The impact of decellularization agents on renal tissue extracellular matrix

去细胞化 细胞外基质 过氧乙酸 胰蛋白酶化 化学 糖胺聚糖 十二烷基硫酸钠 组织工程 细胞生物学 成纤维细胞 再生(生物学) 生物化学 活力测定 细胞 生物医学工程 胰蛋白酶 生物 医学 体外 过氧化氢
作者
Nafiseh Poornejad,Lara B. Schaumann,Evan Buckmiller,Nima Momtahan,Jason Gassman,Ho Hin,Beverly L. Roeder,Paul R. Reynolds,Alonzo D. Cook
出处
期刊:Journal of Biomaterials Applications [SAGE Publishing]
卷期号:31 (4): 521-533 被引量:71
标识
DOI:10.1177/0885328216656099
摘要

The combination of patient-specific cells with scaffolds obtained from natural sources may result in improved regeneration of human tissues. Decellularization of the native tissue is the first step in this technology. Effective decellularization uses agents that lyse cells and remove all cellular materials, leaving intact collagenous extracellular matrices (ECMs). Removing cellular remnants prevents an immune response while preserving the underlying structure. In this study, the impact of five decellularization agents (0.1 N NaOH, 1% peracetic acid, 3% Triton X-100, 1% sodium dodecyl sulfate (SDS), and 0.05% trypsin/EDTA) on renal tissue was examined using slices of porcine kidneys. The NaOH solution induced the most efficient cell removal, and resulted in the highest amount of cell viability and proliferation after recellularization, although it also produced the most significant damage to collagenous fiber networks, glycosaminoglycans (GAGs) and fibroblast growth factor (FGF). The SDS solution led to less severe damage to the ECM structure but it resulted in lower metabolic activity and less proliferation. Peracetic acid and Triton X-100 resulted in minimum disruption of ECMs and the most preserved GAGs and FGF. However, these last two agents were not as efficient in removing cellular materials as NaOH and SDS, especially peracetic acid, which left more than 80% of cellular material within the ECM. As a proof of principle, after completing the comparison studies using slices of renal ECM, the NaOH process was used to decellularize a whole kidney, with good results. The overall results demonstrate the significant effect of cell lysing agents and the importance of developing an optimized protocol to avoid extensive damage to the ECM while retaining the ability to support cell growth.
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