohort). In this case, the non-targted ovary served as an internal control or a within-animal comparison, which is typically not possible, i.e., when only TBI is used. Based on gross assessment of ovarian histological sections, both non-targeted and targeted ovaries still had antral follicles and corpora lutea present in the tissue similar to what we observed in the TBI and T2 cohorts; providing evidence of follicle growth and estrous cyclicity (Fig. 5a and b). However, there was a visible difference in the primordial and primary follicles between the targeted and non-targeted ovaries. Whereas the non-targeted ovaries had clearly visible primordial and primary follicles at the cortex, the targeted ovaries did not (Fig. 5c and d). These observations were confirmed with follicle counting. When examining all follicle classes together, we observed that the targeted ovaries had significantly fewer total follicles relative to the non-targeted ovaries, which were similar to the total in Sham controls (1356.3 ± 2222.5 follicles, 6508.8 ± 2723.4 follicles, and 6689.2 ± 2289.6 follicles, respectively; Additional file 1). When focusing specifically on primordial follicles, we found that the targeted ovaries had significantly less primordial follicles per section compared to the non-targeted ovaries (2.3 ± 4.7 vs. 18.0 ± 11.7 primordial follicle per section, respectively, Fig. 6a). There were also fewer growing follicles in the targeted ovaries compared to the non-targeted ovaries (2.2 ± 2.4 growing follicles per section vs. 6.9 ± 1.5 growing follicles per section, respectively, Fig. 6b), and this was primarily attributable to changes in secondary follicles (Additional file 4). Interestingly, there were no changes in antral follicle counts in the different experimental cohorts, again suggesting that the largest follicles are not sensitive to radiation-induced damage (Additional file 4). To examine whether there was variability among mice, we examined follicle counts across individual animals (Fig. 6c-d, Additional file 4). While the number of primordial follicles in the non-targeted ovaries was similar in three of the four mice, mouse A had significantly more follicles than mouse D (34.1 ± 18.3 primordial follicles per section vs. 6.1 ± 4.7 follicles per section, respectively, Fig. 6c). There were no animal-specific differences in the number of growing follicles (Fig. 6d). Nevertheless, across animals, the targeted ovaries consistently exhibited a significant decrease in both primordial and growing follicle counts compared to their non-targeted counterparts (Fig. 6c and d). When further examining growing follicles according to specific follicle class, the targeted ovaries in each animal had significantly fewer primary and secondary follicles relative to the non-targeted ovary except for mouse B that had similar numbers of primary follicles in both ovaries (Additional file 4). Again across animals, there were no differences in antral follicles between the targeted and non-targeted ovaries (Additional file 4).

Although these results demonstrate that the SARRP is able to deliver precise radiation to a field as small as a single ovary, we wanted to assess whether there was any off-target damage to the non-targeted contralateral ovary. Therefore, we compared follicle counts in the T1 cohort (right ovary: non-targeted; and left ovary: targeted) to those in the Sham cohort (Fig. 6e-f). As expected, we found that when comparing the average primordial follicle counts in Sham controls to the targeted ovary in the T1 cohort, there was a marked decrease in primordial follicle counts: 17.8 ± 2.0 and 2.3 ± 4.7 primordial follicles per section, respectively (Fig. 6e). This decrease was also true for growing follicles where there were 9.9 ± 1.4 growing follicles per section in the Sham cohort but only 2.2 ± 2.4 growing follicles per section in the targeted ovaries from the T1 cohort (Fig. 6f). In contrast, there was no difference when comparing the average follicle counts in the Sham ovaries relative to the counts in non-targeted ovaries from the T1 cohort for either primordial or growing follicles, indicating negligible off target effects (Fig. 6e-f). Interestingly, when examining the growing follicles according to class, there did appear to be a decrease in primary follicles between the Sham and non-targeted cohorts, suggesting that primary follicles may be sensitive to off-target radiation effects (Additional file 4).

Female CD-1 mice (6 weeks old) from Envigo (Indianapolis, IN) were used in this study. Mice were housed in a controlled barrier facility at the University of Kansas Medical Center (KUMC) under constant temperature, humidity, and a 12 h light/dark cycle. Food and water were provided ad libitum. All animal experiments were approved by the Institutional Animal Care and Use Committee and were performed in accordance with the National Institutes of Health Guidelines.

Mice were randomized into experimental cohorts 1) those that were exposed to total body irradiation (TBI), 2) those that received radiation targeted to both ovaries (T2), and 3) those that received radiation targeted to one ovary (T1) (Fig. 1a). Sham mice served as controls. Between 3 and 5 mice were used in each experimental cohort. The Xstrahl Small Animal Radiation Research Platform (SARRP, Xstrahl Inc., Suwanee, GA) was used to deliver a conformal dose of 1 Gy at a dose rate of 0.037 Gy/sec with an exposure time of 27 s to a designated field (Fig. 1b-c). Mice were anesthetized using a subcutaneous injection of buprenorphine (0.05–0.1 mg/kg) and then placed on the irradiator platform (Fig. 1b). The mice in the TBI group were irradiated in a field containing the whole mouse with the collimator removed. Mice in the T2 cohort were irradiated in a 20 mm × 10 mm collimated field containing both ovaries, whereas mice in the T1 cohort had only the left ovary exposed to radiation in a 10 mm × 10 mm collimated field (Fig 1c). The spine and the knee served as landmarks for defining the exposure field. Sham mice were handled the same way as those that were irradiated (i.e. handled, anesthetized, placed in the microirradiator) but were not exposed to radiation. Mice in all cohorts were monitored post-exposure to ensure that there were no visible acute effects of radiation and were weighed and euthanized 2 weeks post-procedure.

Ovaries were harvested from all mice, and the bursa was removed by careful dissection under a light microscope. The right and left ovaries for each mouse were processed separately. Ovaries were fixed in Modified Davidson’s fixative which is a prepared combination of 14% ethyl alcohol, 37.5% formalin, 37–39% glacial acetic acid, in 1 L of deionized water (Electron Microscopy Sciences, Hatfield, PA). Ovaries were rocked gently in fixative for 6 h at room temperature and then transferred to 4 °C overnight (~ 15 h). Samples were washed in 70% ethanol and processed and dehydrated using an automated tissue processor (Leica Biosystems, Buffalo Grove, IL). Ovaries were placed in molds and embedded in paraffin wax (Leica EG1160, Leica Biosystems, Buffalo Grove, IL). Paraffin embedded ovarian blocks were serial sectioned at a thickness of 5 μm using a Leica RM2335 microtome (Leica Biosystems, Buffalo Grove, IL). Every fifth section was placed on a separate slide designated for hematoxylin and eosin (H&E) staining to facilitate follicle counting. Stained sections were counted as a proxy for ovarian size to determine any differences between experimental groups (Fig. 1e). Slides were H&E stained using the AutostainerXL (Leica Biosystems, Buffalo Grove, IL). Whole slides were digitally imaged at the University of Washington Histology and Imaging Core using the Hamamatsu-HT imaging system (Hamamatsu Photonics, Hamamatsu City, Japan). NanoZoomer Digital Pathology Software (Hamamatsu Photonics) was used to analyze the images for follicle counting.

We used established morphological criteria to classify and count healthy follicles [38]. Atretic follicles with pyknotic granulosa cells or abnormal oocytes were excluded. In brief, a primordial follicle was defined as an oocyte surrounded by a complete or incomplete layer of squamous granulosa cells; a primary follicle was defined as an oocyte surrounded by a single complete layer of cuboidal granulosa cells; a secondary follicle was defined as an oocyte surrounded by two or more layers of granulosa cells; finally, antral follicles were defined as an oocyte surrounded by multiple layers of granulosa cells and containing a clear fluid filled cavity. Secondary and antral follicles were only counted if the oocyte nucleus was visible to avoid double counting. Follicles were grouped into two classes: primordial and growing. Growing follicles were defined as any follicle that was primary, secondary, or antral. Follicles were counted on every 5th section and either reported as total counts per experimental cohort or the number of follicles per total number of sections counted for each respective ovary.