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人气管支气管基底细胞。体内和体外重塑/修复表型的正常对照。

Human tracheobronchial basal cells. Normal versus remodeling/repairing phenotypes in vivo and in vitro.

机构信息

1 Department of Pediatrics.

出版信息

Am J Respir Cell Mol Biol. 2013 Dec;49(6):1127-34. doi: 10.1165/rcmb.2013-0049OC.

Abstract

Human tracheobronchial epithelial (TBE) basal cells (BCs) function as progenitors in normal tissue. However, mechanistic studies are typically performed in vitro and frequently use BCs recovered from patients who die of nonrespiratory disease. It is not known whether the cadaveric epithelium (1) is undergoing homeostatic remodeling and/or repair, or (2) yields BC clones that represent homeostatic processes identified in tissue. We sought to compare the phenotype of TBE-BCs with that of BCs cultured under optimal clone-forming conditions. TBE pathology was evaluated using quantitative histomorphometry. The cultured BC phenotype was determined by fluorescence-activated cell sorter analysis. Clone organization and cell phenotype were determined by immunostaining. The cadaveric TBE is 20% normal. In these regions, BCs are keratin (K)-5(+) and tetraspanin CD151(+), and demonstrate a low mitotic index. In contrast, 80% of the cadaveric TBE exhibits homeostatic remodeling/repair processes. In these regions, BCs are K5(+)/K14(+), and a subset expresses tissue factor (TF). Passage 1 TBE cells are BCs that are K5(+)/TF(+), and half coexpress CD151. Optimal clone formation conditions use an irradiated NIH3T3 fibroblast feeder layer (American Type Culture Collection, Frederick, MD) and serum-supplemented Epicult-B medium (Stemcell Technologies, La Jolla, CA). The TF(+)/CD151(-) BC subpopulation is the most clonogenic BC subtype, and is enriched with K14(+) cells. TF(+)/CD151(-) BCs generate clones containing BCs that are K5(+)/Trp63(+), but K14(-)/CD151(-). TF(+) cells are limited to the clone edge. In conclusion, clonogenic human TBE BCs (1) exhibit a molecular phenotype that is a composite of the normal and remodeling/reparative BC phenotypes observed in tissue, and (2) generate organoid clones that contain phenotypically distinct BC subpopulations.

摘要

人气管支气管上皮 (TBE) 基底细胞 (BC) 在正常组织中作为祖细胞发挥功能。然而,机制研究通常在体外进行,并且经常使用从死于非呼吸道疾病的患者中回收的 BC。尚不清楚尸体上皮 (1) 是否正在进行稳态重塑和/或修复,或者 (2) 是否产生代表组织中鉴定的稳态过程的 BC 克隆。我们试图比较 TBE-BC 的表型与在最佳克隆形成条件下培养的 BC 的表型。使用定量组织形态计量学评估 TBE 病理学。通过荧光激活细胞分选分析确定培养的 BC 表型。通过免疫染色确定克隆组织和细胞表型。尸体 TBE 的 20%是正常的。在这些区域,BC 是角蛋白 (K)-5(+)和四跨膜蛋白 CD151(+),并表现出低有丝分裂指数。相比之下,尸体 TBE 的 80%表现出稳态重塑/修复过程。在这些区域,BC 是 K5(+)/K14(+),并且亚群表达组织因子 (TF)。TBE 细胞的传代 1 是 K5(+)/TF(+)的 BC,并且有一半共同表达 CD151。最佳克隆形成条件使用辐照 NIH3T3 成纤维细胞饲养层 (美国典型培养物保藏中心,弗雷德里克,MD) 和血清补充的 Epicult-B 培养基 (Stemcell Technologies,拉霍亚,CA)。TF(+)/CD151(-)BC 亚群是最具克隆形成能力的 BC 亚型,并且富含 K14(+)细胞。TF(+)/CD151(-)BC 产生含有 K5(+)/Trp63(+)但 K14(-)/CD151(-)的 BC 的克隆。TF(+)细胞仅限于克隆边缘。总之,克隆形成的人 TBE BC (1) 表现出一种分子表型,该表型是组织中观察到的正常和重塑/修复 BC 表型的组合,并且 (2) 产生包含表型不同的 BC 亚群的类器官克隆。

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