Farrerol and cisplatin (15663-27-1) were obtained from Chengdu Pufei De Biotech Co., Ltd. (Chengdu, China) and MedChemExpress (New Jersey, United States), respectively. Primary antibodies against Nrf2(ab31163), Keap1 (ab139729), HO-1 (ab68477), NQO1 (ab80588), PINK1 (p0076), NOX4 (A11274) and β-actin (km9001) were obtained from Sigma-Aldrich (St. Louis, MO, United States), Sungene Biotech Co., Ltd (Tianjin, China) and Abcam (Cambridge, MA, United States). Antibodies specific to KIM-1 (AF 1817), NGAL (AF 1857), TGF-β (E-AB-33090), E-cadherin (E-AB-70249), Smad (E-AB-21040), collagen I (E-AB-34264), α-SMA (E-AB-21040), NLRP3 (MAB7578) and p-NF-Κb (13346) were purchased from R&D Systems (Minnesota, MN, United States), Elabscience Biotechnology (Wuhan, China) and Cell Signaling Technology (Boston, MA, United States).

C57BL/6 wildtype and Nrf2-knockout mice were purchased from Vital River (Beijing, China) and Jackson Laboratory (Bar Harbor, ME, United States), respectively. C57BL/6 wild-type and Nrf2 knockout mice were randomly assigned to experimental groups receiving the following treatments: control (saline), CDDP (10 mg/kg) only, farrerol (10 mg/kg) only, or CDDP (10 mg/kg) + farrerol (10 mg/kg). The mice were administered farrerol at 10 mg/kg body weight by intraperitoneal injection beginning 1 day before the first CDDP injection and daily until the day of harvest in the CDDP-AKI mouse group or 5 days after the second cisplatin injection in the CDDP-CKD mouse group. The mice were euthanized on day 3 (CDDP-AKI) or day 38 (CDDP-CKD) after the first administration of cisplatin. C57BL/6 wild-type and Nrf2 knockout mice were maintained on a normal diet and provided free access to drinking water during this experiment. All mice were kept in a specific pathogen-free facility, and this experiment was approved by the Animal Health and Research Ethics Committee of Jilin University.

Kidney function was analyzed according to the BUN and SCr levels. Serum samples of BUN and SCr were collected and measured using the relevant kits purchased from Nanjing Jiancheng Bioengineering Institute (Nanjing, China), and then the content of BUN (640 nm) and SCr (546 nm) in the serum sample is obtained by measuring the OD value and data processing. In addition, kidneys were homogenized and dissolved in extraction buffer, and the levels of MPO, MDA, SOD, and GSH were analyzed using kits (Keygen Biotech. Co., Ltd., Nanjing, China) according to the manufacturer’s instructions.

Fresh kidney tissue was dissected and immediately fixed with 4% paraformaldehyde. Then, a microscope was used to analyze sections from the paraffin-embedded mouse kidneys stained with hematoxylin and eosin (H&E) or Masson reagents. The damaged tubule scores were divided into the following levels: grade 0, no damage; grade 1, <25%; grade 2, 25–49%; grade 3, 50–74%; and grade 4, ≥75%. Additionally, Masson’s staining was used to evaluate the renal tissue fibrosis area.

The kidney tissue protein was separated by 10 or 12.5% sodium lauryl sulfate polyacrylamide gel electrophoresis and transferred to a polyvinylidene fluoride membrane. The membrane was blocked and shaken in 5% skim milk and then incubated with the corresponding primary and secondary antibodies for protein detection. Then, we used ECL to observe the bands and utilized ImageJ gel analysis software to quantitatively analyze the band intensities.

Paraffin-embedded kidney sections were deparaffinized and rehydrated. Then, we processed and microwaved the slices in citrate buffer and subsequently blocked them with 5% BSA for 20 min. The slides were incubated with primary antibodies against α-SMA and then incubated with secondary antibodies. Then, an optical microscope was used to observe the changes in kidney morphology and the area of positive staining.

Fresh kidneys were harvested and prefixed with glutaraldehyde and then fixed with osmium tetroxide. Afterwards, the samples were dehydrated in ethanol containing 3% uranyl acetate and embedded in epoxy resin and propylene oxide. After polymerization, the samples were cut into 70 nm-thick sections, stained, and then inspected with TEM. The quantification of mitochondrial contour measurements (feret minimum and maximum, area, perimeter, aspect ratio, shape factor, and roundness) in the kidney tissue sample were calculated using ImageJ software. Feret minimum and maximum represent the longest and shorted diameter in mitochondrial. Area, perimeter, aspect ratio, and roundness describe the degree of flatness of a contour. The shape factor corresponds to the outline of a contours. Contour measures are related as follows: A s p e c t   R a t i o   =   M a x D i a m e t e r M i n D i a m e t e r S h a p e   f a c t o r   =   P e r i m e t e r A r e a R o u n d n e s s   =   4 ⋅ A r e a π ⋅ M a x D i a m e t e r 2

Human renal tubular epithelial cells line (HK-2) obtained from Chinese Cell Bank (Beijing, China) were maintained in DMEF containing 10% fetal bovine serum, 100U/ml penicillin-streptomycin, in a 37°C, 5% CO2 incubator. After 72 h of transfection of HK-2 cells with the control siRNA or Nrf2 siRNA, HK-2 cells were seeded in a 6-well plate (5 × 105 cells/well), treated with or without farrerol (20 μM) for 24 h, and then collected cells for western blotting.

The data are presented as the mean ± SEM and were analyzed using SPSS 19.0 (IBM). The experimental data were compared by one-way analysis of variance (ANOVA). Statistical significance was defined as p < 0.05.

Firstly, we compared the changes in body weight, kidney index, BUN, and SCr of farrerol pretreatment before cisplatin injection and farrerol (not pretreatment) after cisplatin injection in mice to establish a reasonable mice model. As shown in Supplementary Figure S1, we found that farrerol pretreatment before cisplatin injection exert more pronounced protective effect on the kidneys than farrerol (not pretreatment) after cisplatin injection. Therefore, we chose to use farrerol pretreatment to evaluate the protective effect of farrerol against recurrent cisplatin treatment. On the day before the first intraperitoneal injection of cisplatin, the mice were pretreated with intraperitoneal farrerol (10 mg/kg) or vehicle, and farrerol administration was continued daily until 5 days after the second intraperitoneal injection of cisplatin (day -1 to day 12, 10 mg/kg). The mice were sacrificed on the 3rd and 38th days after the first injection of cisplatin to establish AKI and CKD models, respectively (Figure 1A). As shown in Figure 1B, the weight of mice treated with cisplatin decreased significantly, and farrerol significantly reversed this trend. Moreover, analysis of the kidney index also indicated that farrerol significantly improved the CKD caused by cisplatin (Figure 1C). In addition, farrerol improved CDDP-CKD, and this protective effect was demonstrated by renal index analysis (Figure 1C). In addition, farrerol pretreatment substantially alleviated the levels of BUN, SCr and the proximal tubular damage marker proteins NGAL and KIM1 (Figures 1D–G). We further elucidated the protective effect of farrerol on the mouse model by scoring H&E-stained sections and found that farrerol markedly reduced CDDP-induced histological lesions, such as tubular dilation and brush-border loss (Figures 1H,I).

Notably, damaged tubular epithelial cells can cause the release of a variety of proinflammatory cytokines to induce kidney inflammation (Lorenz et al., 2014). To determine whether cisplatin induces inflammation in renal tubular epithelial cells, immunoblotting was performed to detect the levels of inflammation-mediated proteins. As shown in Figures 2A,B, cisplatin stimulation significantly increased the expression of p-NF-κB and NLRP3 and upregulated downstream cleaved caspase-1 and IL-1β. Furthermore, farrerol significantly reduced the inflammatory response by inhibiting p-NF-κB and its downstream targets. In addition, persistent kidney damage and unresolved inflammation may lead to failure of tissue repair, thereby promoting the development of fibrosis (Qin et al., 2016). Mice treated with cisplatin showed a significant increase in fibrosis area that was reduced with farrerol pretreatment (Figure 2C). Moreover, cisplatin-induced fibrosis led to a substantial increase in TGF-β, stimulated the expression of fibrosis-related proteins (such as Smad, collagen I and α-SMA) and decreased the level of the antifibrotic protein E-cadherin (Figures 2D,E). To further illustrate that farrerol has a therapeutic effect on cisplatin-induced fibrosis, we conducted immunostaining of collagen I and α-SMA and confirmed that farrerol improves renal fibrosis (Figure 2F).

Repeated stimulation with cisplatin induces the production and accumulation of excess ROS in the proximal tubules of the kidney, causing an imbalance in the body’s redox system. After pretreatment with farrerol, the contents of MDA and MPO, which are key to the ROS-induced imbalance of the CKD redox system, were greatly reduced, and the contents of the antioxidant enzymes GSH and SOD were increased (Figures 3A–D). Previous experiments have shown that the antioxidant capacity of farrerol involves the activation of Nrf2. Therefore, we examined whether the antioxidant effect of farrerol on CDDP-CKD is related to the upregulation of Nrf2-mediated signaling pathways. The results showed that farrerol can effectively activate Nrf2 and its downstream target proteins HO-1 and NQO1 while reducing the levels of Keap1 and NOX4 (Figures 3E,F).

Mitophagy eliminates damaged mitochondria in renal tubular cells during the process of kidney damage and repair (Lin Q. et al., 2019). Moreover, Nrf2 also restores the mitochondrial dynamics of renal tubular cells by regulating PINK1-mediated mitophagy (Xiao et al., 2017). Thus, the possible involvement of the Nrf2/PINK1-mediated mitophagy pathway was tested in our experimental model. Similar to previous results, farrerol, as a Nrf2 activator, triggered PINK1/Parkin-mediated mitophagy on the 38th day of cisplatin administration, increased the accumulation of LC3 and decreased the protein expression of translocase of mitochondrial inner membrane 23 (TIM23), translocase homolog of mitochondrial outer membrane 20 (TOM20) and P62 (Figures 4A–C). Then, we also evaluated the effect of cisplatin on mitochondria through TEM and found that farrerol can reduce mitochondrial damage and activated mitophagy in the kidney (Figures 4D,E; Table 1). To better understand the role of mitophagy in cisplatin-induced kidney injury, we compared acute and chronic cisplatin-related mouse models. In our study, we found that Nrf2, PINK1, and Parkin were significantly increased on the third day of cisplatin stimulation. Moreover, we also found accumulation of LC3II, which suggested that autophagy was activated, and reduced levels of TIM23 and TOM20, indicating mitochondrial clearance by mitophagy. Most importantly, we also found that the changes in these proteins were significantly reversed on day 38 of cisplatin stimulation (Figures 4F–H). In addition, we also observed clear autophagosomes/mitophagosomes on the 3rd day of cisplatin stimulation, but on the 38th day, we observed a large number of damaged mitochondria and almost no autophagosomes/mitophagosomes unobserved on the 38th day, accompanied by a large number of damaged mitochondria (Figures 4I,J; Table 2).

Next, we assessed whether Nrf2 knockdown exacerbates kidney damage in mice. Changes in body weight, renal function index (BUN, SCr, KIM1, NGAL) and histological characteristics (H&E staining) were measured to assess kidney function in the mouse model. Compared with that of wild-type mice, the kidney function of Nrf2 knockout mice deteriorated significantly after treatment with cisplatin (Figures 5A–H). Most importantly, these results indicated that farrerol had little protective effect on Nrf2-deficient mice. In addition, compared with the wild-type mice, the Nrf2 knockout mice pretreated with farrerol did not exhibit a decrease in the area of fibrosis. In contrast, more fibrotic areas, a decrease in the antifibrotic protein E-cadherin, and an increase in the fibrosis-related protein collagen I were observed (Figures 6A–E).

To test whether the effect of farrerol on chronic oxidative stress induced by repeated CDDP stimulation is Nrf2 dependent, we measured and compared various oxidative stress markers in Nrf2 knockout and wild-type mice. As shown in Figures 7A,B, we observed no significant changes in Nrf2 or its downstream targets HO-1 and NQO1 in wild-type mice. In addition, in Nrf2 knockout mice, the increase in MPO and MDA and the decrease in SOD and GSH content induced by cisplatin were more pronounced, and this phenomenon was not reversed by farrerol pretreatment (Figures 7C–F).

Nrf2 null mice and wild-type mice were utilized to further explore the relationship between Nrf2 and PINK1. After analyzing the Western blot in Figures 8A–E, we found that farrerol did not upregulate the expression of the mitophagy-related proteins PINK1 and Parkin in Nrf2 knockout mice but resulted in an increase in TIM23 and TOM20 protein expression, which indicated that the knockout of the Nrf2 gene partially eliminated PINK1/Parkin-mediated mitophagy. Furthermore, TEM analysis showed that mitochondria were more damaged in Nrf2 knockout mice, and autophagosomes/mitophagosomes were hardly observed (Figures 8F,G; Table 3). These data indicated that the protective effect of farrerol against CDDP-CKD is mediated via activation of Nrf2 and PINK1/Parkin-mediated mitophagy. In order to directly observe the relationship between Nrf2 expression regulation and PINK1 transcription, based on the previous experiment (Ma et al., 2019), we treated the HK-2 cells with farrerol for 24 h. The results showed that farrerol could hardly activate the protein expression of PINK1. This result further proveed the above conclusion that Nrf2 can play a role mainly by regulating the expression of PINK1(Figures 8H,I).