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高效II型细胞增强绿色荧光蛋白表达有助于细胞识别、追踪和分离。

High-efficiency type II cell-enhanced green fluorescent protein expression facilitates cellular identification, tracking, and isolation.

作者信息

Vanderbilt Jeff N, Gonzalez Robert F, Allen Lennell, Gillespie AnneMarie, Leaffer David, Dean Willow B, Chapin Cheryl, Dobbs Leland G

机构信息

1 Cardiovascular Research Institute and.

Departments of 2 Pediatrics and.

出版信息

Am J Respir Cell Mol Biol. 2015 Jul;53(1):14-21. doi: 10.1165/rcmb.2014-0348MA.

Abstract

We have developed a transgenic mouse expressing enhanced green fluorescent protein (EGFP) in virtually all type II (TII) alveolar epithelial cells. The CBG mouse (SPC-BAC-EGFP) contains a bacterial artificial chromosome modified to express EGFP within the mouse surfactant protein (SP)-C gene 3' untranslated region. EGFP mRNA expression is limited to the lung. EGFP fluorescence is both limited to and exhibited by all cells expressing pro-SP-C; fluorescence is uniform throughout all lobes of the lung and does not change as mice age. EGFP(+) cells also express SP-B but do not express podoplanin, a type I (TI) cell marker. CBG mice show no evidence of lung disease with aging. In 3 hours, TII cells can be isolated in >99% purity from CBG mice by FACS; the yield of 3.7 ± 0.6 × 10(6) cells represents approximately 25 to 60% of the TII cells in the lung. By FACS analysis, approximately 0.9% of TII cells are in mitosis in uninjured lungs; after bleomycin injury, 4.1% are in mitosis. Because EGFP fluorescence can be detected for >14 days in culture, at a time that SP-C mRNA expression is essentially nil, this line may be useful for tracking TII cells in culture and in vivo. When CBG mice are crossed to transgenic mice expressing rat podoplanin, TI and TII cells can be easily simultaneously identified and isolated. When bred to other strains of mice, EGFP expression can be used to identify TII cells without the need for immunostaining for SP-C. These mice should be useful in models of mouse pulmonary disease and in studies of TII cell biology, biochemistry, and genetics.

摘要

我们培育出了一种转基因小鼠,其几乎所有II型(TII)肺泡上皮细胞中都表达增强型绿色荧光蛋白(EGFP)。CBG小鼠(SPC-BAC-EGFP)包含一个经过修饰的细菌人工染色体,可在小鼠表面活性蛋白(SP)-C基因的3'非翻译区内表达EGFP。EGFP mRNA的表达仅限于肺部。EGFP荧光仅限于所有表达前SP-C的细胞并由这些细胞发出;荧光在肺的所有叶中均匀分布,并且不会随着小鼠年龄增长而改变。EGFP(+)细胞也表达SP-B,但不表达I型(TI)细胞标志物血小板内皮细胞黏附分子。CBG小鼠未显示出随着年龄增长出现肺部疾病的迹象。在3小时内,通过荧光激活细胞分选术(FACS)可从CBG小鼠中分离出纯度>99%的TII细胞;3.7±0.6×10⁶个细胞的产量约占肺中TII细胞的25%至60%。通过FACS分析,在未受伤的肺中,约0.9%的TII细胞处于有丝分裂状态;博来霉素损伤后,有4.1%处于有丝分裂状态。由于在培养中可检测到EGFP荧光超过14天,而此时SP-C mRNA表达基本为零,因此该品系可能有助于在培养中和体内追踪TII细胞。当CBG小鼠与表达大鼠血小板内皮细胞黏附分子的转基因小鼠杂交时,TI和TII细胞可轻松同时被识别和分离。当与其他品系的小鼠杂交时,EGFP表达可用于识别TII细胞,而无需对SP-C进行免疫染色。这些小鼠应可用于小鼠肺部疾病模型以及TII细胞生物学、生物化学和遗传学研究。

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