Abstract 239: Integrated computational image analysis of cellular and acellular tissue components as a method for detailed tumor tissue mapping and structural patterns recognition

G. Vasiukov, Tatiana Novitskaya, M. Senosain, A. Menshikh, A. Zijlstra, S. Novitskiy, P. Massion
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Abstract

Tumor microenvironment (TME) represents an integrated system that affects cancer cell behavior and contributes directly to disease outcome. Systemic approach to analysis of TME should uncover its complexity and facilitate discovery of mechanisms orchestrating tumor development and metastasis. Multiplex fluorescence tissue staining followed by spatial analysis of tumor tissue architecture can provide insights to pivotal interactions of cellular and acellular components of TME. Extracellular matrix (ECM is represented mainly by collagen deposition. Number of reports indicates that ECM contribution to TME state not only depends upon amount of accumulated collagen but its geometrical features and spatial orientation of fibers. These characteristics of collagen fibers contribute directly to physical and mechanical properties of tissue and can change tumor growth and metastasis. Current methods of computational image analysis of tissue implement assessment of cellular or acellular components separately. The goal of current work was to develop a new computational tool to perform integrated analysis of fibrous and cellular components of tumor tissue in spatial dependent manner to achieve detailed tumor tissue mapping and structural patterns recognition. To pursue this goal, we generated images of human lung adenocarcinoma tissue characterized by indolent and aggressive behavior. We performed multiplex immunofluorescence staining for following markers: CD3 - marker of T-lymphocytes, PanCytokeratin - marker of epithelial/tumor cells, collagen hybridizing peptide (3Helix) - marker of collagen, DAPI - nuclear counterstain. To develop image analysis pipeline, we utilized an open source graphical interface analytical platform KNIME, where we generated modular workflow. For ECM analysis, we integrated Python written code into KNIME node. Segmentation of collagen fibers was performed using skeletonization with subsequent calculation of geometrical properties (length, alignment, widths) and orientation of each fiber. Data, collected from single cell analysis and ECM architecture assessment, were combined and forwarded to downstream spatial analysis, where distances from cell to cell or cell to ECM were computed and neighborhood analysis was performed. We demonstrated that tumor cells in aggressive adenocarcinoma samples were co-localized with a smaller number of collagen fibers. In addition, length of that fibers was less in comparison to indolent group. Correlation analysis revealed positive correlation between length of collagen fibers and number of tumor cells in indolent group, but we did not observe this phenomenon in indolent group. Developed computational method provides additional dimensionality to tissue image analysis and can reveal underrecognized structural patterns of the tumor microenvironment. Citation Format: Georgii Vasiukov, Tatiana Novitskaya, Maria-Fernanda Senosain, Anna Menshikh, Andries Zijlstra, Sergey Novitskiy, Pierre Massion. Integrated computational image analysis of cellular and acellular tissue components as a method for detailed tumor tissue mapping and structural patterns recognition [abstract]. In: Proceedings of the American Association for Cancer Research Annual Meeting 2021; 2021 Apr 10-15 and May 17-21. Philadelphia (PA): AACR; Cancer Res 2021;81(13_Suppl):Abstract nr 239.
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239:细胞和非细胞组织成分的集成计算图像分析作为详细肿瘤组织定位和结构模式识别的方法
肿瘤微环境(Tumor microenvironment, TME)是一个影响癌细胞行为并直接影响疾病预后的综合系统。系统的方法分析TME应该揭示其复杂性,并有助于发现协调肿瘤发展和转移的机制。多重荧光组织染色,然后对肿瘤组织结构进行空间分析,可以为TME细胞和非细胞成分的关键相互作用提供见解。细胞外基质(ECM)主要以胶原沉积为代表。大量报道表明,ECM对TME状态的贡献不仅取决于胶原积累的数量,还取决于其几何特征和纤维的空间取向。胶原纤维的这些特性直接影响组织的物理和机械特性,并能改变肿瘤的生长和转移。目前的组织计算图像分析方法分别对细胞或非细胞成分进行评估。目前的工作目标是开发一种新的计算工具,以空间依赖的方式对肿瘤组织的纤维和细胞成分进行综合分析,以实现详细的肿瘤组织制图和结构模式识别。为了实现这一目标,我们生成了以惰性和侵袭性行为为特征的人肺腺癌组织图像。我们对以下标记物进行多重免疫荧光染色:t淋巴细胞CD3标记物,上皮/肿瘤细胞PanCytokeratin标记物,胶原杂交肽(3Helix) -胶原标记物,DAPI -核反染。为了开发图像分析管道,我们利用了开源图形界面分析平台KNIME,并在该平台上生成了模块化的工作流程。为了进行ECM分析,我们将Python编写的代码集成到KNIME节点中。使用骨架化对胶原纤维进行分割,随后计算每根纤维的几何特性(长度、排列、宽度)和方向。从单细胞分析和ECM架构评估中收集的数据被合并并转发给下游空间分析,在那里计算细胞到细胞或细胞到ECM的距离,并进行邻域分析。我们证明侵袭性腺癌样本中的肿瘤细胞与较少数量的胶原纤维共定位。此外,这些纤维的长度也比惰性组短。相关分析显示,慵懒组胶原纤维长度与肿瘤细胞数呈正相关,而慵懒组未见此现象。开发的计算方法为组织图像分析提供了额外的维度,可以揭示肿瘤微环境的未被识别的结构模式。引文格式:Georgii Vasiukov, Tatiana Novitskaya, Maria-Fernanda Senosain, Anna Menshikh, Andries Zijlstra, Sergey Novitskiy, Pierre Massion。细胞和非细胞组织成分的集成计算图像分析作为详细肿瘤组织定位和结构模式识别的方法[摘要]。见:美国癌症研究协会2021年年会论文集;2021年4月10日至15日和5月17日至21日。费城(PA): AACR;癌症杂志,2021;81(13 -增刊):摘要nr 239。
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