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日本恶性胸膜间皮瘤患者细胞系的建立及其分子特征分析

Establishment and molecular characterization of cell lines from Japanese patients with malignant pleural mesothelioma.

作者信息

Suzawa Ken, Yamamoto Hiromasa, Murakami Tomoyuki, Katayama Hideki, Furukawa Masashi, Shien Kazuhiko, Hashida Shinsuke, Okabe Kazunori, Aoe Keisuke, Soh Junichi, Asano Hiroaki, Tsukuda Kazunori, Mimura Yusuke, Toyooka Shinichi, Miyoshi Shinichiro

机构信息

Department of Thoracic, Breast and Endocrinological Surgery, Okayama University Graduate School of Medicine, Dentistry and Pharmaceutical Sciences, Okayama 700-8558, Japan.

Department of Thoracic, Breast and Endocrinological Surgery, Okayama University Graduate School of Medicine, Dentistry and Pharmaceutical Sciences, Okayama 700-8558, Japan; Department of Thoracic Surgery, National Hospital Organization Yamaguchi-Ube Medical Center, Ube, Yamaguchi 755-0241, Japan; Department of Clinical Research, National Hospital Organization Yamaguchi-Ube Medical Center, Ube, Yamaguchi 755-0241, Japan.

出版信息

Oncol Lett. 2016 Jan;11(1):705-712. doi: 10.3892/ol.2015.3955. Epub 2015 Nov 23.

Abstract

Malignant pleural mesothelioma (MPM) is an aggressive disease that is resistant to conventional therapies. Cell lines are useful models for studying the biological characteristics of tumors; therefore, the establishment of MPM cell lines is valuable for exploring novel therapeutic strategies for MPM. In the present study, 4 MPM cell lines (YUMC8, YUMC44, YUMC63, and YUMC64) were established, which consisted of 2 epithelioid and 2 sarcomatoid mesothelioma histological subtypes, from Japanese patients with MPM. The DNA methylation status, mutations, copy number gains, protein expression of representative genes, and the sensitivity to several drugs were examined in these 4 cell lines. Methylation of was demonstrated in 3/4 cell lines, in which the protein expression of p16 was lost. Methylation of was observed in 3/4 cell lines. Copy number gains of , or were not detected in the 4 cell lines. Mutations in various genes, including , , , , and , which are frequently detected in non-small cell lung cancer, were not detected in the 4 cell lines. microRNA-34b/c is a direct transcriptional target of p53 and is often silenced in MPM by promoter methylation. In the present study, miR-34b/c was heavily methylated in 2/4 established MPM cell lines. For cell adhesion molecules, E-cadherin expression was detected in the 2 epithelioid MPM cell lines, whereas N-cadherin expression was detected in all 4 established cell lines by western blotting. Vimentin was strongly expressed in the 2 sarcomatoid MPM cell lines. None of the established MPM cell lines demonstrated significant responses to the drugs tested, including NVP-AUY922, 17-DMAG, Trichostatin A, and Vorinostat. Although novel molecular findings were not observed in the current characterization of these MPM cell lines, these lines will be useful for future extensive analyses of the biological behavior of MPM and the development of novel therapeutic strategies.

摘要

恶性胸膜间皮瘤(MPM)是一种侵袭性疾病,对传统疗法具有抗性。细胞系是研究肿瘤生物学特性的有用模型;因此,建立MPM细胞系对于探索MPM的新型治疗策略具有重要价值。在本研究中,从日本MPM患者中建立了4种MPM细胞系(YUMC8、YUMC44、YUMC63和YUMC64),其中包括2种上皮样和2种肉瘤样间皮瘤组织学亚型。检测了这4种细胞系中的DNA甲基化状态、突变、拷贝数增加、代表性基因的蛋白质表达以及对几种药物的敏感性。在4种细胞系中的3种中证实了 的甲基化,其中p16的蛋白质表达缺失。在4种细胞系中的3种中观察到了 的甲基化。在这4种细胞系中未检测到 、 或 的拷贝数增加。在这4种细胞系中未检测到在非小细胞肺癌中经常检测到的包括 、 、 、 和 在内的各种基因的突变。微小RNA-34b/c是p53的直接转录靶点,在MPM中常因启动子甲基化而沉默。在本研究中,在2/4已建立的MPM细胞系中,miR-34b/c高度甲基化。对于细胞粘附分子,通过蛋白质印迹法在2种上皮样MPM细胞系中检测到E-钙粘蛋白表达,而在所有4种已建立的细胞系中均检测到N-钙粘蛋白表达。波形蛋白在2种肉瘤样MPM细胞系中强烈表达。所建立的MPM细胞系对所测试的药物,包括NVP-AUY922、17-DMAG、曲古抑菌素A和伏立诺他,均未表现出显著反应。尽管在这些MPM细胞系的当前特征中未观察到新的分子发现,但这些细胞系将有助于未来对MPM生物学行为的广泛分析和新型治疗策略的开发。

相似文献

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DNA copy number gains in malignant pleural mesothelioma.恶性胸膜间皮瘤中的DNA拷贝数增加
Oncol Lett. 2015 Nov;10(5):3274-3278. doi: 10.3892/ol.2015.3652. Epub 2015 Aug 27.

本文引用的文献

1
Malignant pleural mesothelioma: an epidemiological perspective.恶性胸膜间皮瘤:一种流行病学视角。
Ann Cardiothorac Surg. 2012 Nov;1(4):491-6. doi: 10.3978/j.issn.2225-319X.2012.11.04.
7
Lung cancer cell lines as tools for biomedical discovery and research.肺癌细胞系作为生物医学发现和研究的工具。
J Natl Cancer Inst. 2010 Sep 8;102(17):1310-21. doi: 10.1093/jnci/djq279. Epub 2010 Aug 2.

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