Histo-pillar strip for optimal histogel block construction and biomarker analysis in 3D-lung cancer patient-derived organoids.

IF 8.2 2区 医学 Q1 ENGINEERING, BIOMEDICAL
Sang-Yun Lee, Eunyoung Lee, Ji-O Ryu, Kyuhwan Kim, Yongki Hwang, Bosung Ku, Seok Whan Moon, Mi Hyoung Moon, Kyung Soo Kim, Kwanyong Hyun, Jeong Uk Lim, Chan Kwon Park, Sung Won Kim, Chang Dong Yeo, Dong Woo Lee, Seung Joon Kim
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Abstract

This study proposed an optimized histogel construction method for histological analysis by applying lung cancer patient-derived organoids (PDOs) to the developed histo-pillar strip. Previously, there is the cultured PDOs damage problem during the histogel construction due to forced detachment of the Matrigel spots from the 96-well plate bottom. To address this issue, we cultured PDO on the proposed Histo-pillar strips and then immersed them in 4% paraformaldehyde fixation solution to self-isolate PDO without damage. The 4μl patient-derived cell (PDC)/Matrigel mixtures were dispensed on the surface of a U-shaped histo-pillar strip, and the PDCs were aggregated by gravity and cultured into PDOs. Cultured PDOs were self-detached by simply immersing them in a paraformaldehyde fixing solution without physical processing, showing about two times higher cell recovery rate than conventional method. In addition, we proposed a method for embedding PDOs under conditions where the histogel temperature was maintained such that the histogel did not harden, thereby improving the problem of damaging the histogel block in the conventional sandwich histogel construction method. We performed histological and genotyping analyses using tumor tissues and PDOs from two patients with lung adenocarcinoma. Therefore, the PDO culture and improved histogel block construction method using the histo-pillar strip proposed in this study can be employed as useful tools for the histological analysis of a limited number of PDCs.

在三维肺癌患者衍生器官组织中优化组织凝胶块构建和生物标记分析的组织柱条。
本研究提出了一种用于组织学分析的优化组织凝胶构建方法,将肺癌患者衍生的器官组织(PDOs)应用于开发的组织柱条带。以前,在构建组织凝胶的过程中,由于 matrigel 点与 96 孔板底部的强制分离,存在培养的 PDOs 损坏问题。为了解决这个问题,我们在拟议的组织柱条上培养 PDO,然后将其浸入 4% 多聚甲醛固定液中,使 PDO 自我隔离而不受损伤。将 4 μL 患者衍生细胞(PDC)/Matrigel 混合物分配到 U 形组织柱条带表面,PDC 在重力作用下聚集并培养成 PDO。将培养好的 PDOs 浸入多聚甲醛固定液中即可自行脱落,无需物理处理,细胞回收率比传统方法高出约两倍。此外,我们还提出了一种包埋 PDO 的方法,即在保持组凝胶温度的条件下,组凝胶不会变硬,从而改善了传统三明治组凝胶构建方法中组凝胶块受损的问题。我们利用两名肺腺癌患者的肿瘤组织和 PDO 进行了组织学和基因分型分析。因此,本研究提出的 PDO 培养和使用组织柱条的改进型组织凝胶块构建方法可作为有用的工具,用于对有限数量的 PDC 进行组织学分析。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
Biofabrication
Biofabrication ENGINEERING, BIOMEDICAL-MATERIALS SCIENCE, BIOMATERIALS
CiteScore
17.40
自引率
3.30%
发文量
118
审稿时长
2 months
期刊介绍: Biofabrication is dedicated to advancing cutting-edge research on the utilization of cells, proteins, biological materials, and biomaterials as fundamental components for the construction of biological systems and/or therapeutic products. Additionally, it proudly serves as the official journal of the International Society for Biofabrication (ISBF).
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