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一种在无饲养层条件下制备的新型肺泡上皮细胞片,有望用于肺再生治疗。

A novel alveolar epithelial cell sheet fabricated under feeder-free conditions for potential use in pulmonary regenerative therapy.

作者信息

Mitsuboshi Shota, Homma Jun, Sekine Hidekazu, Takagi Ryo, Shimizu Tatsuya, Kanzaki Masato

机构信息

Department of Thoracic Surgery, Tokyo Women's Medical University, 8-1 Kawada-cho, Shinjuku-ku, Tokyo 162-8666, Japan.

Institute of Advanced Biomedical Engineering and Science, Tokyo Women's Medical University, 8-1 Kawada-cho, Shinjuku-ku, Tokyo 162-8666, Japan.

出版信息

Regen Ther. 2022 Feb 5;19:113-121. doi: 10.1016/j.reth.2022.01.005. eCollection 2022 Mar.

Abstract

INTRODUCTION

Lung transplantation is the only effective treatment option for many patients with irreversible pulmonary injury, and the demand for lung transplantation is increasing worldwide and expected to continue to outstrip the number of available donors. Regenerative therapy with alveolar epithelial cells (AECs) holds promise as an alternative option to organ transplantation. AECs are usually co-cultured with mouse-derived 3T3 feeder cells, but the use of xenogeneic tissues for regenerative therapy raises safety concerns. Fabrication of AEC sheets under feeder-free conditions would avoid these safety issues. We describe a novel feeder-free method of fabricating AEC sheets that may be suitable for pulmonary regenerative therapy.

METHODS

Lung tissues excised from male outbred rats or transgenic rats expressing green fluorescent protein (GFP) were finely minced and dissociated with elastase. The isolated AECs were cultured under four different feeder-free conditions according to whether a rho kinase (ROCK) inhibitor was included in the low-calcium medium (LCM) and whether the tissue culture dish was coated with recombinant laminin-511 E8 fragment (rLN511E8). The expanded cells were cultured on temperature-responsive dishes and subsequently harvested as AEC sheets. Engraftment of GFP-AEC sheets after their transplantation onto a partially resected region of the left lung was assessed in athymic rats.

RESULTS

AECs proliferated and reached confluence when cultured in LCM containing a ROCK inhibitor on tissue culture dishes coated with rLN511E8. When both the ROCK inhibitor and rLN511E8-coated culture dish were used, the number of AECs obtained after 7 days of culture was significantly higher than that in the other three groups. Immunohistochemical analyses revealed that aquaporin-5, surfactant protein (SP)-A, SP-C, SP-D and Axin-2 were expressed by the cultured AECs. AEC sheets were harvested successfully from temperature-responsive culture dishes (by lowering the temperature) when the expanded AECs were cultured for 7 days in LCM + ROCK inhibitor and then for 3 days in LCM + ROCK inhibitor supplemented with 200 mg/L calcium chloride. The AEC sheets were firmly engrafted 7 days after transplantation onto the lung defect and expressed AEC marker proteins.

CONCLUSIONS

AEC sheets fabricated under feeder-free conditions retained the features of AECs after transplantation onto the lung . Further improvement of this technique may allow the bioengineering of alveolar-like tissue for use in pulmonary regenerative therapy.

摘要

引言

肺移植是许多不可逆肺损伤患者唯一有效的治疗选择,全球对肺移植的需求不断增加,预计仍将持续超过可用供体的数量。肺泡上皮细胞(AEC)再生疗法有望成为器官移植的替代选择。AEC通常与小鼠来源的3T3饲养层细胞共培养,但异种组织用于再生疗法引发了安全问题。在无饲养层条件下制备AEC片层可避免这些安全问题。我们描述了一种新的无饲养层制备AEC片层的方法,该方法可能适用于肺再生疗法。

方法

从雄性远交系大鼠或表达绿色荧光蛋白(GFP)的转基因大鼠切除的肺组织切成小块,用弹性蛋白酶解离。根据低钙培养基(LCM)中是否包含rho激酶(ROCK)抑制剂以及组织培养皿是否包被重组层粘连蛋白-511 E8片段(rLN511E8),将分离的AEC在四种不同的无饲养层条件下培养。将扩增的细胞接种在温度响应培养皿上,随后收获得到AEC片层。在无胸腺大鼠中评估GFP-AEC片层移植到左肺部分切除区域后的植入情况。

结果

当在包被rLN511E8的组织培养皿中于含ROCK抑制剂的LCM中培养时,AEC增殖并达到汇合。当同时使用ROCK抑制剂和包被rLN511E8的培养皿时,培养7天后获得的AEC数量显著高于其他三组。免疫组织化学分析显示,培养的AEC表达水通道蛋白-5、表面活性蛋白(SP)-A、SP-C、SP-D和Axin-2。当扩增的AEC在LCM + ROCK抑制剂中培养7天,然后在补充有200 mg/L氯化钙的LCM + ROCK抑制剂中培养3天时,成功从温度响应培养皿中(通过降低温度)收获AEC片层。AEC片层在移植到肺缺损后7天牢固植入,并表达AEC标记蛋白。

结论

在无饲养层条件下制备的AEC片层在移植到肺后保留了AEC的特性。该技术的进一步改进可能使肺泡样组织的生物工程用于肺再生疗法。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/ec80/9073894/b9e453c500f9/gr1.jpg

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