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Guidance for Removal of Fetal Bovine Serum from Cryopreserved Heart Valve Processing

机译:从冷冻保存的心脏瓣膜处理中去除胎牛血清的指南

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摘要

Bovine serum is commonly used in cryopreservation of allogeneic heart valves; however, bovine serum carries a risk of product adulteration by contamination with bovine-derived infectious agents. In this study, we compared fresh and cryopreserved porcine valves that were processed by 1 of 4 cryopreservation formulations, 3 of which were serum-free and 1 that utilized bovine serum with 1.4 M dimethylsulfoxide. In the first serum-free group, bovine serum was simply removed from the cryopreservation formulation. The second serum-free formulation had a higher cryoprotectant concentration, i.e. 2 M dimethylsulfoxide, in combination with a serum-free solution. A colloid, dextran 40, was added to the third serum-free group with 2 M dimethylsulfoxide due to theoretical concerns that removal of serum might increase the incidence of tissue cracking. Upon rewarming, the valves were inspected and subjected to a battery of tests. Gross pathology revealed conduit cracking in 1 of 98 frozen heart valves. Viability data for the cryopreserved groups versus the fresh group demonstrated a loss of viability in half of the comparisons (p < 0.05). No significant differences were observed between any of the cryopreserved groups, with or without bovine serum. Neither routine histology, autofluorescence-based multiphoton imaging nor semiquantitative second-harmonic generation microscopy of extracellular matrix components revealed any statistically significant differences. Biomechanics analyses also revealed no significant differences. Our results demonstrate that bovine serum can be safely removed from heart valve processing and that a colloid to prevent cracking was not required. This study provides guidance for the assessment of changes in cryopreservation procedures for tissues.
机译:牛血清常用于同种异体心脏瓣膜的冷冻保存中。但是,牛血清会受到牛源性传染病菌的污染而导致产品掺假的风险。在这项研究中,我们比较了由4种冷冻保存配方中的1种处理过的新鲜和低温保存的猪瓣膜,其中3种无血清,1种使用牛血清与1.4 M二甲基亚砜。在第一个无血清组中,仅从冷冻保存制剂中除去牛血清。第二种无血清制剂与无血清溶液组合具有较高的冷冻保护剂浓度,即2M二甲基亚砜。由于理论上担心去除血清可能会增加组织破裂的发生率,因此将胶体右旋糖酐40与2 M二甲基亚砜一起加入了第三个无血清组。重新加热后,检查阀门并进行一系列测试。大体病理显示98个冰冻的心脏瓣膜中有1个出现导管破裂。冷藏组与新鲜组的生存力数据表明,在一半的比较中,生存力下降(p <0.05)。在有或没有牛血清的任何冷冻保存组之间均未观察到显着差异。常规组织学,基于自发荧光的多光子成像或细胞外基质成分的半定量二次谐波生成显微镜均未显示任何统计学上的显着差异。生物力学分析也没有发现显着差异。我们的结果表明,牛血清可以安全地从心脏瓣膜处理中去除,不需要胶体来防止破裂。这项研究为评估组织冷冻保存程序的变化提供了指导。

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