Isoginkgetin-loaded reactive oxygen species scavenging nanoparticles ameliorate intervertebral disc degeneration via enhancing autophagy in nucleus pulposus cells

Excessive reactive oxygen species (ROS) in nucleus pulposus cells (NPCs) promote extracellular matrix (ECM) degradation and cellular inflammatory responses by activating a variety of cellular pathways, ultimately inducing cell apoptosis and leading to the development of low back pain. Here, we designed and fabricated an isoginkgetin-loaded ROS-responsive delivery system (IGK@SeNP) based on diselenide block copolymers. Successfully encapsulated IGK was released intelligently and rapidly in a microenvironment with high ROS levels in degenerative disc. Controlled-release IGK not only efficiently scavenged ROS from the intervertebral disc together with diselenide block copolymers but also effectively enhanced autophagy in NPCs to inhibit ECM degradation and cell apoptosis, and showed significant therapeutic effects in the rat intervertebral disc degeneration (IDD) model. Overall, the synergistic effects of IGK@SeNP in ROS scavenging and autophagy enhancement endowed it with an attractive therapeutic strategy for IDD treatment.

Low back pain caused by intervertebral disc degeneration (IDD) has become an important public health concern [1, 2]. In degenerated discs, excessive ROS promote organelle damage, extracellular matrix (ECM) degradation, and cellular inflammatory responses by activating various pathways, ultimately inducing functional cell death in the disc, causing spinal motor unit instability and radicular pain [3,4,5,6,7]. As there are no blood vessels in the intervertebral disc, the concentration of drugs in the intervertebral disc is low, and the efficacy is poor when administered systemically [8, 9]. Currently, the commonly used conservative treatment for IDD is pharmacological analgesia and dehydration [10]. However, these methods can only temporarily relieve pain and eliminate nerve swelling, but cannot remove excessive ROS to delay the progress of IDD, let alone achieve the purpose of curing IDD.

The intervertebral disc consists of a gelatinous inner nucleus pulposus and tough outer annulus fibrosus. The nucleus pulposus is the site of initial degeneration caused by oxidative stress [11]. Early recognition and removal of excessive ROS is a viable therapeutic strategy [12, 13]. For instance, Yang et al. [14] designed an injectable composite hydrogel, which sustained the release of Prussian blue nanoparticles to clear excessive ROS and showed good therapeutic effects in a rat IDD model. Although this strategy can effectively remove excessive ROS, nucleus pulposus cells (NPCs) cannot completely repair oxidative damaged biomolecules and organelles, which seriously affects the metabolic balance and cell viability, and may eventually lead to apoptosis [15, 16]. Therefore, it is necessary to develop a new therapeutic strategy that can not only remove too much ROS in NPCs but also promote the rapid repair of oxidative damage.

When NPCs are subjected to oxidative stress, cells can repair themselves by regulating the level of autophagy to breakdown damaged cellular components [17]. However, when ROS are cleared, cellular autophagy is downregulated, and cells cannot effectively clear damaged organelles, which may cause the cells to undergo apoptosis. Several studies have shown that upregulation of autophagy in NPCs can promote the repair of oxidative damage and reduce apoptosis [18,19,20]. Isoginkgetin (IGK), a natural flavonoid extracted from ginkgo biloba leaves, can enhance autophagy and scavenge ROS [21, 22]. We believe that it may be a potential drug for the treatment of IDD.

In this study, we designed and prepared an ROS-responsive IGK-loaded nanodelivery system (IGK@SeNP) that contained Se-Se bonds and showed good biocompatibility. The encapsulated IGK was intelligently released under the stimulation of high levels of ROS in the degenerative intervertebral disc. Under the combined treatment of IGK and Se-Se bonds, intracellular ROS was effectively cleared. Moreover, controlled-release IGK increased the autophagy level in NPCs, which balanced the anabolism and catabolism of ECM, inhibited apoptosis, and showed a significant therapeutic effect on IDD in vivo (Scheme 1). The strategy of removing intracellular ROS and enhancing autophagy to repair oxidative damage provides a safe and effective novel treatment for IDD.

Diagram of IGK@SeNP for the treatment of IDD. A ginkgo biloba extract, IGK, is loaded in Se-Se bond-containing nanoparticles (SeNP). IGK@SeNP is easily taken up by NPCs, and then SeNP scavenges ROS and releases IGK to enhance autophagy, which synergistically protects the ECM of NPCs and reduces cell apoptosis under oxidative stress

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Construction and characterization of IGK@SeNP

The diselenide-containing polymer (Se polymer) was synthesized according to our previous study (Fig. 1A). Briefly, di(1-hydroxylundecyl) diselenide was first synthesized, polymerized with isophorone diisocyanate (IPDI), and finally reacted with methoxypolyethylene glycol (mPEG). The ¹H NMR spectrum demonstrated the successful synthesis of di(1-hydroxylundecyl) diselenide (Additional file 1: Fig. S1) and Se-polymer (Fig. 1B). GPC analysis determined the molecular weight of the Se-polymer to be 11950 g/mol (Additional file 1: Fig. S2).

Construction and characterization of SeNP. A Synthetic route of diselenide-containing polymer. B ¹H NMR characterization of diselenide-containing polymer. C TEM image and size distribution of SeNP. Scale bar = 200 nm. D Cumulative drug release curves of Cy5@SeNP at different concentrations of H₂O₂. n = 3, mean ± SD

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Owing to its amphiphilicity, the Se-polymer can self-assemble into nanoparticles (SeNP) in aqueous solution. The amphiphilic Se-polymer and hydrophobic IGK self-assembled into micelle nanoparticles in aqueous solution (hereafter referred to as IGK@SeNP). Transmission electron microscopy (TEM) revealed that the IGK@SeNP possessed a spherical morphology with an average diameter of approximately 100 nm (Fig. 1C). Dynamic light scattering (DLS) indicated that the average hydrodynamic diameter was approximately 108 nm, with a polydispersity index of 0.25.

In vitro drug release

The in vitro ROS-responsive drug release behavior of the nanoparticles was investigated. Insoluble Cy5 was loaded as the model cargo given its easy detectability (named Cy5@SeNP hereafter). Different concentrations of hydrogen peroxide (H₂O₂) divided this experiment into four groups: (a) PBS control group, (b) 50 μM H₂O₂ co-treatment group, (c) 100 μM H₂O₂ co-treatment group, and (d) 200 μM H₂O₂ co-treatment group.

As shown in Fig. 1D, in the control group, Cy5@SeNP achieved a drug release rate of only ~ 9% at 36 h, which indicated that Cy5@SeNP had favorable stability under physiological conditions. In contrast, in the three H₂O₂ treatment groups, the release rate significantly increased with increasing concentrations of H₂O₂. For example, under the stimulation of 200 μM H₂O₂, the drug was released rapidly, with a cumulative release percentage of  ~ 63% at 36 h. The above results suggest that SeNP exhibited an excellent property of controlled release in the presence of ROS. Therefore, we expect SeNP to release drugs to treat IDD under oxidative conditions.

Biocompatibility and ROS-scavenging properties in vitro

To determine the biocompatibility of the nanoparticles, we first treated NPCs with various concentrations of SeNP. The CCK-8 assay results showed that SeNP at 0–60 μg/ml had no significant toxicity on NPCs within 72 h (Fig. 2A). Therefore, we chose the concentration of SeNP to be 60 μg/ml in the subsequent study. IGK@SeNP at the above concentrations were co-incubated with NPCs for 72 h to detect their biocompatibility. Live/dead staining indicated that NPCs maintained good growth ability after co-culture with IGK@SeNP for 72 h, and the percentage of viable cells was not statistically different from that in the 24 h group (Fig. 2B, D). These results showed that the IGK@SeNP had excellent compatibility with NPCs.

Biocompatibility and ROS scavenging properties in vitro. A CCK-8 assay was used to evaluate the cell cytotoxicity of SeNP and IGK@SeNP against NPCs after incubation for 24 h, 48 h, and 72 h. n = 6, mean ± SD. B, D Live/dead staining and cell viability of NPCs co-cultured with IGK@SeNP (60 μg/ml) for 24 h, 48 h, and 72 h. Scale bar = 200 μm. n = 3, mean ± SD. ns, not significant. C Fluorograph of the cellular uptake of Cy5@SeNP by NPCs. Scale bar = 100 μm. E, F Flow cytometry analysis and relative geometric mean fluorescence intensity of intracellular ROS levels in NPCs treated with H₂O₂ (200 μM) and different treatments. n = 3, mean ± SD. *p < 0.05 compared to the H₂O₂ group

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Cy5 was used as a drug model to assess cellular internalization of the nanocarriers. As shown in Fig. 2C, when NPCs were co-cultured with Cy5@SeNP (red) for 2 h, red fluorescence was observed in cells, indicating that Cy5@SeNP was internalized into NPCs. After 6 h of culture, the red fluorescence intensity was significantly enhanced, indicating that more Cy5@SeNP were internalized by the NPCs. These results indicate that SeNP can be effectively internalized by NPCs.

To verify the ROS scavenging ability of IGK, SeNP, and IGK@SeNP, we established a cell model of oxidative stress in NPCs by co-incubating the NPCs with 200 μM H₂O₂ for 24 h and calculated the intracellular ROS content using geometric mean fluorescence intensity (gMFI). We found that intracellular ROS levels in the H₂O₂ group (gMFI = 1891 ± 53) increased 21-fold compared with the control group (gMFI = 77 ± 3). Subsequently, different NPC treatments were administered. As shown in Fig. 2E, F, IGK decreased intracellular ROS levels (gMFI = 683 ± 66), but its effect was weaker than that of SeNP (gMFI = 506 ± 44). In contrast, IGK@SeNP exhibited the strongest antioxidant capacity (158 ± 52). These results indicate that IGK@SeNP has an excellent synergistic effect in eliminating excessive ROS in NPC.

Anti‑ECM degradation effects of IGK@SeNP on NPCs

Western blotting was performed to evaluate the protective effect of IGK@SeNP on ECM (Fig. 3A, B). H₂O₂ treatment decreased the expression of the ECM anabolic proteins COL2, SOX9, and ACAN and increased the expression of the ECM catabolic enzymes MMP3, MMP13, and ADAMTS5. These changes indicate that oxidative stress tilts the metabolic balance of the ECM toward catabolism. Supplementation with IGK, SeNP, or IGK@SeNP reversed the disordered ECM metabolism induced by H₂O₂. However, the correction of protein expression in the IGK group was slightly weaker than that in the SeNP group, which may be due to the poor water solubility of IGK and its difficulty in entering cells to exert biological effects. Notably, in the IGK@SeNP group, the expression of ECM metabolism-related proteins was significantly restored, with a better effect than that in the IGK and SeNP groups. Furthermore, immunofluorescence (IF) staining was conducted for the representative component (ACAN) and stromelysin (MMP3) in the nucleus pulposus (Fig. 3C–F). Consistent with previous results, the IGK@SeNP group most significantly increased the fluorescence intensity of ACAN and decreased the fluorescence intensity of MMP3. Collectively, the above data showed that H₂O₂-induced oxidative stress can disrupt the metabolic balance of ECM, while the combination of SeNP and IGK can better regulate the anabolism and catabolism of ECM than individual treatments.

IGK@SeNP attenuates H₂O₂-induced ECM degradation. A Western blotting analysis of the expression of ECM anabolic proteins (COL2, SOX9, and ACAN) and ECM catabolic enzymes (MMP3, MMP13, and ADAMTS5) in 200 μM H₂O₂-induced NPCs treated with IGK (20 μM), SeNP (60 μg/ml), and IGK@SeNP (60 μg/ml). B Densitometric analysis of ECM metabolism-related protein levels. C–F IF staining of ACAN and MMP3 in NPCs. Scale bar = 100 μm. n = 3, mean ± SD. *p < 0.05 compared to the H₂O₂ group, †p < 0.05 compared to the IGK group

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Anti‑apoptosis effects of IGK@SeNP on NPCs

To determine the protective effect of the nanodrug delivery system on NPCs under oxidative stress, western blotting was used to detect changes in the expression of key proteins in the apoptotic pathway (Fig. 4A, B). After treatment with H₂O₂ for 24 h, the expression of BCL2 was downregulated, while BAX and cleaved caspase3 (CASP3) were upregulated, indicating that apoptosis was activated by oxidative stress. However, after treatment with IGK, SeNP, and especially IGK@SeNP, the changes in the expression of the above proteins became weaker, indicating that the apoptosis pathway was blocked.

IGK@SeNP inhibits H₂O₂-induced NPC apoptosis. A Western blotting analysis of the expression of an antiapoptotic protein (BCL2) and pro-apoptosis proteins (BAX and cleaved CASP3). B Densitometric analysis of apoptosis-related protein levels. C, D IF staining of cleaved CASP3 in NPCs. Scale bar = 100 μm. E, F TUNEL staining of NPCs after different treatments. Scale bar = 100 μm. G, H Flow cytometry analysis with FITC-annexin V/PI assay. *p < 0.05 compared to the H₂O₂ group, †p < 0.05 compared to the IGK group

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Accumulation of ROS has been demonstrated to increase the activity of CASP3, a critical protein in the apoptosis pathway, leading to amplification of the proteolytic cleavage cascade, ultimately causing cell apoptosis [23]. IF staining showed that the high level of cleaved CASP3 induced by H₂O₂ decreased in the IGK, SeNP, and IGK@SeNP groups, in which IGK@SeNP achieved the optimal effect (Fig. 4C, D). TUNEL staining showed increased DNA fragmentation in the H₂O₂ group, indicating that the NPCs underwent apoptosis under H₂O₂ stimulation (Fig. 4E, F). Fortunately, the number of TUNEL-positive cells decreased in the three experimental groups, and again, the IGK@SeNP group showed the strongest cytoprotection. These results were also confirmed with flow cytometry, showing that the apoptosis rate was 4.93 ± 0.28% in the control groups and 17.49 ± 0.75% in the H₂O₂ groups, which was reduced to 11.18 ± 0.14%, 9.71 ± 0.44%, and 7.02 ± 0.98% in the IGK, SeNP, and IGK@SeNP groups, respectively (Fig. 4G, H). The above results indicated that IGK@SeNP could effectively inhibit NPC apoptosis induced by H₂O₂.

Pro-autophagy effects of IGK@SeNP on NPCs

Moderate autophagy helps cells survive in harsh environments, whereas excessive autophagy also induces cell death [24,25,26]. Therefore, we explored the role of autophagy in the process of IGK treatment in IDD. As autophagy is regulated by multiple proteins at different stages, several key indicators are used to reflect changes in autophagic flux. For example, Beclin1 (BECN1) binds to pre-autophagosomes to initiate autophagosome formation. ATG7 participates in the assembly of autophagosomes by promoting the conjugation of ATG12 to ATG5 and the conversion of LC3I to LC3II. Then, LC3II binds to autophagosome membranes and is widely used as a marker for autophagy. Eventually, SQSTM1/p62 delivers autophagic substrates to the autophagosome and is degraded with these substrates in autolysosomes. As shown in Fig. 5A, B, H2O2 activated autophagy, marked by the upregulated expression of BECN1 and ATG7 and the ratio of LC3B II/I, while downregulating the expression of SQSTM1/p62. Treatment with IGK further amplified these changes in the protein levels. IF staining of LC3B also confirmed that there were more punctate structures in the IGK and IGK@SeNP groups, suggesting that the number of autophagosomes combined with LC3B II might be increased (Fig. 5C, D).

IGK@SeNP promotes autophagy in H₂O₂-treated NPCs. A Western blotting analysis of the expression of autophagy-related proteins (BECN1, ATG7, LC3B, and SQSTM1/p62). B Densitometric analysis of autophagy-related protein levels. C, D IF staining of LC3B in NPCs incubated with IGK, SeNP, and IGK@SeNP in the presence of H₂O₂ stimulation. Scale bar = 20 μm. E, F TEM analysis of morphology and the number of autophagosomes and autolysosomes in NPCs. Red arrows indicate autolysosomes with single membranes, while black arrows indicate autophagosomes with double membranes. M indicates mitochondria. Scale bar = 1 μm (upper row) and 500 nm (lower row). n = 3, mean ± SD. *p < 0.05 compared to the H₂O₂ group, †p < 0.05 compared to the IGK group

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Autophagy is a complex process because an increase in LC3II levels may be caused by either enhanced autophagic flux or insufficient autolysosomes [27]. Therefore, we detected autophagy-associated vesicles by TEM. As shown in Fig. 5E, in the H₂O₂ group, autolysosomes wrapped the damaged organelles, and mitochondria dissolved into vacuoles, suggesting that oxidative stress damaged mitochondria. However, the dysfunctional mitochondria were not completely cleared, which may have led to their continuous production of ROS and eventually induced apoptosis of NPCs. In addition, a higher number of autophagy-associated vesicles was observed after IGK treatment, especially in the IGK@SeNP group, indicating that the SeNP drug delivery system favored the autophagy-enhancing properties of IGK (Fig. 5F).

We also noticed that the SeNP group showed a slight inhibition of autophagy compared with the H₂O₂ group, but interestingly, the IGK-loaded SeNP still showed a more obvious autophagy enhancement effect. These results indicate that the autophagy stimulator IGK was steadily transferred and released from the ROS-responsive SeNP and more effectively enhanced autophagy, thus regulating ECM metabolism and restraining apoptosis of NPCs.

Effects of autophagy blockers on the therapeutic efficacy of IGK@SeNP

To confirm that IGK protects NPCs by enhancing autophagy, we treated NPCs with 10 μM chloroquine (CQ), an autophagic blocker that inhibits the fusion of autophagosomes with lysosomes. The protein levels of LC3B and SQSTM1/p62 increased after treatment with CQ, indicating an interrupted autophagic flux (Fig. 6A, B). Moreover, in the presence of CQ, the effect of IGK@SeNP in regulating the expression of ECM metabolism-related proteins (COL2, SOX9, ACAN, MMP3, MMP13, and ADAMTS5) and apoptosis-related proteins (BCL2, BAX, and cleaved CASP3) decreased (Fig. 6C–F). These results further verified that IGK@SeNP protects NPCs by enhancing autophagy under oxidative stress.

Autophagy blocker reduces the anti-ECM degradation effect and anti-apoptotic effect of IGK@SeNP. A Western blotting analysis of the expression of autophagy-related proteins in NPCs induced by H₂O₂ with or without CQ (10 μM) for 24 h. B Densitometric analysis of autophagy-related protein levels. C Western blotting analysis of the expression of ECM metabolism-related proteins in NPCs induced by H₂O₂ with or without CQ (10 μM) for 24 h. D Densitometric analysis of ECM metabolism-related protein levels. E Western blotting analysis of the expression of apoptosis-related proteins in NPCs induced by H₂O₂ with or without CQ (10 μM) for 24 h. F Densitometric analysis of apoptosis-related protein levels. n = 3, mean ± SD. *p < 0.05 compared to the H₂O₂ group, †p < 0.05 compared to the IGK group, #p < 0.05 compared to the same treatment groups without CQ

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Therapeutic efficacy of IGK@SeNP in the rat IDD model

Given the favorable results of in vitro anti-ECM degradation and anti‑apoptosis potential, the efficacy of IGK@SeNP in treating IDD in vivo was further evaluated in a rat model (Fig. 7A). The IDD rat model was established using needle puncture. Degenerative discs were locally injected with PBS, IGK, SeNP, or IGK@SeNP. Imaging examinations, including X-ray and magnetic resonance imaging (MRI), were used to evaluate the degree of disc degeneration 4 and 8 weeks after surgery. As shown in Fig. 7B, C, intervertebral height was significantly preserved in the IGK@SeNP group compared to that in the IDD group. However, the intervertebral height in the IGK group gradually decreased in 8 weeks, indicating that in vivo treatment with IGK alone is not very effective, while combining it with the SeNP drug delivery system enhanced the therapeutic effect. MRI revealed that the T2-weighted signal in the IDD group had declined, indicating a loss of water in these discs (Fig. 7D). After 6 weeks of treatment, the water content was preserved in the IGK@SeNP group, with significantly low signals in the IGK groups. The Pfirrmann grade results further confirmed that IGK@SeNP had superior efficacy for treating IDD in vivo (Fig. 7E).

IGK@SeNP protects the nucleus pulposus in needle puncture-induced IDD rats. A Treatment schedule of animal experiments. Two weeks after surgery, the IDD model was validated by MRI. PBS, IGK, SeNP, and IGK@SeNP were injected weekly thereafter. Imaging examinations were performed at weeks 4 and 8. B X-ray images of rat coccygeal spines at the 4th and 8th-week post-surgery. C Intervertebral heights of rat coccygeal spines measured on the X-ray. D T2-weighted MRI of coccygeal discs at the 4th and 8th-week post-surgery. E Pfirrmann grade scores of coccygeal discs measured on MRI. F, G HE and SF staining of rat coccygeal discs. Glycosaminoglycans are shown with safranin O. Scale bar = 1 mm. H Histological grade scores of coccygeal discs at the 4th and 8th-week post-surgery. n = 5, mean ± SD. *p < 0.05 compared to the IDD group, †p < 0.05 compared to the IGK group

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Histological sections were collected at 4 and 8 weeks after surgery. Hematoxylin–eosin (HE) staining was used to observe the morphology of the nucleus pulposus and annulus fibrosus (Fig. 7F). The nucleus pulposus of the IDD group prominently decreased in volume and was replaced by fibrous tissue at 8 weeks, and the arrangement of the annulus fibrosus was disordered. In addition, a substantial loss of glycosaminoglycans was observed at 4 and 8 weeks in the IDD group by safranin O-fast green (SF) staining (Fig. 7G). Histological changes induced by needle puncture were weakened in the IGK@SeNP group. However, in the IGK and SeNP groups, the loss of the nucleus pulposus was evident with destruction of the disc structure. Based on the histological grade, the IDD group recorded the highest score, whereas the IGK@SeNP group recorded the lowest score, except for the control group (Fig. 7H).

We performed immunochemical (IHC) staining to analyze the expression levels of ACAN and MMP3, which are representative indices of matrix metabolism in the nucleus pulposus. After needle puncture surgery, the expression of ACAN in all model groups was degraded, while the IGK@SeNP group maintained the highest ACAN expression among the model groups (Fig. 8A). Conversely, the expression of MMP3 was substantially increased in the IDD group and was relatively restrained in the IGK, SeNP, and particularly in the IGK@SeNP group, indicating that the ECM of the nucleus pulposus was rescued (Fig. 8B).

IGK@SeNP attenuates matrix degradation and cell apoptosis in vivo. A, B IHC staining of ACAN and MMP3 in rat coccygeal discs. C Quantitative analysis of ACAN- and MMP3-positive rates in different groups. D IF staining of cleaved CASP3 in rat coccygeal discs. E TUNEL staining of rat coccygeal discs. F Quantitative analysis of cleaved CASP3- and TUNEL-positive cells in different groups. Scale bar = 100 μm. n = 5, mean ± SD. *p < 0.05 compared to the IDD group, †p < 0.05 compared to the IGK group

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Subsequently, we used TUNEL assay and IF staining of cleaved CASP3 to analyze the apoptosis of NPCs in degenerative discs (Fig. 8D, E). In the IDD group, the apoptosis pathway was upregulated, and the apoptosis rate increased remarkably with time. However, treatment with IGK@SeNP inhibited this pathological progression in vivo. The above results indicate that IGK@SeNP exerts a prominent therapeutic effect on IDD in vivo.

The incidence of IDD increases with age and can lead to spinal instability, radicular pain, and even disability, making it a critical health issue [2, 28]. Many studies have found that ROS accumulation and high levels of oxidative stress are important causes of IDD development because they can cause ECM degradation and NPC death [29, 30]. Therefore, ROS have become a key target for the treatment of IDD. However, traditional therapeutic agents have difficulty accessing the interior of avascular intervertebral discs, so they can only reduce inflammation and temporarily relieve pain outside the intervertebral disc but cannot remove accumulated ROS, which makes them unable to fundamentally prevent the progression of IDD [31, 32]. Although some studies have used novel biomaterials to deliver drugs into the intervertebral disc and effectively reduce ROS levels, oxidatively damaged organelles are not removed simultaneously, which may cause blockage in the repair of cell viability and metabolic function, ultimately affecting the therapeutic effect [14, 33, 34]. Therefore, there is an urgent need to develop new strategies to effectively treat IDD by removing damaged organelles and reducing ROS. In this study, we fabricated an ROS-responsive nanodelivery system based on diselenide block copolymers that can load and intelligently release IGK, a natural autophagy stimulator. Our experiments confirmed that IGK@SeNP could effectively scavenge ROS and delay the progression of IDD in rats by enhancing autophagy to degrade oxidatively damaged mitochondria. Moreover, blocking autophagy attenuated the protective function of IGK@SeNP in regulating ECM metabolism and inhibiting apoptosis, indicating that IGK@SeNP has the dual efficacy of ROS clearance and autophagy enhancement, which makes it advantageous for IDD treatment.

Oxidative stress plays an important role in many physiological processes, such as cell signaling and immune responses. An important mechanism is that ROS can promote the expression of BAX and release cytochrome C by increasing the permeability of the outer mitochondrial membrane, which activates caspase-mediated cascade amplification and promotes apoptosis, resulting in tissue entrapment into a pathological state. Cheng et al. [33] revealed that the combination of antioxidants and thermosensitive hydrogels could decrease oxidative stress induced by H₂O₂ and restore the content of GAGs in the early stages of IDD. Bai et al. [35] developed a rapamycin-loaded hydrogel and successfully induced macrophage differentiation into the M2 phenotype, thereby alleviating the inflammatory microenvironment of the intervertebral disc. Zhu et al. [34] used MnO₂ nanoparticles to control the release of TGF-β3, and this approach suppressed H₂O₂-induced oxidative damage by increasing the expression of antioxidative genes. Our study showed that SeNP was able to scavenge ROS owing to the reducibility of Se-Se bonds, which prevented H₂O₂-induced ECM degradation and NPC apoptosis. However, this effect was insufficient. We found that although SeNP removed intracellular ROS, the autophagy level decreased, marked by the downregulation of initiation-related proteins (BECN1, ATG7, and LC3B). This deficiency resulted in the inability of NPCs to repair oxidatively damaged organelles, as vacuolization in mitochondria was observed in the SeNP group (Fig. 5E), and eventually induced NPC apoptosis.

Chen et al. [36] revealed that the PERK/eIF2α pathway could promote autophagy; however, blocking the PERK/eIF2α pathway or inhibiting autophagy reduced NPC viability. Further experiments that supported the cellular protective effect of autophagy showed that H₂O₂ induced DNA damage in NPCs and caused AIM2-associated inflammatory cascades. After enhancing autophagy, autophagy-dependent secretion promotes AIM2 inflammasome secretion from NPCs, which inhibits cellular DNA damage and apoptosis, thus delaying the progression of IDD [18]. In our experiments, IGK significantly activated autophagy and protected NPCs by removing damaged organelles. A recent study confirmed that IGK can inhibit proteasome degradation to stabilize the Nrf2 protein, thus promoting nuclear translocation of Nrf2, which in turn triggers the activation of the antioxidant system and plays a role in protecting mitochondria [37]. In the dysfunctional mitochondria, more electrons leak from mitochondrial complexes, which subsequently generate H₂O₂ under the catalysis of superoxide dismutase [38]. Endogenous ROS can destroy intracellular biomacromolecules and cause cellular dysfunction or even death. As an autophagy stimulator, IGK can both resist mitochondrial collapse and induce impaired mitochondrial clearance; thus, it has powerful therapeutic potential in ROS-induced IDD.

Many studies have attempted to treat IDD using multidrug administration. This strategy allows the pharmacological effects of several drugs to be superimposed on each other and achieves greater therapeutic effects at lower drug concentrations [39,40,41]. A recent study revealed that dysfunction of either autophagy or antioxidant systems can lead to aggravated detrimental effects of H₂O₂ on intervertebral disc cells [42]. Therefore, we combined an autophagy stimulator (IGK) with ROS scavenger (SeNP) and found that the assembled nanodelivery system exerted superior efficacy. Moreover, an autophagy blocker attenuated the therapeutic effects of IGK@SeNP on ECM metabolism regulation and inhibition of apoptosis, indicating that IGK-induced autophagy is necessary for NPC self-repair. In addition, SeNP allows IGK to be more stably present within the disc, which is beneficial in reducing the frequency of medication and the complications of intradiscal injection. These characteristics make its clinical application promising.

However, we also considered the limitations of this study. Although we employed H₂O₂ to induce NPC degeneration, there may be more complex pathophysiological features in the actual degenerated discs [43]. Therefore, we will use NPCs obtained from patients with IDD for further validation. Moreover, the intervertebral disc is an avascular closed structure, and nanoparticles injected in situ are rarely distributed to other organs [31]. Thus, our study did not investigate blood compatibility and toxicity in vivo. Although HE staining of intervertebral discs showed no obvious inflammatory cell infiltration, we will verify the in vivo biocompatibility if IGK@SeNP is used in other disease models. Overall, we propose a novel ROS-responsive nanodrug delivery system that can delay the progression of IDD by synergistically enhancing autophagy and scavenging ROS.

In this study, we synthesized a novel ROS-responsive nanodelivery system for SeNP loaded with IGK for IDD treatment. Our findings demonstrated that the nanoparticles had an ROS-stimulated responsive drug release effect. SeNP combined with IGK synergistically eliminated ROS and enhanced autophagy. IGK@SeNP protected NPCs and delayed the pathological process of IDD, both in vitro and in vivo. Collectively, this study suggests that IGK@SeNP may be an attractive therapeutic agent for treating IDD.

Materials and reagents

Selenium powder, sodium borohydride, isophorone diisocyanate (IPDI), methoxypolyethylene glycol (mPEG), dibutyltin dilaurate (DBTDL), 11-bromoundecanol, methoxypolyethylene glycols, Tetrahydrofuran (THF), hydrogen peroxide (H₂O₂), Cy 5 (Aladdin, Shanghai, China). Isoginkgetin (IGK), chloroquine (CQ), (MedChemExpress, Monmouth Junction, USA). Primary antibodies against aggrecan, collagen II, SOX9, MMP3, MMP13, ADAMTS5, ATG7, Beclin1, LC3B, SQSTM1/p62 (Abcam, Cambridge, UK), primary antibodies against BCL2, BAX and cleaved caspase-3 (Cell Signalling Technology, Danvers, USA), primary antibodies against β-actin (Proteintech, Wuhan, China). Goat anti-rabbit IgG H&L (Alexa Fluor^® 488), goat anti-rabbit IgG H&L (Alexa Fluor^® 594), (Abcam, Cambridge, UK), HRP-labeled goat anti-rabbit IgG (Proteintech, Wuhan, China). Penicillin–streptomycin (Sigma-Aldrich, St. Louis, USA). Cell counting kit-8 (CCK-8), Calcein/PI assay kit, ROS assay kit, and TUNEL apoptosis assay kit (Beyotime, Shanghai, China). Phosphate-buffered saline (PBS), FITC-annexin V/PI apoptosis detection kit, fetal bovine serum (FBS), DMEM/F12 (Thermo Fisher Scientific, Waltham, USA). Nitrocellulose membranes (Pall, New York, USA). Electrochemiluminescence substrate (Meilunbio, Dalian, China). Zoletile (Virvac, Carros, France).

Synthesis of IGK@SeNP

The synthesis of SeNP was consistent with our previous work description [44]. In brief, selenium powder (1 g, 12.7 mmol) was dissolved in deionized water (15 mL) with stirring under N₂ flow. Sodium borohydride solution (0.1 g/mL, 10 mL) was dropwise added to the reaction for 15 min. Secondly, another selenium powder (1 g, 12.7 mmol) was added and reacted for 15 min. Afterward, 11-bromoundecanol (6.33 g, 25.2 mmol) was dissolved in THF (25 mL) and added to the reaction system. The mixture was heated at 50 °C and maintained for 24 h, and then filtered while hot. The obtained solution was extracted three times with 20 mL of dichloromethane and dried with anhydrous sodium sulfate. The product was purified by column chromatography with a 1:4 mixture of ethyl acetate and methylene chloride as eluent. The di(1-hydroxylundecyl) diselenide was obtained after removing the solvent by rotary evaporation. Di(1-hydroxylundecyl) diselenide (2 g, 4 mmol) and IPDI (0.98 g, 4.40 mmol) were dissolved in THF (60 mL) under N₂ flow. Then DBTDL (0.05 mg, 0.1 mmol) was added as a catalyst. After a reaction for 2 h at 50 °C, mPEG₂₀₀₀ (13 g, 6.50 mmol) was added and the reaction was continued at 50 °C for 24 h. THF was removed by rotary evaporation. The obtained Se-polymer was purified by cold methanol precipitated and collected after vacuum drying.

IGK (1 mg), triethylamine (50 μL), and Se-polymer (10 mg) were dissolved in N,N-dimethylformamide (DMF, 2 mL) and stirred for 2 h. Deionized water (10 mL) was slowly added with stirring. Subsequently, the solution was dialyzed for 24 h (MWCO 3500 Da) against deionized water. IGK-loaded nanoparticles (IGK@SeNP) were obtained by ultrafiltration centrifugation (MWCO 10000 Da). The SeNP and Cy5@SeNP were constructed using the same method. IGK@SeNP were freeze-dried and dissolved in DMSO, then detected using a UV−vis spectrometer. The IGK loading content was 8.69% and the drug entrapment efficiency was 41.78%.

Characterization

¹H NMR spectroscopy was used to detect the Se-polymer modified with IPDI and mPEG. The number-average molecular weight (M̅n) and weight-average molecular weights (M̅w) of the Se-polymers were determined using gel permeation chromatography (GPC). The morphology of SeNP was observed and reported using a transmission electron microscope (TEM) at an acceleration voltage of 120 kV. The particle diameters and dispersion of particle size were reported by dynamic light scattering (DLS).

ROS-responsive drug release

5 mL of Cy5@SeNP solution was treated with gradient concentrations of H₂O₂ (0, 50, 100, 200 μM). The Cy5 content was measured using a fluorescence spectrophotometer at 650 nm excitation wavelength.

Cell culture and treatment

Human nucleus pulposus cells (NPCs, ScienCell, Carlsbad, USA) were cultured in DMEM/F12 medium supplemented with 10% FBS, 1% penicillin–streptomycin at 37 °C and 5% CO2. To simulate an oxidative microenvironment of degenerative disc, NPCs were pretreated with PBS, IGK, SeNP, or IGK@SeNP for 4 h, then stimulated with 200 μM H₂O₂ for 24 h.

Cellular uptake

Due to the lack of fluorescent properties of IGK, we used Cy5 as a drug model to investigate the cellular uptake of Cy5@SeNP in NPCs [45]. NPCs were seeded in 24-well plates. After washes with PBS, Hoechst 33342 was incubated with the cells for 30 min at 37 °C. Subsequently, the culture medium contained Cy5@SeNP replaced the original medium. The cellular uptake was observed by fluorescence microscope.

Live/dead staining assay

NPCs were seeded into 24-well plates and co-cultured with IGK@SeNP (60 μg/mL). After washing with PBS, the Calcein/PI staining dye was added and incubated for 30 min at 37 °C for 24, 48, and 72 h. After incubation, the cells were washed again and observed under a fluorescence microscope.

ROS-scavenging evaluation

Intracellular ROS level was detected by DCFH-DA. NPCs were cultured in 6-well plates and were treated as per the aforementioned protocol. Afterward, the cells were stained with DCFH-DA (10 μM) for 20 min at 37 °C and washed 3 times with serum-free DMEM/F12. The flow cytometer analysis was executed by FACSVerse.

Rat IDD model and treatment

All animal experiments were performed following the Ethics Committee for Animal Experiments. A total of sixty 8-week-old male SD rats were randomly allocated to 5 groups: Control, IDD, IGK, SeNP, and IGK@SeNP. The IDD model was established by needle puncture [46]. Rats were intraperitoneally anesthetized with 50 mg/kg Zoletile and 3 mg/kg xylazine hydrochloride. After successful anesthesia, the rats were placed prone on a clean operating table. The rat tails were disinfected and draped, and a 20G needle was used to penetrate 5 mm percutaneously into the dorsal center on Co 7/8 and Co 8/9. The needle was rotated 360° and removed after staying for 30 s. The surgical area was disinfected again to avoid infection.

To determine whether the modeling was successful, a magnetic resonance imaging (MRI) examination was conducted after 2 weeks. The degenerative discs were orthotopically injected with PBS (2 μL), IGK (2 μL, 20 μM), SeNP (2 μL, 60 μg/mL), or IGK@SeNP (2 μL, 60 μg/mL) using a 33G needle.

Radiology evaluation

X-rays and MRI were performed at 4 and 8 weeks after IDD construction. The anesthetized rats were placed supine and the tails were straightened. The intervertebral heights were measured by image J on X-ray images. A 1.5 T MRI scanner was used to acquire the intervertebral disc signals on T2 weighted phase. Further, the severity of IDD was assessed according to the modified Pfirrmann grading system [47]

Histological analysis

The rats were sacrificed by injecting over a dose of pentobarbital sodium at 4 weeks or 8 weeks. Intervertebral discs were harvested under aseptic conditions and fixed in 4% paraformaldehyde for 24 h. After decalcification by 10% EDTA for 2 weeks, the discs were sliced into 4 μm thick sections. Hematoxylin–eosin (HE), safranin O-fast green (SF), immunochemical (IHC), and IF staining were performed according to the manufacturer’s instructions [48, 49]. The morphology of intervertebral discs was observed under a light microscope and determined the histological grade [50].

Statistical analysis

All statistical analyses were conducted with SPS software version 26.0 (IBM SPSS Corp. Chicago, USA). Data were presented as mean ± standard deviations (SD). Student’s t-test or one-way analysis of variance (ANOVA) was used to evaluate the differences among various treatment groups. P < 0.05 was considered statistically significant. (*, †, and # denoted P < 0.05).

The datasets generated and/or analyzed during the current study are not publicly available but are available from the corresponding author on reasonable request.

IDD:

Intervertebral disc degeneration

ECM:

Extracellular matrix

NPCs:

Nucleus pulposus cells

IGK:

Isoginkgetin

CQ:

Chloroquine

Cy5:

Cyanine5

ROS:

Reactive oxygen species

H₂O₂ :

Hydrogen peroxide

SeNP:

Diselenide-containing nanoparticles

IGK@SeNP:

Isoginkgetin-loaded diselenide-containing nanoparticles

Se-polymer:

Diselenide-containing polymer

IPDI:

Diisocyanate

DBTDL:

Dibutyltin dilaurate

mPEG:

Methoxypolyethylene glycol (mPEG)

THF:

Tetrahydrofuran

PBS:

Phosphate-buffered saline

FBS:

Fetal bovine serum

EDTA:

Ethylene diamine tetraacetic acid

TEM:

Transmission electron microscopy

DLS:

Dynamic light scattering

gMFI:

Geometric mean fluorescence intensity

COL2:

Collagen II

SOX9:

Sex-determining region Y-type high mobility group box protein 9;

ACAN:

Aggrecan

MMP3:

Matrix metalloproteinases 3

MMP13:

Matrix metalloproteinases 13

ADAMTS5:

A disintegrin and metalloproteinase with thrombospondin motifs 5

BCL2:

B-cell lymphoma 2

BAX:

BCL2 associated X

CASP3:

Caspase 3

ATG7:

Autophagy related 7

BECN1:

Beclin 1

LC3:

Microtubule associated protein 1 light chain 3

SQSTM1/p62:

Sequestosome 1

CCK8:

Cell counting kit-8

TUNEL:

Terminal-deoxynucleoitidyl transferase mediated nick end labeling

MRI:

Magnetic resonance imaging

HE:

Hematoxylin–eosin

SF:

O-fast green

IF:

Immunofluorescence

IHC:

Immunochemistry

Not applicable.

This work was supported by the National Natural Science Foundation of China [Grant Number 82172506].

1. Hao Yu and Yun Teng are contributed equally to this article

Authors and Affiliations

1. Department of Orthopaedic Surgery, The First Affiliated Hospital of Soochow University, 188 Shizi St., Suzhou, 215006, Jiangsu, China

   Hao Yu, Yun Teng, Jun Ge, Ming Yang, Haifeng Xie, Tianyi Wu, Qi Yan & Jun Zou

2. Department of Nephrology, The First Affiliated Hospital of Soochow University, 188 Shizi St., Suzhou, 215006, Jiangsu, China

   Mengting Jia, Qing Zhu & Yanping Shen

3. College of Life Sciences, Zhejiang University, 866 Yuhangtang Rd., Hangzhou, 310027, Zhejiang, China

   Lianxue Zhang

Contributions

JZ, LZ, and YS designed the experiments. LZ and HY synthesized the material and performed characterization. HY, YT performed the cellular studies and analyzed data. HY, YT, JG, MY, HX, and TW built the animal model and were responsible for animal experiments. QY, MJ, and QZ helped with various experiments. HY, YT, and YS co-wrote the paper. JZ provided funding support and YS supervised the experiments. All authors read and approved the final manuscript.

Corresponding authors

Correspondence to Yanping Shen, Lianxue Zhang or Jun Zou.

Ethics approval and consent to participate

The study was approved by Ethics Committee of Soochow University, all methods were carried out in accordance with relevant guidelines and regulations. This study was carried out in compliance with the ARRIVE guidelines.

Consent for publication

Not applicable.

Competing interests

The authors declare that they have no competing interests.

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