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肿瘤切片外植体的建立与分析作为诊断测试的前提条件

Establishment and Analysis of Tumor Slice Explants As a Prerequisite for Diagnostic Testing.

作者信息

Nagaraj Ashwini S, Bao Jie, Hemmes Annabrita, Machado Mafalda, Närhi Katja, Verschuren Emmy W

机构信息

Institute for Molecular Medicine Finland (FIMM), HiLIFE, University of Helsinki.

Institute for Molecular Medicine Finland (FIMM), HiLIFE, University of Helsinki;

出版信息

J Vis Exp. 2018 Nov 29(141). doi: 10.3791/58569.

Abstract

Organotypic primary tissue explant cultures, which include precision-cut slices, represent the three-dimensional (3-D) tissue architecture as well as the multicellular interactions of native tissue. Tissue slices immediately cut from freshly resected tumors preserve spatial aspects of intratumor heterogeneity (ITH), thus making them useful surrogates of in vivo biology. Careful optimization of tissue slice preparation and cultivation conditions is fundamental for the predictive diagnostic potential of tumor slice explants. In this regard, murine models are valuable, as these provide a consistent flow of tumor material to perform replicate and reproducible experiments. This protocol describes the culturing of murine lung tumor-derived tissue slices using a rotating incubation unit, a system that enables intermittent exposure of tissues to oxygen and nutrients. Our previous work showed that the use of rotating incubation units improves the viability of tissue compared to other culture methods, particularly floating slices and stagnant filter supports. Here, we further show that slice thickness influences the viability of cultured slices, suggesting that optimization of slice thickness should be done for different tissue types. Pronounced ITH in relevant oncogenic functions, such as signaling activities, stromal cell infiltration or expression of differentiation markers, necessitates evaluation of adjacent tissue slices for the expression of markers altered by drug treatment or cultivation itself. In summary, this protocol describes the generation of murine lung tumor slices and their culture on a rotating incubation unit and demonstrates how slices should be systematically analyzed for the expression of heterogeneous tissue markers, as a prerequisite prior to drug response studies.

摘要

器官型原代组织外植体培养,包括精密切片,代表了三维(3-D)组织结构以及天然组织的多细胞相互作用。从新鲜切除的肿瘤中立即切下的组织切片保留了肿瘤内异质性(ITH)的空间特征,因此使其成为体内生物学的有用替代物。仔细优化组织切片制备和培养条件对于肿瘤切片外植体的预测诊断潜力至关重要。在这方面,小鼠模型很有价值,因为它们提供了一致的肿瘤材料流以进行重复和可再现的实验。本方案描述了使用旋转培养装置培养小鼠肺肿瘤来源的组织切片,该系统能使组织间歇性暴露于氧气和营养物质中。我们之前的工作表明,与其他培养方法相比,使用旋转培养装置可提高组织的活力,特别是漂浮切片和静止滤膜支持物。在这里,我们进一步表明切片厚度会影响培养切片的活力,这表明应针对不同组织类型优化切片厚度。在相关致癌功能中,如信号传导活性、基质细胞浸润或分化标志物的表达,存在明显的ITH,因此有必要评估相邻组织切片中因药物治疗或培养本身而改变的标志物的表达。总之,本方案描述了小鼠肺肿瘤切片的生成及其在旋转培养装置上的培养,并展示了在进行药物反应研究之前,应如何系统分析切片中异质组织标志物的表达。

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