Optimizing decellularization protocols for human thyroid tissues: a step towards tissue engineering and transplantation.

Özge Karabıyık Acar, Gülnihal Bozdağ, Ezgi Hacıhasanoğlu, A Alperen Tuncer, Erhan Aysan, Gamze Torun Köse
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Abstract

Hypothyroidism is caused by insufficient stimulation or disruption of the thyroid. However, the drawbacks of thyroid transplantation have led to the search for new treatments. Decellularization allows tissue transplants to maintain their biomimetic structures while preserving cell adhesion, proliferation, and differentiation. This study aimed to decellularize human thyroid tissues using a structure-preserving optimization strategy and present preliminary data on recellularization. Nine methods were used for physical and chemical decellularization. Quantitative and immunohistochemical analyses were performed to investigate the DNA and extracellular matrix components of the tissues. Biomechanical properties were determined by compression test, and cell viability was examined after seeding MDA-T32 papillary thyroid cancer (PTC) cells onto the decellularized tissues. Decellularized tissues exhibited a notable decrease (<50 ng mg-1DNA, except for Groups 2 and 7) compared to the native thyroid tissue. Nonetheless, collagen and glycosaminoglycans were shown to be conserved in all decellularized tissues. Laminin and fibronectin were preserved at comparatively higher levels, and Young's modulus was elevated when decellularization included SDS. It was observed that the strain value in Group 1 (1.63 ± 0.14 MPa) was significantly greater than that in the decellularized tissues between Groups 2-9, ranging from 0.13 ± 0.03-0.72 ± 0.29 MPa. Finally, viability assessment demonstrated that PTC cells within the recellularized tissue groups successfully attached to the 3D scaffolds and sustained metabolic activity throughout the incubation period. We successfully established a decellularization optimization for human thyroid tissues, which has potential applications in tissue engineering and transplantation research. Our next goal is to conduct recellularization using the methods utilized in Group 1 and transplant the primary thyroid follicular cell-seeded tissues into anin vivoanimal model, particularly due to their remarkable 3D structural preservation and cell adhesion-promoting properties.

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优化人类甲状腺组织的脱细胞方案:向组织工程和移植迈出的一步。
甲状腺功能减退症是由甲状腺受到的刺激不足或破坏引起的。然而,甲状腺移植的缺点导致人们开始寻找新的治疗方法。脱细胞技术可使组织移植保持其仿生结构,同时保留细胞的粘附性、增殖性和分化性。本研究旨在采用结构保留优化策略对人体甲状腺组织进行脱细胞处理,并提供再细胞化的初步数据。研究采用了九种方法进行物理和化学脱细胞。通过定量和免疫组化分析,研究了组织中的 DNA 和细胞外基质成分。在脱细胞组织上播种 MDA-T32 甲状腺乳头状癌(PTC)细胞后,对细胞存活率进行了检测。与原生甲状腺组织相比,脱细胞组织的DNA含量明显下降(除第2组外,均小于50 ng/mg DNA)。尽管如此,胶原蛋白和糖胺聚糖在所有脱细胞组织中都得到了保留。层粘连蛋白和纤连蛋白的保存水平相对较高,在脱细胞过程中加入 SDS 时,杨氏模量会升高。据观察,第 1 组的应变值(1.63 ± 0.14 兆帕)明显高于第 2-9 组脱细胞组织的应变值(0.13 ± 0.03 至 0.72 ± 0.29 兆帕)。最后,存活率评估表明,再细胞化组织组中的 PTC 细胞成功附着在三维支架上,并在整个培养期间保持新陈代谢活性。我们成功建立了人类甲状腺组织的脱细胞优化方法,这在组织工程和移植研究中具有潜在的应用价值。我们的下一个目标是采用第 1 组中使用的方法进行再细胞化,并将原代甲状腺滤泡细胞播种组织移植到体内动物模型中,特别是由于其显著的三维结构保存和细胞粘附促进特性。
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