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The effect of cobalt chrome and stainless steel particles generated by Total Disc Replacements on the viability of cells of the CNS

机译:全椎间盘置换术产生的钴铬和不锈钢颗粒对中枢神经系统细胞活力的影响

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Introduction: Degeneration of the intervertebral disc causes significant pain to patients, surgical interventions include spinal fusion or total disc replacement (TDR). Fusion procedures reduce spinal mobility and are commonly associated with adjacent level effects (hastened degeneration of the functional spinal unit neighbouring the immobilized region). Devices aiming to preserve the spinal motion, in particular metal on metal TDR's have been introduced clinically. There is a growing concern regarding wear of these devices and the adverse biological effects this will have on the spinal cord. There is evidence that nanoscale metallic debris may breach the meninges, the protective barrier around the cord, and could lead to pseudotumor formation, potentially impinging upon and altering the functionality of the cord. This study aims to understand the toxicity of cobalt chrome and stainless steel wear debris and ions to cells of the CNS. Materials and Methods: A six-station pin on plate wear rig was used to generate clinically relevant cobalt chrome (CoCr) and stainless steel wear debris which was similar in size and morphology to that generated by Metal on Metal Cervical Total Disc Replacements.To determine the effect of these metal particles on the viability of CNS cells a 3D collagen hydrogel seeded with primary astrocytes and microglia in co-culture (isolated from the cortex of P2 rat pups) and astrocytes in isolation (microglia shaken off) were used. The cells were dosed with increasing particle volumes; 0.5-50μm~3 debris per cell for 28 hours and 5 days. The particle doses were selected based on MOM TDR wear rates and scaled down accordingly. The effect on viability was determined using a Live Dead assay. A comet assay was used to determine the effect of metallic wear particles on the integrity of primary astrocyte and microglia DNA after 48 hours and 5 days in culture. Results and Discussion: A significant reduction in viability was observed after 48 hours when primary astrocytes were cultured in 3D with the highest particle dose of CoCr (50μm~3 debris per cell). After 5 days in culture a significant reduction in viability was observed at the highest particle dose and the mid dose of 5μm~3 CoCr debris per cell (Figure 1). Similar results were seen when astrocytes and microglia were cultured with CoCr debris.vSignificant effects on viability were not observed when primary astrocytes were cultured with stainless steel wear particles, at any volume dose. A significant reduction in viability was seen when primary astrocytes in isolation were cultured with cobalt chrome ions from the 50μm3 and 5μm3 particle doses for 48 hours and 5 days. No significant effects on viability were observed when primary astrocytes with microglia were cultured with cobalt chrome ions or on any cells with stainless steel ions. Interestingly similar levels of DNA damage were seen between the two biomaterials when primary astrocytes and microglia in co-culture and in isolation were cultured with metallic wear debris. Conclusion: The two different biomaterials have differing effects in the viability of primary astrocytes and microglia in co-culture and astrocytes in isolation. As these materials are introduced into relatively young patients and the wear debris has potential to build up and disseminate throughout the body over long periods of time additional research is necessary to further understand the response of the body to metal particles.
机译:简介:椎间盘退变会给患者带来严重的疼痛,外科手术包括脊柱融合术或全椎间盘置换术(TDR)。融合手术会降低脊柱活动度,并且通常与邻近的水平效应(邻近固定区域的功能性脊柱单位的退化持续)相关。临床上已经引入了旨在保持脊柱运动的设备,尤其是金属TDR上的金属。这些设备的磨损及其对脊髓的不利生物学影响越来越引起人们的关注。有证据表明,纳米级金属碎片可能会破坏脑膜,即脐带周围的保护性屏障,并可能导致假瘤的形成,从而可能影响并改变脐带的功能。这项研究旨在了解钴铬和不锈钢磨损碎片和离子对中枢神经系统细胞的毒性。材料和方法:使用六工位销钉在平板磨机上产生临床相关的钴铬合金(CoCr)和不锈钢磨屑,其大小和形态与金属颈椎间盘全金属置换术产生的相似。这些金属颗粒对CNS细胞生存力的影响使用共培养的原代星形胶质细胞和小胶质细胞(从P2大鼠幼崽的皮层分离)接种的3D胶原水凝胶和分离的星形胶质细胞(摇动的小胶质细胞)使用。给细胞增加颗粒体积。每格0.5-50μm〜3碎片,持续28小时5天。基于MOM TDR磨损率选择颗粒剂量,并相应地按比例缩小。使用活死测定法确定对生存力的影响。在培养48小时和5天后,使用彗星试验确定金属磨损颗粒对原代星形胶质细胞和小胶质细胞DNA完整性的影响。结果与讨论:48小时后,当原始星形胶质细胞以最高剂量的CoCr(每个细胞50μm〜3碎片)进行3D培养时,观察到活力显着降低。培养5天后,在每个细胞的最高颗粒剂量和5μm〜3 CoCr碎片的中等剂量下,观察到活力显着降低(图1)。当用CoCr碎片培养星形胶质细胞和小胶质细胞时,观察到相似的结果。v当用任何体积剂量的不锈钢磨损颗粒培养原代星形胶质细胞时,未观察到对生存力的显着影响。当分离的原代星形胶质细胞与来自50μm3和5μm3剂量的钴铬离子一起培养48小时和5天时,发现活力显着降低。当用钴铬离子培养小胶质细胞原代星形胶质细胞或用不锈钢离子培养任何星形胶质细胞时,均未观察到对存活率的显着影响。有趣的是,当将原代星形胶质细胞和小胶质细胞共培养和单独培养时,用金属磨损碎片培养时,两种生物材料之间的DNA损伤水平相似。结论:两种不同的生物材料对原代星形胶质细胞和小胶质细胞共培养以及分离的星形胶质细胞的生存能力有不同的影响。随着这些材料被引入相对年轻的患者中,磨损碎片可能会在很长一段时间内积聚并散布到全身,这需要进一步的研究来进一步了解人体对金属颗粒的反应。

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