Creating Matched In vivo/In vitro Patient-Derived Model Pairs of PDX and PDX-Derived Organoids for Cancer Pharmacology Research

被引:7
|
作者
Xu, Xiaoxi [1 ]
Shang, Limei [1 ]
Wang, Philip [2 ]
Zhou, Jun [2 ]
Ouyang, Xuesong [2 ]
Zheng, Meiling [1 ]
Mao, Binchen [2 ]
Zhang, Likun [2 ]
Chen, Bonnie [1 ]
Wang, Jingjing [2 ]
Chen, Jing [3 ]
Qian, Wubin [2 ]
Guo, Sheng [2 ]
Huang, Yujun [2 ]
Li, Qi-Xiang [3 ]
机构
[1] Crown Biosci Inc, Beijing, Peoples R China
[2] Crown Biosci Inc, Taicang, Jiangsu, Peoples R China
[3] Crown Biosci Inc, San Diego, CA 92127 USA
来源
关键词
TUMOR XENOGRAFTS; STEM-CELLS; CETUXIMAB; PREDICT; BIOBANK;
D O I
10.3791/61382
中图分类号
O [数理科学和化学]; P [天文学、地球科学]; Q [生物科学]; N [自然科学总论];
学科分类号
07 ; 0710 ; 09 ;
摘要
Patient-derived tumor xenografts (PDXs) are considered the most predictive preclinical models, largely believed to be driven by cancer stem cells (CSC) for conventional cancer drug evaluation. A large library of PDXs is reflective of the diversity of patient populations and thus enables population based preclinical trials ("Phase II-like mouse clinical trials"); however, PDX have practical limitations of low throughput, high costs and long duration. Tumor organoids, also being patient-derived CSC-driven models, can be considered as the in vitro equivalent of PDX, overcoming certain PDX limitations for dealing with large libraries of organoids or compounds. This study describes a method to create PDX-derived organoids (PDXO), thus resulting in paired models for in vitro and in vivo pharmacology research. Subcutaneously-transplanted PDX-CR2110 tumors were collected from tumor-bearing mice when the tumors reached 200-800 mm(3), per an approved autopsy procedure, followed by removal of the adjacent non-tumor tissues and dissociation into small tumor fragments. The small tumor fragments were washed and passed through a 100 mu m cell strainer to remove the debris. Cell clusters were collected and suspended in basement membrane extract (BME) solution and plated in a 6-well plate as a solid droplet with surrounding liquid media for growth in a CO2 incubator. Organoid growth was monitored twice weekly under light microscopy and recorded by photography, followed by liquid medium change 2 or 3 times a week. The grown organoids were further passaged (7 days later) at a 1:2 ratio by disrupting the BME embedded organoids using mechanical shearing, aided by addition of trypsin and the addition of 10 mu M Y-27632. Organoids were cryopreserved in cryo-tubes for long-term storage, after release from BME by centrifugation, and also sampled (e.g., DNA, RNA and FFPE block) for further characterization.
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页数:11
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