Male Balb/c mice (age, 6 weeks; weight, 20–23 g) were purchased from Unilever (Shanghai, China). All mice had free access to water and food; they were kept in a room maintained at 60±10% relative humidity and 20±2°C with a 12 h light/dark cycle. There were 5 mice per cage. A total of 60 mice were randomly assigned into 3 groups (n=20 per group) as follows: i) Control (non-irradiated mice fed a standard diet without LF); ii) IR (whole-body irradiated mice fed a standard diet without LF); and iii) IR+LF (whole-body irradiated mice fed a diet containing 0.1% bovine LF; Sigma-Aldrich, Merck KGaA, Darmstadt, Germany). The mice in the IR and IR+LF groups were exposed to a sublethal radiation dose (7.0 Gy). The control mice were sham irradiated. The mice were irradiated using a 6-MV linear accelerator at a dose rate of 0.865 Gy/min (PRIMUS High Energy; Siemens AG, Munich, Germany). The mice were fed for 7 days prior to irradiation and for 30 continuous days following irradiation. The study protocol was approved by the Ethics Committee of Qianfoshan Hospital of Shandong Province (Jinan, China).

Blood was collected from the mice via the tail vein in EDTA tubes (BD Biosciences, Franklin Lakes, NJ, USA) on days 0, 1, 2, 3, 9, 14, 19 and 29 following irradiation. The blood was centrifuged at 1,000 × g for 20 min at 20±2°C and evaluated using an automated hematology analyzer (pocH-100i; Sysmex Corporation, Kobe, Japan) to provide the complete blood cell counts. The measurements included leukocyte, erythrocyte and platelet (PLT) counts, as well the hemoglobin. The normal references value of hematological parameters were described previously (21).

A volume of 0.15 ml whole blood was layered onto the lymphocyte separation medium (cat. no. MRGMA0; R&D Systems, Inc., Minneapolis, MN, USA) and centrifuged for 2 min at 3,500 × g at 20±2°C. The lymphocytes were subsequently transferred to a 1.5 ml tube containing 1.2 ml 0.1 M PBS and centrifuged for 5 min at 2,000 × g at 20±2°C. The lymphocytes were washed twice with PBS. The cells were then suspended in PBS and the density was adjusted to 5–6×10⁴/ml. A comet assay was performed under neutral conditions as described by Banath et al (22), with a slight modification. Specifically, special comet slides were used as opposed to conventional slides. All comet images were analyzed using CASP Lab software (version 1.2.3b2; CASPLab, Wroclaw, Poland) (23) and the percentage of DNA in the Olive Tail Moment (OTM) was recorded to characterize the lymphocytic DNA damage.

The livers were removed, fixed in 4% paraformaldehyde solution at room temperature for 20 min and ground 30 days after radiation (5 mice per group). The obtained cells were washed with PBS and suspended in EDTA. Superoxide dismutase (SOD) and malondialdehyde (MDA) activities in the liver were analyzed using SOD and MDA assay kits (Beyotime Institute of Biotechnology, Haimen, China) according to the manufacturer's protocol.

Data are presented as the mean ± standard deviation (≥5 mice per group at each time point). Statistical analysis was performed using one-way analysis of variance with a post hoc Tukey's test (multiple comparison test) to determine the significance of differences among multiple groups. P<0.05 was considered to indicate a statistically significant difference. SPSS version 13.0 software (SPSS, Inc., Chicago, IL, USA) was used for the analyses.

In the present study, mice in the IR and IR+LF groups were exposed to 7 Gy radiation. The survival rate was monitored on days 1–30 following irradiation (Fig. 1). Kaplan-Meier analysis indicated that survival rates were significantly higher in the IR+LF group compared with the IR group between day 12 and 30 (P<0.05). On day 30 the survival rate of the IR+LF group was 50% and the survival rate of the IR group was 33%. The survival rate in the IR+LF group was significantly higher compared with that of the IR group (P<0.05). The differences between the IR+LF group and the control were also statistically significant (P<0.05). These results suggest that LF increased the survival rate of mice following exposure to radiation.

The body weights of the mice were measured at various time points following irradiation and the mean weight ± standard deviation was calculated among surviving mice (Fig. 2). The results revealed that the body weights significantly increased in the control group, remained mostly constant in the IR+LF group and decreased slightly in the IR group between day 8 and 10 after irradiation. Statistical analysis indicated that body weight was significantly higher in the IR+LF group compared with the IR group between days 20 and 30 (P<0.05). Furthermore, the body weights of the mice in the control group were significantly greater compared with the IR+LF group on days 20 and 25 (P<0.05). Furthermore, on day 30, no significant differences in body weight were identified between the control group and the IR+LF group.

Hematological parameters were recorded following irradiation, including changes in the leukocyte count (Fig. 3). The leukocyte count in the IR+LF group exhibited a progressive decline to 1.9×10⁹/l on day 3. In addition, the leukocyte count appears to stay steady between days 9 and 14 in the IR+LF group at ~2.6×10³/µl. On day 29 the leukocyte count of the IR+LF mice had stabilized to within the normal range (7.6×10⁹−10.9×10⁹/l) (21). The significant difference was identified between the control group and the IR+LF group except on day 29 (P<0.05). However, the leukocyte count of the IR mice remained low (0.35×10⁹/l) until day 14. Between day 9 and 29, the leukocyte counts in the IR group were significantly lower compared with the IR+LF group (P<0.05).

In the IR+LF group the erythrocyte count decreased to 4.6×10¹²/l on day 9 and gradually recovered to a value of 6.47×10¹²/l on day 14 (Fig. 4). No significant difference was identified between the control group and the IR+LF group on day 29. In the IR group the erythrocyte count decreased to 2.17×10¹²/l on day 9. From day 9, the erythrocyte count in the IR+LF group was significantly greater compared with the IR group (P<0.05). The control group was significantly greater compared with the IR group between day 3 and 29 (P<0.05). These results indicate that LF improved erythrocyte repopulation in the mice.

Following a decrease post irradiation, the PLT count in the IR+LF group was restored to within a normal range on day 19 (Fig. 5) (21). However, in the IR group, the PLT count decreased to a minimum value at day 9 and slowly increased to a normal level (21) by day 29. The IR+LF group was significantly greater compared with the IR group between day 1 aand 9, and 19 and 29 (P<0.05). The control group was significantly greater compared with the IR and IR+LF group (P<0.05). No significant difference was identified between the control group and the IR+LF group on day 29. These results indicate that LF improved PLT repopulation in the mice.

The results also demonstrated that IR induced a significant decrease in the level of hemoglobin between days 7 and 21 following irradiation. Post irradiation, the hemoglobin levels in the IR+LF and IR groups were significantly lower compared with the control group (P<0.05; Fig. 6). The hemoglobin level recovered faster and was consistently increased in the IR+LF group compared with the IR group. The hemoglobin levels in the IR+LF group were significantly higher compared with the IR group (P<0.05). These results indicate that LF significantly enhanced the recovery of hemoglobin during the experimental period compared with the IR group.

The MDA level is associated with lipid peroxidation in the liver (24). The MDA level in hepatic tissue was significantly lower in the IR+LF group compared with the IR group, which suggests that the LF diet prevented hepatic lipid peroxidation (Table I). SOD activity indicates the generation of oxidative stress (25). The protective response to oxidative damage in the liver of IR mice decreased significantly following irradiation compared with the control group. However, the LF diet significantly prevented the change in SOD activity compared with the IR group.

Irradiation led to the breakage of DNA chains. The OTM percentage 24, 48 and 72 h post irradiation in the IR+LF group was significantly greater and lesser compared with the control and IR groups, respectively (P<0.05; Fig. 7). Following unwinding, DNA was affected by the electric field in the electrophoresis liquid, forming the distinctive comet tail formation (Fig. 8).