Multichannel 3D-Printed Bioactive Scaffold Combined with Small Interfering RNA Delivery to Promote Neurological Recovery after Spinal Cord Injury

Spinal Cord Injury (SCI) is a devastating neurological disorder that often leads to permanent neural dysfunction. Current treatments fail to address the core challenges of insufficient intrinsic axonal regeneration, lack of directional guidance, and an inhibitory pathological microenvironment. There is an urgent need for synergistic therapeutic strategies that integrate structural support, molecular regulation, and microenvironment optimization to achieve effective neural function recovery.

Now, a joint research team from Zhejiang University and Fuzhou University has developed a collaborative treatment platform combining a multichannel 3D-printed bioactive scaffold with a small interfering RNA (siRNA) delivery system. This innovative approach simultaneously provides physical guidance, improves the inhibitory microenvironment, and activates the intrinsic regenerative capacity of neurons. In animal experiments, the combined therapy significantly enhanced long-distance parallel axon regeneration, promoted myelination and synaptic formation, and remarkably improved hindlimb motor function in SCI rats, with BBB scores significantly higher than other treatment groups from the 6th week post-surgery.

"The treatment of spinal cord injury has long been limited by the inability of single strategies to tackle multiple pathological barriers," said corresponding author Dr. Wei Wei, a professor at Zhejiang University. "Our integrated platform merges physical cues, biological signaling, and microenvironment regulation, offering a promising solution to overcome the bottlenecks in SCI therapy and advancing the translation from basic research to clinical application."

Jin Zhang, a professor at Fuzhou University and co-corresponding author, added: "The precision 3D-printed scaffold, functional hydrogel, and siRNA delivery system work synergistically to reconstruct neural circuits. This design not only enhances axonal regeneration but also ensures functional integration, laying a solid foundation for future clinical transformation."

Synergistic Triple-Function Design
The research team integrated three core functions into a single therapeutic system through innovative design:
1. A high-precision 3D-printed GM-PEGDA scaffold with parallel channels provides clear "growth paths" for axon regeneration, matching the structural characteristics of spinal cord conduction bundles.
2. GM-RA4IV bioactive hydrogel filled in the channels mimics the natural extracellular matrix, delivers neurotrophic support, and regulates the immune microenvironment by inhibiting the activation of harmful M1 macrophages.
3. siRNA-loaded lipid nanoparticles (siRNA@LNPs) efficiently knock down the PTEN gene, activate the mTOR signaling pathway, and significantly enhance the intrinsic regenerative potential of neurons.

The GM-RA4IV hydrogel exhibits excellent physical properties, including rapid gelation within 10 seconds under UV irradiation, a porous structure with an average pore size of 16.44 ± 4.03 μm, and stable mechanical strength (284.67 ± 12.83 Pa). It maintains structural integrity in vivo for approximately one month, providing long-term support for axon regeneration. Immunofluorescence analysis confirmed that the combined therapy induced axons to regenerate in a long-distance, parallel manner with an average projection angle of only 9.67° ± 6.82°, and the number of regenerated axons doubled compared to control groups.

Research Significance and Future Outlook
This study marks a critical advancement in SCI treatment by pioneering the integration of multichannel 3D-printed bioactive scaffolds, laminin-derived peptide hydrogels, and PTEN-targeted siRNA delivery—breaking the limitations of traditional single-target strategies. By simultaneously resolving the three core bottlenecks (insufficient intrinsic axonal regeneration, lack of directional guidance, and inhibitory microenvironment), it realizes the synergistic effect of physical support, molecular regulation, and microenvironment optimization. Moreover, the research identifies the key role of the Ephrin/Eph signaling pathway in guiding parallel axon regeneration, deepening the understanding of molecular mechanisms underlying SCI repair and opening new avenues for targeted therapy research. The GM-RA4IV hydrogel’s favorable properties (appropriate mechanical strength, low swelling rate, controllable degradability), the 3D-printed scaffold’s structural compatibility with spinal cord tracts, and the siRNA delivery system’s high efficiency and low toxicity collectively lay a robust material and technical foundation for clinical translation, bridging the gap between basic SCI research and clinical application.

For future development, the team plans to expand the therapeutic platform’s clinical translation scenarios: validating its efficacy in more clinically relevant models, such as chronic SCI cases, complete spinal cord transection models (simulating severe injuries), and large animal models. Additionally, efforts will focus on optimizing intervention timing and surgical delivery methods, addressing practical challenges like large-scale production and long-term implantation stability to advance the strategy from rat experiments to human clinical trials. The team also intends to explore combinations of this integrated platform with other therapies—such as stem cell treatment, electrical stimulation, and organoids—to strengthen "axon highway-pathway network" construction and further improve neural circuit regeneration outcomes.

The complete study is accessible via DOI:10.34133/research.0951

https://spj.science.org/doi/10.34133/research.0951

Title: Multichannel 3D-Printed Bioactive Scaffold Combined with Small Interfering RNA Delivery to Promote Neurological Recovery after Spinal Cord Injury
Authors: JINGJIA YE, FENGLU LI, ZHENGFA WEN, JUNSHENG HE, GAOXING PAN, XINRANG ZHAI, LINRAN SONG, XIANZHU ZHANG, XUEFEI ZHOU, XUDONG YAO, YANLANG WANG, JIN ZHANG , AND WEI WEI
Journal: 21 Oct 2025 Vol 8 Article ID: 0951
DOI:10.34133/research.0951

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Fig. 1. Schematic illustration showing fabrication of 3D-printed multi-channel scaffold incorporated with siRNA delivery system as well as their promotion effect on axonal regeneration for SCI.
Fig. 2. Basic physical properties of GM-RA4IV hydrogel. (A) Fabrication of GM-RA4IV hydrogel. (B) Sol–gel transition of GM-RA4IV after UV exposure. (C) SEM images and pore-size distributions of GM and GM-RA4IV hydrogels. (D) Average pore diameter based on SEM images (n = 3). (E) Rheological properties of GM-RA4IV solution upon UV-initiated polymerization. (F) Frequency sweep measurement of GM-RA4IV hydrogel. (G) Compressive stress–strain curves of GM and GM-RA4IV hydrogels. (H) Swelling and (I) degradation ratios of GM and GM-RA4IV hydrogels during 2 months in vitro (n = 3). (J) Fluorescence images and (K) quantification of region of interest (ROI) of GM and GM-RA4IV hydrogels about degradation during a period of 1 month in vivo (n = 3). Images in same roll were from same animal. All statistical data are represented as mean ± SD (*P < 0.05, **P < 0.01, ***P < 0.001). T test was used in (D), (H), (I), and (K).
Fig. 3. Biocompatibility and axonal outgrowth in vitro. (A) Live/Dead staining images and (B) quantification of viability of PC12 cells cocultured with PLL, GM-PEGDA, and GM-RA4IV hydrogels for 24 h (n = 3). (C) Tuj-1 immune staining images of DRG neurons cocultured with PLL-, GM-PEGDA-, and GM-RA4IV-coated plates for 24 h. (D) OD values of DRG neurons incubated in 3 conditions (n = 3). (E) Observation of DRG neurons grown in GM-PEGDA and GM-RA4IV half-coated plate. (F) Representative images of axonal extension of DRG neurons cocultured with PLL, Gel-PEGDA, and GM-RA4IV coating plates for 5 d. Quantitative analysis of (G) maximum branch numbers and (I) average length of axon branches in different conditions (n = 18). (H) Quantification of branch number of axons in different lengths (n = 3). All statistical data are represented as mean ± SD (**P < 0.01). One-way ANOVA followed by Tukey’s test was used in (D), (H), and (I).
Fig. 4. GM-RA4IV hydrogel protected residual tissue and promoted axon regeneration in vivo. (A) Experimental timeline. (B) Preparation of longitudinal slices. (C) Optical and H&E staining images of injured spinal cord after 8 weeks. Red and yellow dotted lines indicate edges of spinal tissue and damaged sites, respectively. (D) Representative immunofluorescence staining and magnified images of sagittal sections for GFAP (green)- and AAV2/9-mCherry (red)-traced axons under different conditions after 8 weeks. White dotted lines indicate edges of SCI, and yellow pentagons represent enlarged position. Immunofluorescence staining images of (E) CD68 and (F) Iba1 in 3 groups at 8 weeks post-injury. (G) Quantitative analysis of cavity areas in Ctrl, GM-PEGDA, and GM-RA4IV groups (n = 7). (H) Quantification of axon number at injury site per mm2 (n = 5). Fluorescence intensities of (I) CD68 and (J) Iba1 per area in different groups (n = 5). All statistical data are represented as mean ± SD (**P < 0.01). One-way ANOVA followed by Tukey’s test was used in (G) to (J).
Fig. 5. siRNA@LNPs down-regulated expression level of PTEN and improved axon extension in vitro and in vivo. (A) Particle size and (B) zeta potential of LNPs and siRNA@LNPs. (C) Encapsulation ratio of siRNA (n = 3). (D) Relative expression level of PTEN in Ctrl, LNPs, and siRNA@LNPs groups (n = 3). (E) OD values of DRG neurons cocultured in 3 conditions for 24 h after siRNA transfection (n = 3). (F) Tuj-1 staining images of DRG neurons in different conditions. (G) Percentage of long axon branches over 1,000 μm quantified dependent on Tuj-1 staining images (n = 3). (H) Branch numbers of different lengths ranging from 0 to 3,500 μm for 3 conditions. (I) Fluorescence signals of siRNA delivery in Intact and siRNA@LNPs groups. Images on the right are magnified version of yellow quadrilateral on the left. (J) Western blot analyses presenting expression level of PTEN at 2 weeks after siRNA@LNPs injection (n = 3). (K) Quantification of expression level of PTEN based on Western blotting images (n = 3). (L) Representative image of axonal regeneration in the siRNA@LNPs + GM-RA4IV group at 8 weeks post-injury. All statistical data are represented as mean ± SD (*P < 0.05, **P < 0.01). One-way ANOVA followed by Tukey’s test was used in (D), (G), and (K).
Fig. 6. siRNA@LNPs + GM-3Dpro group reconstructed spinal cord circuits and promoted hind-limb locomotion function recovery of rats. (A) Schematic diagram of GM-3Dpro scaffold preparation and partial physical image. (B) EMG recording of TA and GS muscles and (C) color-coded stick views of kinematic hind-limb movement of Intact, Ctrl, GM-PEGDA-treated, GM-RA4IV-treated, and siRNA@LNPs + GM-3Dpro-treated groups. Quantitative analysis of (D) body weight support, (E) stride length, and (F) BBB scores weekly of 5 groups (n = 5). (G) Quantification of maximum angle variations of hip, knee, and ankle movements in free-walking animals (n = 5). (H) Correlation matrix of hip, knee, ankle movement, axon number, and axon projection orientation in Intact, Ctrl, GM-RA4IV, and siRNA@LNPs + GM-3Dpro groups. All statistical data are represented as mean ± SD (*P < 0.05, **P < 0.01). One-way ANOVA followed by Tukey’s test was used in (D) to (G).
Fig. 7. siRNA@LNPs + GM-3Dpro group induced parallel oriented axons regeneration in vivo. (A) AAV2/9-mCherry-traced axons and MBP (magenta)-/synaptophysin (green)-stained sagittal sections in the siRNA@LNPs + GM-3Dpro group. Enlarged images present longitudinally projected axons in (A1) long-distance and (A2) locally parallel projected axons. White arrow represents direction of axon extension. (B) Representative images of DAPI (blue), GFAP (green), 5-HT (red), and NF200 (magenta) at 12 weeks in the siRNA@LNPs + GM-3Dpro group. Right panels present higher magnifications of areas within white rectangles in left panels (B1 to B3), and white dashed lines present damaged areas. Quantification of (C) projection angle and (D) number of axons in GM-RA4IV, siRNA@LNPs + GM-RA4IV, and siRNA@LNPs + GM-3Dpro groups (n = 5). Quantitative analysis of (E) 5-HT+ and (F) NF200+ axon numbers per mm2 in 4 conditions (n = 6). All statistical data are represented as mean ± SD (*P < 0.05, **P < 0.01, ***P < 0.001). One-way ANOVA followed by Tukey’s test was used in (C) to (F).
Fig. 8. SC-RNA-seq analyses revealed mechanism of parallel orientation of regenerated axons in the siRNA@LNPs + GM-3Dpro group. (A) UMAP visualization of all cell types combined from Ctrl, GM-RA4IV, and siRNA@LNPs + GM-3Dpro based on DEGs. (B) Heatmap presented DEGs in different cell types. (C) Cell−cell connection between 9 cell types corresponding to different pathways and divided 5 patterns presented by river plotting. (D) GO enrichment by DEGs between Ctrl and siRNA@LNPs + GM-3Dpro groups at BP, CC, and MF. (E) UMAP visualization of 5 subclusters in neuron based on DEGs. (F) Cell differentiation trajectory in neuron subpopulation determined by pseudotime analysis (upper: differentiation trajectory of neuron subpopulations; down: differentiation trajectory presented by pseudotime). Circle number 1 and 2 indicated bifurcation of differentiation trajectory. (G) Expressions of Ephb1 and Epha3 to Epha7 in different neuron subpopulations.

01/12/2025 Science and Technology Review Publishing House

Regions: Asia, China

Keywords: Health, Medical, People in health research, Science, Life Sciences

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