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首页> 外文期刊>Journal of biomedical materials research, Part A >Effect of extraction protocols and epidermal growth factor on the cellular repopulation of decellularized anterior cruciate ligament allografts.
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Effect of extraction protocols and epidermal growth factor on the cellular repopulation of decellularized anterior cruciate ligament allografts.

机译:提取方案和表皮生长因子对脱细胞的前交叉韧带同种异体移植细胞再增殖的影响。

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We are developing a decellularized bone-anterior cruciate ligament (ACL)-bone allograft for treatment of ACL disruption in young or active patients. This study demonstrates the feasibility of seeding decellularized ACL tissue with primary ligament fibroblasts. Porcine ACLs were decellularized by one of three protocols, each differing only by the detergent/solvent used during the second wash (SDS, Triton-X, or TnBP). Porcine ACL fibroblasts were obtained by explant and seeded onto tissue samples of decellularized ACL. Culture conditions were varied to compare the relative effect of three different decellularization protocols on cellular repopulation. Culture condition variables included (1) the number of cells used for seeding, (2) the addition of epidermal growth factor (EGF), and (3) culture duration. Cellular ingrowth was assessed by metabolic activity (MTT assay), DNA quantification (Hoescht dye), and histology (H&E staining). Cell counting on histological sections demonstrated that Triton-X-and TnBP-treated ligaments were more receptive to cellular ingrowth than SDS-treated samples. The addition of EGF to culture medium did not significantly increase cellular ingrowth. Both the Triton-X and TnBP decellularization treatments provide suitable, naturally derived scaffolds for the ingrowth of primary ACL fibroblasts, and should be further investigated in the development of an allograft-derived bone-ACL-bone graft.
机译:我们正在开发一种脱细胞的骨前交叉韧带(ACL)-骨同种异体移植物,用于治疗年轻或活跃患者的ACL破坏。这项研究证明了用原韧带成纤维细胞播种去细胞的ACL组织的可行性。猪ACL通过以下三种方案之一脱细胞,每种方案仅在第二次洗涤(SDS,Triton-X或TnBP)期间使用的去污剂/溶剂有所不同。通过外植获得猪ACL成纤维细胞,并接种到脱细胞ACL的组织样品上。改变培养条件以比较三种不同的脱细胞方案对细胞重聚的相对作用。培养条件变量包括(1)用于接种的细胞数量,(2)添加表皮生长因子(EGF),以及(3)培养时间。通过代谢活性(MTT测定),DNA定量(Hoescht染料)和组织学(H&E染色)评估细胞向内生长。组织切片上的细胞计数表明,经Triton-X和TnBP处理的韧带比经SDS处理的样品更容易接受细胞向内生长。向培养基中添加EGF不会显着增加细胞向内生长。 Triton-X和TnBP脱细胞处理都为原ACL成纤维细胞的向内生长提供了合适的,天然来源的支架,在同种异体移植衍生的ACL骨移植物中应进一步研究。

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