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Establishment and identification of human primary lung cancer cell culture in vitro

机译:人原发性肺癌细胞体外培养的建立与鉴定

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摘要

Objective: To explore a simple and practical method for human primary lung cancer cells culture in vitro. Methods: Tumor specimens from 6 lung cancer patients were isolated with collagenase digestion cultured in vitro. Then the characteristics of these cells were analyzed and identified by optical microscope observation, hematoxylin-eosin staining, immunocytochemistry, immunohistochemistry and tumor nude mice inoculation experiments, respectively. Results: Except for the small cell lung cancer, the other 5 samples were successfully isolated and cultured. The cultured cells showed typical characteristics of malignant cells and positive for cytokeratin 7 and 19. Moreover, the cancer cells readily formed subcutaneous tumors in nude mice and the pathological images of the transplanted tumor were consistent with its tumor origin. Conclusion: The primary culture for human lung cancer cells can be successfully achieved with the method of collagenase digestion.
机译:目的:探讨一种简单实用的体外人原代肺癌细胞培养方法。方法:采用体外培养的胶原酶消化法分离6例肺癌患者的肿瘤标本。然后通过光学显微镜观察,苏木精-伊红染色,免疫细胞化学,免疫组织化学和肿瘤裸鼠接种实验来分析和鉴定这些细胞的特性。结果:除小细胞肺癌外,其余5份标本均成功分离培养。培养的细胞显示出恶性细胞的典型特征,并且对细胞角蛋白7和19呈阳性。此外,癌细胞容易在裸鼠中形成皮下肿瘤,并且移植肿瘤的病理图像与其肿瘤来源一致。结论:胶原酶消化法可以成功地实现人肺癌细胞的原代培养。

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