Luc2-tdT标记的小鼠肝癌细胞系的建立及鉴定

doi:10.16352/j.issn.1001-6325.2025.03.0317

基础医学与临床 ›› 2025, Vol. 45 ›› Issue (3): 317-322.doi: 10.16352/j.issn.1001-6325.2025.03.0317

Luc2-tdT标记的小鼠肝癌细胞系的建立及鉴定

郝思嘉, 杨振丽, 卞晓翠, 侯昱宏, 刘玉琴^*

中国医学科学院基础医学研究所北京协和医学院基础学院病理学系细胞资源中心,北京 100005

收稿日期:2025-01-02 修回日期:2025-02-10 发布日期:2025-02-25
通讯作者: ^*liuyuqin@pumc.edu.cn
基金资助:
国家科技基础条件平台项目(NSTI-BMCR24)

Establishment and characterization ofmouse hepatic tumor cell line with luc2-tdT expression

HAO Sijia, YANG Zhenli, BIAN Xiaocui, HOU Yuhong, LIU Yuqin^*

Department of Pathology, Cell Resource Center, Institute of Basic Medical Sciences CAMS, School of Basic Medicine PUMC, Beijing 100005, China

Received:2025-01-02 Revised:2025-02-10 Published:2025-02-25

摘要/Abstract

摘要： 目的建立小鼠肝癌H22瘤株的细胞系及稳定表达tdTomato红色荧光标记和萤火虫荧光素酶的细胞系(H22-luc2-tdT),建立细胞系来源的移植瘤体内成像模型。方法利用小鼠肝癌H22移植瘤,进行原代培养,建立连续传代的细胞系。检测细胞体外增殖,进行染色体分析、体内成瘤监测、体内生长、HE梁色和免疫组化检测、aFP、CK7、CK15等标志物表达,并将移植瘤组取材后进行类器官培养。确认建系成功后,通过慢病毒感染的方式使H22细胞稳定表达红色荧光蛋白和萤光素酶融合蛋白Luc2-tdT,后经流式分选获得的Luc2-tdT阳性细胞群,进行体内、体外荧光成像观察。对所建细胞系进行支原体检测、种属检测。结果连续培养的H22细胞系体外已传代至P50。第22代的细胞在C57小鼠皮下和腹腔移植,成瘤率均为100%。皮下移植瘤HE观察形态与原瘤株一致、CK阳性、AFP阳性,表明其为肝癌来源。染色体众数40~44条染色体、端着丝粒。体外细胞生长d0~d3为潜伏期,d3~d5为指数增殖期,d6出现下降趋势。将P22代的H22细胞转染luc2-tdT质粒,筛选后荧光阳性率100%,命名为H22-luc2-tdT细胞,形态与H22细胞一致,荧光显微镜下观察和体内移植瘤活体观察荧光表达强。H22细胞的移植瘤组织可培养形成类器官。细胞培养上清支原体检测阴性,PCR种属鉴定证明来源于小鼠。结论成功建立了双荧光标记的小鼠肝癌细胞系,便于体外、体内肝癌模型及肝癌转移示踪模型的建立和应用,利用活体成像可全周期观察肿瘤生长及转移情况,还可通过荧光定量进行定量研究。已由国家生物医学实验细胞资源库(http://www.cellresource.cn)收藏、提供共享。

关键词: 小鼠肝癌细胞系, 荧光标记, 活体成像, 类器官

Abstract: Objective The mouse autologous tumor model H22 is more valuable for tumor immunological-related research. This paper aims to establish mouse hepatic tumor cell line (H22-luc2-tdT)that stably express the tandem-dimer tomato(tdTomato) and luciferase genes.Establish an in vivo imaging model of cell line derived transplanted tumors。Methods Using transplanted H22 tumor tissue, primary culture and continuous passage in vitro were performed to establish a continuous cell line. Cell proliferation, chromosome analysis, organoid culture, tumorigenicity, HE and ICH of aFP,CK7, CK15 were performed to charaterize the cell line. Then the luc2-tdTplasmid was transfected into H22 cells of P22, flow cytometry and in vitro/in vivo imaging were employed to screen and verify fluorescence expression. Mycoplasma detection and species verification of the established cell lines were performed. Results The H22 cells had been continuously passaged over 50 times. The cells of passsge 22(P22) were transplanted subcutaneously and intraperitoneally into C57 and Kunming mice, with a 100% tumor formation. The HE morphology of subcutaneous transplanted tumor were consistent with the original tumor. CK⁺/AFP⁺proved that it was of liver cancer origin. The H22 cells were hypo-triploid with a modal number of 40-44 chromosomes and telocentromeres, verifing its mouse origin. The latent phase for in vitro growth of H22 lasted from d0 to d3, while the exponential phaes d3 to d5, and reach plateou at d6. Successful transfection of H22 cells with the luc2-tdT were observed with in vitro/in vivo 100% fluorescence positivity, thus named H22-luc2-tdT. The transplanted tumor tissue of H22 cells could be primarily cultured to form organoids. The detection of Mycoplasma was negative, and its mouse origin confirmed by PCR. Conclusions H22 and H22-luc2-tdT cell lines are established and characterized, which can be used for the establishment and application of in vitro and in vivo liver cancer research and metastatic cell tracking. These cell lines are deposited at and can obtain from the National Biomedical Cell Resource Center(http://www.cellresource.cn).

Key words: mouse liver cancer cell line, fluorescence labeling, in vivoimaging, organoid

中图分类号:

R735

郝思嘉, 杨振丽, 卞晓翠, 侯昱宏, 刘玉琴. Luc2-tdT标记的小鼠肝癌细胞系的建立及鉴定[J]. 基础医学与临床, 2025, 45(3): 317-322.

HAO Sijia, YANG Zhenli, BIAN Xiaocui, HOU Yuhong, LIU Yuqin. Establishment and characterization ofmouse hepatic tumor cell line with luc2-tdT expression[J]. Basic & Clinical Medicine, 2025, 45(3): 317-322.

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Luc2-tdT标记的小鼠肝癌细胞系的建立及鉴定

Establishment and characterization ofmouse hepatic tumor cell line with luc2-tdT expression

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