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一种用于研究肿瘤细胞迁移和抗侵袭药物对患者特异性影响的人胶质母细胞瘤器官型切片培养模型。

A Human Glioblastoma Organotypic Slice Culture Model for Study of Tumor Cell Migration and Patient-specific Effects of Anti-Invasive Drugs.

作者信息

Parker Jonathon J, Lizarraga Marcela, Waziri Allen, Foshay Kara M

机构信息

Department of Neurosurgery, Stanford University Hospital, Stanford University School of Medicine.

Inova Neuroscience Institute.

出版信息

J Vis Exp. 2017 Jul 20(125):53557. doi: 10.3791/53557.

Abstract

Glioblastoma (GBM) continues to carry an extremely poor clinical prognosis despite surgical, chemotherapeutic, and radiation therapy. Progressive tumor invasion into surrounding brain parenchyma represents an enduring therapeutic challenge. To develop anti-migration therapies for GBM, model systems that provide a physiologically relevant background for controlled experimentation are essential. Here, we present a protocol for generating slice cultures from human GBM tissue obtained during surgical resection. These cultures allow for ex vivo experimentation without passaging through animal xenografts or single cell cultures. Further, we describe the use of time-lapse laser scanning confocal microscopy in conjunction with cell tracking to quantitatively study the migratory behavior of tumor cells and associated response to therapeutics. Slices are reproducibly generated within 90 min of surgical tissue acquisition. Retrovirally-mediated fluorescent cell labeling, confocal imaging, and tumor cell migration analyses are subsequently completed within two weeks of culture. We have successfully used these slice cultures to uncover genetic factors associated with increased migratory behavior in human GBM. Further, we have validated the model's ability to detect patient-specific variation in response to anti-migration therapies. Moving forward, human GBM slice cultures are an attractive platform for rapid ex vivo assessment of tumor sensitivity to therapeutic agents, in order to advance personalized neuro-oncologic therapy.

摘要

尽管进行了手术、化疗和放疗,胶质母细胞瘤(GBM)的临床预后仍然极差。肿瘤向周围脑实质的进行性侵袭是一个持久的治疗挑战。为了开发针对GBM的抗迁移疗法,提供生理相关背景以进行可控实验的模型系统至关重要。在此,我们展示了一种从手术切除获得的人类GBM组织生成切片培养物的方案。这些培养物允许进行体外实验,而无需通过动物异种移植或单细胞培养传代。此外,我们描述了结合细胞追踪使用延时激光扫描共聚焦显微镜来定量研究肿瘤细胞的迁移行为以及对治疗的相关反应。切片可在手术获取组织后的90分钟内重复生成。逆转录病毒介导的荧光细胞标记、共聚焦成像和肿瘤细胞迁移分析随后在培养的两周内完成。我们已成功使用这些切片培养物来揭示与人类GBM中迁移行为增加相关的遗传因素。此外,我们已验证该模型检测患者对抗迁移疗法反应的特异性差异的能力。展望未来,人类GBM切片培养物是一个有吸引力的平台,可用于快速体外评估肿瘤对治疗药物的敏感性,以推进个性化神经肿瘤治疗。

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