Intisar Aseer, Kim Woon-Hae, Shin Hyun Young, Kim Min Young, Kim Yu Seon, Lim Heejin, Kang Hyun Gyu, Mo Yun Jeoung, Aly Mohamed Aly Saad, Lee Yun-Il, Kim Minseok S
Department of New Biology, DGIST, Daegu 42988, Republic of Korea.
CTCELLS Corp., Daegu 42988, Republic of Korea.
Biofabrication. 2022 Jan 6;14(1). doi: 10.1088/1758-5090/ac457c.
As the myelin sheath is crucial for neuronal saltatory conduction, loss of myelin in the peripheral nervous system (PNS) leads to demyelinating neuropathies causing muscular atrophy, numbness, foot deformities and paralysis. Unfortunately, few interventions are available for such neuropathies, because previous pharmaceuticals have shown severe side effects and failed in clinical trials. Therefore, exploring new strategies to enhance PNS myelination is critical to provide solution for such intractable diseases. This study aimed to investigate the effectiveness of electrical stimulation (ES) to enhance myelination in the mouse dorsal root ganglion (DRG)-anmodel of the PNS. Mouse embryonic DRGs were extracted at E13 and seeded onto Matrigel-coated surfaces. After sufficient growth and differentiation, screening was carried out by applying ES in the 1-100 Hz range at the beginning of the myelination process. DRG myelination was evaluated via immunostaining at the intermediate (19 days(DIV)) and mature (30 DIV) stages. Further biochemical analyses were carried out by utilizing ribonucleic acid sequencing, quantitative polymerase chain reaction and biochemical assays at both intermediate and mature myelination stages. Imaging of DRG myelin lipids was carried out via time-of-flight secondary ion mass spectrometry (ToF-SIMS). With screening ES conditions, optimal condition was identified at 20 Hz, which enhanced the percentage of myelinated neurons and average myelin length not only at intermediate (129% and 61%) but also at mature (72% and 17%) myelination stages. Further biochemical analyses elucidated that ES promoted lipid biosynthesis in the DRG. ToF-SIMS imaging showed higher abundance of the structural lipids, cholesterol and sphingomyelin, in the myelin membrane. Therefore, promotion of lipid biosynthesis and higher abundance of myelin lipids led to ES-mediated myelination enhancement. Given that myelin lipid deficiency is culpable for most demyelinating PNS neuropathies, the results might pave a new way to treat such diseases via electroceuticals.
由于髓鞘对于神经元的跳跃式传导至关重要,外周神经系统(PNS)中髓鞘的丧失会导致脱髓鞘性神经病变,进而引起肌肉萎缩、麻木、足部畸形和瘫痪。不幸的是,针对此类神经病变的干预措施很少,因为先前的药物已显示出严重的副作用且在临床试验中失败。因此,探索增强PNS髓鞘形成的新策略对于解决此类难治性疾病至关重要。本研究旨在调查电刺激(ES)增强小鼠背根神经节(DRG)(一种PNS模型)髓鞘形成的有效性。在胚胎第13天提取小鼠胚胎DRG,并接种到基质胶包被的表面。在充分生长和分化后,在髓鞘形成过程开始时通过施加1-100Hz范围内的ES进行筛选。通过免疫染色在中间阶段(第19天(DIV))和成熟阶段(第30天DIV)评估DRG髓鞘形成。在中间和成熟髓鞘形成阶段,通过核糖核酸测序、定量聚合酶链反应和生化分析进行进一步的生化分析。通过飞行时间二次离子质谱(ToF-SIMS)对DRG髓鞘脂质进行成像。通过筛选ES条件,确定最佳条件为20Hz,这不仅在中间(129%和61%)而且在成熟(72%和17%)髓鞘形成阶段提高了有髓神经元的百分比和平均髓鞘长度。进一步的生化分析表明,ES促进了DRG中的脂质生物合成。ToF-SIMS成像显示髓鞘膜中结构脂质、胆固醇和鞘磷脂的丰度更高。因此,脂质生物合成的促进和髓鞘脂质的更高丰度导致了ES介导的髓鞘形成增强。鉴于髓鞘脂质缺乏是大多数脱髓鞘性PNS神经病变的原因,这些结果可能为通过电疗治疗此类疾病开辟一条新途径。
