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灌注去细胞喉支架制备及喉肌重建可行性的初步研究

[A preliminary study on the preparation of perfusion-decellularized laryngeal scaffold and the feasibility of laryngeal muscle reconstruction].

作者信息

Hou Nan, Cui Peng-Cheng, Chen Wen-Xian, Luo Jia-Sheng, Ma Rui-Na

机构信息

Department of Otorhinolaryngology, Tangdu Hospital, Fourth Military Medical University, Xi'an 710038, China.

出版信息

Zhonghua Er Bi Yan Hou Tou Jing Wai Ke Za Zhi. 2009 Jul;44(7):586-90.

Abstract

OBJECTIVE

To prepare a decellularized whole laryngeal scaffold by utilizing a perfusion-decellularized technique, reseed cells on it, and construct decellularized laryngeal muscles.

METHODS

Perfusion decellularized larynxes were obtained by common carotid arterious perfusion with detergents. Then they were performed by macroscopic view, histological examination, scanning electron microscopy (SEM) and cartilage viability. Decellularized laryngeal scaffold were then reseeded with inducted mesenchymal stem cells (MSCs). Composites were transferred into greater omentums of rabbits after one day's adherence and harvested after eight weeks. Macroscopic view, histological examination and immunohistochemistry were performed.

RESULTS

Perfusion larynxes became transparent after two hours. Histology and SEM indicated that perfusion method showed better decullularized effect. More vintages and collagen fibers but no intact cell or nuclei were retained in the decellularized matrix. Porosity measured by Image pro plus 6.0 was 80.4% +/- 3.2% (x +/- s). Chondrocyte vitality assay indicated chondrocyte vitality rate in the perfusion group was 86.9% +/- 1.5%. After eight weeks, vascularization formed and integrated cartilage frameworks still remained. Histological examination could clearly show the presence of muscle bundles and vessels. Immunohistochemical examination indicated that sarcomeric-alpha actin expressed positively in corresponding areas.

CONCLUSIONS

It is feasible to reseed MSCs into the decellularized laryngeal muscle matrix for constructing tissue-engineered laryngeal muscles. This in vivo maturation into the omentum could be the first step before in situ implantation of the construct.

摘要

目的

利用灌注脱细胞技术制备去细胞全喉支架,在其上接种细胞,构建去细胞喉肌。

方法

通过颈总动脉灌注去污剂获得灌注去细胞喉。然后对其进行大体观察、组织学检查、扫描电子显微镜(SEM)检查和软骨活力检测。接着将诱导的间充质干细胞(MSCs)接种到去细胞喉支架上。接种一天后,将复合物转移到兔大网膜中,8周后取出。进行大体观察、组织学检查和免疫组织化学检查。

结果

灌注2小时后喉变得透明。组织学和SEM显示灌注法脱细胞效果更好。去细胞基质中保留了更多的纤维和胶原纤维,但没有完整的细胞或细胞核。用Image pro plus 6.0测量的孔隙率为80.4%±3.2%(x±s)。软骨细胞活力检测表明灌注组软骨细胞活力率为86.9%±1.5%。8周后,形成了血管化,完整的软骨框架仍然存在。组织学检查能清楚地显示肌束和血管的存在。免疫组织化学检查表明肌节α肌动蛋白在相应区域呈阳性表达。

结论

将MSCs接种到去细胞喉肌基质中构建组织工程化喉肌是可行的。在大网膜中进行这种体内成熟可能是该构建体原位植入前的第一步。

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