Tumor-on-a-chip platform to interrogate the role of macrophages in tumor progression.

IF 1.5 4区生物学 Q4 CELL BIOLOGY Integrative Biology Pub Date : 2020-09-30 DOI:10.1093/intbio/zyaa017

Ye Bi, Venktesh S Shirure, Ruiyang Liu, Cassandra Cunningham, Li Ding, J Mark Meacham, S Peter Goedegebuure, Steven C George, Ryan C Fields

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Abstract

Tumor-infiltrating leukocytes, in particular macrophages, play an important role in tumor behavior and clinical outcome. The spectrum of macrophage subtypes ranges from antitumor 'M1'-type to protumor 'M2'-type macrophages. Tumor-associated macrophages (TAMs) typically display phenotypic features of both M1 and M2, and the population distribution is thought to be dynamic and evolves as the tumor progresses. However, our understanding of how TAMs impact the tumor microenvironment remains limited by the lack of appropriate 3D in vitro models that can capture cell-cell dynamics at high spatial and temporal resolution. Using our recently developed microphysiological 'tumor-on-a-chip' (TOC) device, we present here our findings on the impact of defined macrophage subsets on tumor behavior. The TOC device design contains three adjacent and connected chambers in which both the upper and lower chambers are loaded with tumor cells, whereas the central chamber contains a dynamic, perfused, living microvascular network. Introduction of human pancreatic or colorectal cancer cells together with M1-polarized macrophages significantly inhibited tumor growth and tumor-induced angiogenesis. Protein analysis and antibody-based neutralization studies confirmed that these effects were mediated through production of C-X-C motif chemokines (CXCL9), CXCL10 and CXCL11. By contrast, M2-macrophages mediated increased tumor cell migration into the vascularized chamber and did not inhibit tumor growth or angiogenesis. In fact, single-cell RNA sequencing showed that M2 macrophages further segregated endothelial cells into two distinct subsets, corresponding to static cells in vessels versus active cells involved in angiogenesis. The impact of M2 macrophages was mediated mostly by production of matrix metalloproteinase 7 and angiopoietin 2. In summary, our data demonstrate the utility of the TOC device to mechanistically probe biological questions in a 3D in vitro microenvironment.

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肿瘤芯片平台询问巨噬细胞在肿瘤进展中的作用。

肿瘤浸润性白细胞，特别是巨噬细胞，在肿瘤行为和临床结果中起着重要作用。巨噬细胞的亚型范围从抗肿瘤的M1型到肿瘤的M2型。肿瘤相关巨噬细胞(tam)通常表现出M1和M2的表型特征，其种群分布被认为是动态的，并随着肿瘤的进展而演变。然而，我们对tam如何影响肿瘤微环境的理解仍然受到缺乏适当的3D体外模型的限制，这些模型可以在高空间和时间分辨率下捕获细胞-细胞动力学。使用我们最近开发的微生理“肿瘤芯片”(TOC)设备，我们在这里介绍了我们关于定义的巨噬细胞亚群对肿瘤行为影响的研究结果。TOC装置设计包含三个相邻和连接的腔室，其中上下腔室都装载肿瘤细胞，而中央腔室包含一个动态的、灌注的、活的微血管网络。将人胰腺癌或结直肠癌细胞与m1极化巨噬细胞一起引入，可显著抑制肿瘤生长和肿瘤诱导的血管生成。蛋白分析和基于抗体的中和研究证实，这些作用是通过产生C-X-C基序趋化因子(CXCL9)、CXCL10和CXCL11介导的。相比之下，m2 -巨噬细胞介导的肿瘤细胞向血管化腔的迁移增加，不抑制肿瘤生长或血管生成。事实上，单细胞RNA测序显示M2巨噬细胞进一步将内皮细胞分成两个不同的亚群，分别是血管中的静态细胞和参与血管生成的活性细胞。M2巨噬细胞的影响主要通过产生基质金属蛋白酶7和血管生成素2介导。总之，我们的数据证明了TOC装置在体外三维微环境中机械地探测生物学问题的实用性。

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来源期刊

Integrative Biology 生物-细胞生物学

CiteScore

4.90

自引率

0.00%

发文量

审稿时长

1 months

期刊介绍： Integrative Biology publishes original biological research based on innovative experimental and theoretical methodologies that answer biological questions. The journal is multi- and inter-disciplinary, calling upon expertise and technologies from the physical sciences, engineering, computation, imaging, and mathematics to address critical questions in biological systems. Research using experimental or computational quantitative technologies to characterise biological systems at the molecular, cellular, tissue and population levels is welcomed. Of particular interest are submissions contributing to quantitative understanding of how component properties at one level in the dimensional scale (nano to micro) determine system behaviour at a higher level of complexity. Studies of synthetic systems, whether used to elucidate fundamental principles of biological function or as the basis for novel applications are also of interest.