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Optimized decellularization protocol including α-Gal epitope reduction for fabrication of an acellular porcine annulus fibrosus scaffold

机译:优化的脱细胞方案包括α-Gal表位还原用于制备脱细胞猪纤维环支架

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摘要

Recent advances in tissue engineering have led to potential new strategies, especially decellularization protocols from natural tissues, for the repair, replacement, and regeneration of intervertebral discs. This study aimed to validate our previously reported method for the decellularization of annulus fibrosus (AF) tissue and to quantify potentially antigenic α-Gal epitopes in the decellularized tissue. Porcine AF tissue was decellularized using different freeze–thaw temperatures, chemical detergents, and incubation times in order to determine the optimal method for cell removal. The integrity of the decellularized material was determined using biochemical and mechanical tests. The α-Gal epitope was quantified before and after decellularization. Decellularization with freeze–thaw in liquid nitrogen, an ionic detergent (0.1% SDS), and a 24 h incubation period yielded the greatest retention of GAG and collagen relative to DNA reduction when tested as single variables. Combined, these optimal decellularization conditions preserved more GAG while removing the same amount of DNA as the conditions used in our previous study. Components and biomechanical properties of the AF matrix were retained. The decellularized AF scaffold exhibited suitable immune-compatibility, as evidenced by successful in vivo remodeling and a decrease in the α-Gal epitope. Our study defined the optimal conditions for decellularization of porcine AF tissues while preserving the biological composition and mechanical properties of the scaffold. Under these conditions, immunocompatibility was evidenced by successful in vivo remodeling and reduction of the α-Gal epitope in the decellularized material. Decellularized AF scaffolds are potential candidates for clinical applications in spinal surgery.
机译:组织工程学的最新进展已导致潜在的新策略,尤其是天然组织的脱细胞方案,用于修复,置换和再生椎间盘。这项研究旨在验证我们先前报道的纤维环(AF)组织脱细胞方法,并量化脱细胞组织中潜在的抗原性α-Gal表位。使用不同的冻融温度,化学去污剂和孵育时间对猪房颤组织进行脱细胞,以确定最佳的细胞去除方法。使用生化和机械测试确定脱细胞材料的完整性。在脱细胞之前和之后对α-Gal表位进行定量。当作为单个变量进行测试时,相对于DNA还原,在液氮,离子去污剂(0.1%SDS)和24小时的潜伏期中冻融脱细胞可产生最大的GAG和胶原蛋白保留率。综合起来,这些最佳脱细胞条件保留了更多的GAG,同时去除了与我们先前研究中使用的条件相同数量的DNA。 AF基质的成分和生物力学特性得以保留。去细胞的AF支架表现出合适的免疫相容性,如成功的体内重塑和α-Gal表位减少所证明。我们的研究确定了猪房颤组织脱细胞的最佳条件,同时保留了支架的生物学组成和力学性能。在这些条件下,免疫相容性通过成功的体内重塑和脱细胞材料中α-Gal表位的减少而得到证明。去细胞AF支架是脊柱外科临床应用的潜在候选者。

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