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一种在临床前动物模型中检测人循环肿瘤细胞的快速定量方法。

A rapid and quantitative method to detect human circulating tumor cells in a preclinical animal model.

作者信息

Tu Shih-Hsin, Hsieh Yi-Chen, Huang Li-Chi, Lin Chun-Yu, Hsu Kai-Wen, Hsieh Wen-Shyang, Chi Wei-Ming, Lee Chia-Hwa

机构信息

Department of Surgery, School of Medicine, College of Medicine, Taipei Medical University, Taipei, Taiwan.

Division of Breast Surgery, Department of Surgery, Cathay General Hospital, Taipei, Taiwan.

出版信息

BMC Cancer. 2017 Jun 23;17(1):440. doi: 10.1186/s12885-017-3419-x.

Abstract

BACKGROUND

As cancer metastasis is the deadliest aspect of cancer, causing 90% of human deaths, evaluating the molecular mechanisms underlying this process is the major interest to those in the drug development field. Both therapeutic target identification and proof-of-concept experimentation in anti-cancer drug development require appropriate animal models, such as xenograft tumor transplantation in transgenic and knockout mice. In the progression of cancer metastasis, circulating tumor cells (CTCs) are the most critical factor in determining the prognosis of cancer patients. Several studies have demonstrated that measuring CTC-specific markers in a clinical setting (e.g., flow cytometry) can provide a current status of cancer development in patients. However, this useful technique has rarely been applied in the real-time monitoring of CTCs in preclinical animal models.

METHODS

In this study, we designed a rapid and reliable detection method by combining a bioluminescent in vivo imaging system (IVIS) and quantitative polymerase chain reaction (QPCR)-based analysis to measure CTCs in animal blood. Using the IVIS Spectrum CT System with 3D-imaging on orthotropic-developed breast-tumor-bearing mice.

RESULTS

In this manuscript, we established a quick and reliable method for measuring CTCs in a preclinical animal mode. The key to this technique is the use of specific human and mouse GUS primers on DNA/RNA of mouse peripheral blood under an absolute qPCR system. First, the high sensitivity of cancer cell detection on IVIS was presented by measuring the luciferase carried MDA-MB-231 cells from 5 to 5x10 cell numbers with great correlation (R = 0.999). Next, the MDA-MB-231 cell numbers injected by tail vein and their IVIS radiance signals were strongly corrected with qPCR-calculated copy numbers (R > 0.99). Furthermore, by applying an orthotropic implantation animal model, we successfully distinguished xenograft tumor-bearing mice and control mice with a significant difference (p < 0.001), whereas IVIS Spectrum-CT 3D-visualization showed that blood of mice with lung metastasis contained more than twice the CTC numbers than ordinary tumor-bearing mice. We demonstrated a positive correlation between lung metastasis status and CTC numbers in peripheral mouse blood.

CONCLUSION

Collectively, the techniques developed for this study resulted in the integration of CTC assessments into preclinical models both in vivo and ex vivo, which will facilitate translational targeted therapy in clinical practice.

摘要

背景

由于癌症转移是癌症最致命的方面,导致90%的人类死亡,评估这一过程背后的分子机制是药物开发领域研究人员的主要兴趣所在。抗癌药物开发中的治疗靶点识别和概念验证实验都需要合适的动物模型,比如在转基因和基因敲除小鼠中进行异种移植肿瘤移植。在癌症转移的进程中,循环肿瘤细胞(CTC)是决定癌症患者预后的最关键因素。多项研究表明,在临床环境中检测CTC特异性标志物(如流式细胞术)可以提供患者癌症发展的当前状况。然而,这项有用的技术很少应用于临床前动物模型中CTC的实时监测。

方法

在本研究中,我们设计了一种快速可靠的检测方法,通过结合生物发光体内成像系统(IVIS)和基于定量聚合酶链反应(QPCR)的分析来测量动物血液中的CTC。使用IVIS Spectrum CT系统对原位发育的荷乳腺癌小鼠进行三维成像。

结果

在本论文中,我们建立了一种在临床前动物模型中测量CTC的快速可靠方法。该技术的关键是在绝对定量PCR系统下,在小鼠外周血的DNA/RNA上使用特异性的人和小鼠GUS引物。首先,通过测量携带荧光素酶的MDA-MB-231细胞从5到5×10个细胞数量,展示了IVIS对癌细胞检测的高灵敏度,且具有高度相关性(R = 0.999)。其次,尾静脉注射的MDA-MB-231细胞数量与其IVIS辐射信号与qPCR计算的拷贝数高度相关(R > 0.99)。此外,通过应用原位植入动物模型,我们成功区分了荷异种移植肿瘤小鼠和对照小鼠,差异显著(p < 0.001),而IVIS Spectrum-CT三维可视化显示,发生肺转移的小鼠血液中的CTC数量比普通荷瘤小鼠多两倍以上。我们证明了小鼠外周血中肺转移状态与CTC数量之间存在正相关。

结论

总体而言,本研究开发的技术实现了将CTC评估整合到体内和体外的临床前模型中,这将有助于临床实践中的转化靶向治疗。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/269e/5481956/b3e2937f776d/12885_2017_3419_Fig1_HTML.jpg

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