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Microglial SLC25A28 Knockout Mitigates Spinal Cord Injury in Mice by Inhibiting Heme Synthesis and Subsequent NOX2 Activation

作者
Huangtao Chen,Shaochun Guo,Yan‐jun Mi,Ruili Han,Yuxin Xi,Tingwei Peng,Longhui Fu,Weidong Liu,Ruiyu Ma,Beibei Yu,Yongfeng Zhang,Luyao Li,Jing Ye,Shouping Gong
出处
期刊:CNS Neuroscience & Therapeutics [Wiley]
卷期号:31 (11): e70638-e70638
标识
DOI:10.1111/cns.70638
摘要

ABSTRACT Background Microglial overactivation‐driven neuroinflammation exacerbates secondary damage after spinal cord injury (SCI), but the role of mitochondrial iron metabolism in this process is not well understood. This study investigates the function of the mitochondrial iron transporter solute carrier family 25 member 28 (SLC25A28) in post‐SCI neuroinflammation. Methods Microglia‐specific SLC25A28 knockout (A28‐MGKO) mice were generated by crossing SLC25A28 flox/flox mice with Cx3cr1‐CreERT2 mice and subjected to clip‐compression spinal cord injury (SCI) at the T9 level. Motor recovery was evaluated using the Basso Mouse Scale (BMS), while histological and biochemical assessments including hematoxylin–eosin and Nissl staining, Iba1 immunohistochemistry, Evans blue permeability, and tissue water content were performed to evaluate lesion severity, neuronal survival, microglial activation, and blood–spinal cord barrier integrity. In vitro, primary microglia isolated from A28‐MGKO mice and BV2 cells with SLC25A28 overexpression were used to investigate mitochondrial iron homeostasis, heme biosynthesis, and NOX2‐mediated oxidative stress. Mitochondrial iron content was quantified using a ferrozine‐based assay and Mito‐FerroGreen staining, while ROS production, cytokine release, and inflammatory signaling were analyzed by fluorescence imaging, ELISA, and Western blotting under pharmacological modulation of heme synthesis and NOX2 activity. Results We found that SLC25A28 deficiency reduced spinal cord edema, blood‐spinal cord barrier disruption, and motor deficits. Mechanistically, SLC25A28 knockout suppressed mitochondrial iron accumulation, inhibited heme synthesis, and reduced NOX2‐mediated oxidative stress. However, SLC25A28 overexpression enhanced mitochondrial iron overload and NOX2‐driven inflammation, which could be reversed by pharmacological blockade of NOX2 or heme synthesis. Restoration of heme synthesis in A28‐MGKO microglia attenuated the anti‐inflammatory effects of SLC25A28 knockout. Conclusion These findings demonstrate that microglial SLC25A28 regulates neuroinflammation and functional recovery after SCI by promoting mitochondrial iron‐dependent heme synthesis and NOX2 activation. Targeting the SLC25A28–heme–NOX2 axis may provide a novel therapeutic approach for SCI.
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