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

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 li...

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Main Author: HAO Sijia, YANG Zhenli, BIAN Xiaocui, HOU Yuhong, LIU Yuqin
Format: Article
Language:zho
Published: Institute of Basic Medical Sciences and Peking Union Medical College Hospital, Chinese Academy of Medical Sciences / Peking Union Medical College. 2025-03-01
Series:Jichu yixue yu linchuang
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Online Access:https://journal11.magtechjournal.com/Jwk_jcyxylc/fileup/1001-6325/PDF/1001-6325-2025-45-3-281-317.pdf
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author HAO Sijia, YANG Zhenli, BIAN Xiaocui, HOU Yuhong, LIU Yuqin
author_facet HAO Sijia, YANG Zhenli, BIAN Xiaocui, HOU Yuhong, LIU Yuqin
author_sort HAO Sijia, YANG Zhenli, BIAN Xiaocui, HOU Yuhong, LIU Yuqin
collection DOAJ
description 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).
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institution OA Journals
issn 1001-6325
language zho
publishDate 2025-03-01
publisher Institute of Basic Medical Sciences and Peking Union Medical College Hospital, Chinese Academy of Medical Sciences / Peking Union Medical College.
record_format Article
series Jichu yixue yu linchuang
spelling doaj-art-e67bf14523124ae78034213636b8e29d2025-08-20T01:50:33ZzhoInstitute of Basic Medical Sciences and Peking Union Medical College Hospital, Chinese Academy of Medical Sciences / Peking Union Medical College.Jichu yixue yu linchuang1001-63252025-03-0145331732210.16352/j.issn.1001-6325.2025.03.0317Establishment and characterization ofmouse hepatic tumor cell line with luc2-tdT expressionHAO Sijia, YANG Zhenli, BIAN Xiaocui, HOU Yuhong, LIU Yuqin0Department of Pathology, Cell Resource Center, Institute of Basic Medical Sciences CAMS, School of Basic Medicine PUMC, Beijing 100005, ChinaObjective 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).https://journal11.magtechjournal.com/Jwk_jcyxylc/fileup/1001-6325/PDF/1001-6325-2025-45-3-281-317.pdfmouse liver cancer cell line|fluorescence labeling|in vivoimaging|organoid
spellingShingle HAO Sijia, YANG Zhenli, BIAN Xiaocui, HOU Yuhong, LIU Yuqin
Establishment and characterization ofmouse hepatic tumor cell line with luc2-tdT expression
Jichu yixue yu linchuang
mouse liver cancer cell line|fluorescence labeling|in vivoimaging|organoid
title Establishment and characterization ofmouse hepatic tumor cell line with luc2-tdT expression
title_full Establishment and characterization ofmouse hepatic tumor cell line with luc2-tdT expression
title_fullStr Establishment and characterization ofmouse hepatic tumor cell line with luc2-tdT expression
title_full_unstemmed Establishment and characterization ofmouse hepatic tumor cell line with luc2-tdT expression
title_short Establishment and characterization ofmouse hepatic tumor cell line with luc2-tdT expression
title_sort establishment and characterization ofmouse hepatic tumor cell line with luc2 tdt expression
topic mouse liver cancer cell line|fluorescence labeling|in vivoimaging|organoid
url https://journal11.magtechjournal.com/Jwk_jcyxylc/fileup/1001-6325/PDF/1001-6325-2025-45-3-281-317.pdf
work_keys_str_mv AT haosijiayangzhenlibianxiaocuihouyuhongliuyuqin establishmentandcharacterizationofmousehepatictumorcelllinewithluc2tdtexpression