首页> 美国卫生研究院文献>Journal of Biomechanical Engineering >Effects of Cryopreservation on the Depth-Dependent Elastic Modulus in Articular Cartilage and Implications for Osteochondral Grafting
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Effects of Cryopreservation on the Depth-Dependent Elastic Modulus in Articular Cartilage and Implications for Osteochondral Grafting

机译:冷冻保存对关节软骨深度依赖性弹性模量的影响及其对骨软骨移植的影响

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摘要

Cryopreservation of articular cartilage is often used in storage of experimental samples and osteochondral grafts, but the depth-dependence and concentration of glycosaminoglycan (GAG) are significantly altered when cryogenically stored without a cryoprotectant, which will reduce cartilage stiffness and affect osteochondral graft function and long-term viability. This study investigates our ability to detect changes due to cryopreservation in the depth-dependent elastic modulus of osteochondral samples. Using a direct-visualization method requiring minimal histological alterations, unconfined stepwise stress relaxation tests were performed on four fresh (never frozen) and three cryopreserved (−20 °C) canine humeral head osteochondral slices 125 ± 5 μm thick. Applied force was measured and tissue images were taken at the end of each relaxation phase using a 4× objective. Intratissue displacements were calculated by tracking chondrocytes through consecutive images for various intratissue depths. The depth-dependent elastic modulus was compared between fresh and cryopreserved tissue for same-depth ranges using analysis of variance (ANOVA) with Tukey post-test with a 95% confidence interval. Cryopreservation was found to significantly alter the force–displacement profile and reduce the depth-dependent modulus of articular cartilage. Excessive collagen fiber folding occurred at 40–60% relative depth, producing a “black line” in cryopreserved tissue. Force–displacement curves exhibited elongated toe-region in cryopreserved tissue while fresh tissue had nonmeasurable toe-region. Statistical analysis showed significant reduction in the elastic modulus and GAG concentration throughout the tissue between same-depth ranges. This method of cryopreservation significantly reduces the depth-dependent modulus of canine humeral osteochondral samples.
机译:低温保存关节软骨常用于实验样品和骨软骨移植,但是在没有冷冻保护剂的情况下低温保存时,糖胺聚糖(GAG)的深度依赖性和浓度会显着改变,这将降低软骨的硬度并影响软骨移植物的功能和长期保存。长期生存力。这项研究调查了我们检测冷冻保存骨软骨样品的深度依赖性弹性模量变化的能力。采用要求最小的组织学改变的直接可视化方法,对四个新鲜的(从未冷冻过的)和三个冷冻保存的(-20°C)犬肱骨头的骨软骨切片,厚度为125±5μm,进行了无限制的逐步应力松弛测试。测量了施加的力,并在每个弛豫阶段结束时使用4倍物镜拍摄了组织图像。通过跟踪软骨细胞通过连续图像获得各种组织内深度来计算组织内位移。使用方差分析(ANOVA)和具有95%置信区间的Tukey后测,对新鲜和冷冻组织在相同深度范围内的深度相关弹性模量进行比较。发现冷冻保存可显着改变力-位移曲线并降低关节软骨的深度依赖性模量。胶原纤维过度折叠发生在相对深度40–60%处,在冷冻保存的组织中产生“黑线”。力-位移曲线在冷冻保存的组织中显示出伸长的脚趾区域,而新鲜组织的脚趾区域却无法测量。统计分析表明,在相同深度范围内,整个组织的弹性模量和GAG浓度均显着降低。这种冷冻保存方法显着降低了犬肱骨骨软骨样品的深度依赖性模量。

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