An Integrated Pipeline for High-throughput Screening and Profiling of Spheroids Using Simple Live Image Analysis of Frame to Frame Variations

Overview

Journal Methods

Specialty Biochemistry

Date 2020 May 25

PMID 32446959

Citations 7

Authors

Haneen Alsehli

Fuad Mosis

Christopher Thompson

Eva Hamrud

Erika Wiseman

Eileen Gentleman

Davide Danovi

Affiliations

Soon will be listed here.

Abstract

High-throughput imaging methods can be applied to relevant cell culture models, fostering their use in research and translational applications. Improvements in microscopy, computational capabilities and data analysis have enabled high-throughput, high-content approaches from endpoint 2D microscopy images. Nonetheless, trade-offs in acquisition, computation and storage between content and throughput remain, in particular when cells and cell structures are imaged in 3D. Moreover, live 3D phase contrast microscopy images are not often amenable to analysis because of the high level of background noise. Cultures of Human induced pluripotent stem cells (hiPSC) offer unprecedented scope to profile and screen conditions affecting cell fate decisions, self-organisation and early embryonic development. However, quantifying changes in the morphology or function of cell structures derived from hiPSCs over time presents significant challenges. Here, we report a novel method based on the analysis of live phase contrast microscopy images of hiPSC spheroids. We compare self-renewing versus differentiating media conditions, which give rise to spheroids with distinct morphologies; round versus branched, respectively. These cell structures are segmented from 2D projections and analysed based on frame-to-frame variations. Importantly, a tailored convolutional neural network is trained and applied to predict culture conditions from time-frame images. We compare our results with more classic and involved endpoint 3D confocal microscopy and propose that such approaches can complement spheroid-based assays developed for the purpose of screening and profiling. This workflow can be realistically implemented in laboratories using imaging-based high-throughput methods for regenerative medicine and drug discovery.

Citing Articles

Morphogen-driven differentiation is precluded by physical confinement in human iPSCs spheroids.

Alsehli H, Roy E, Williams T, Kuziola A, Guo Y, Dreiss C Front Bioeng Biotechnol. 2024; 12:1467412.

PMID: 39588360 PMC: 11586224. DOI: 10.3389/fbioe.2024.1467412.

Engineered organoids for biomedical applications.

de Barros N, Wang C, Maity S, Peirsman A, Nasiri R, Herland A Adv Drug Deliv Rev. 2023; 203:115142.

PMID: 37967768 PMC: 10842104. DOI: 10.1016/j.addr.2023.115142.

A deep learning-based pipeline for analyzing the influences of interfacial mechanochemical microenvironments on spheroid invasion using differential interference contrast microscopic images.

Ngo T, Yang S, Mao B, Nguyen T, Ng Q, Kuo Y Mater Today Bio. 2023; 23:100820.

PMID: 37810748 PMC: 10558776. DOI: 10.1016/j.mtbio.2023.100820.

Everything You Always Wanted to Know About Organoid-Based Models (and Never Dared to Ask).

Hautefort I, Poletti M, Papp D, Korcsmaros T Cell Mol Gastroenterol Hepatol. 2022; 14(2):311-331.

PMID: 35643188 PMC: 9233279. DOI: 10.1016/j.jcmgh.2022.04.012.

A multiparametric calcium signal screening platform using iPSC-derived cortical neural spheroids.

Boutin M, Strong C, Van Hese B, Hu X, Itkin Z, Chen Y SLAS Discov. 2022; 27(4):209-218.

PMID: 35092840 PMC: 9177534. DOI: 10.1016/j.slasd.2022.01.003.

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