A method for reproducible high‐resolution imaging of 3D cancer cell spheroids

Author:

Phillips Thomas A.1,Caprettini Valeria2,Aggarwal Nandini13,Marcotti Stefania1,Tetley Rob4,Mao Yanlan4,Shaw Tanya3,Chiappini Ciro2,Parsons Maddy1ORCID,Cox Susan1

Affiliation:

1. Randall Centre for Cell and Molecular Biophysics King's College London London UK

2. Centre for Craniofacial & Regenerative Biology King's College London London UK

3. Department of Inflammation Biology School of Immunology & Microbial Sciences King's College London London UK

4. Laboratory for Molecular Cell Biology and Institute for the Physics of Living Systems University College London London UK

Abstract

AbstractMulticellular tumour cell spheroids embedded within three‐dimensional (3D) hydrogels or extracellular matrices (ECM) are widely used as models to study cancer growth and invasion. Standard methods to embed spheroids in 3D matrices result in random placement in space which limits the use of inverted fluorescence microscopy techniques, and thus the resolution that can be achieved to image molecular detail within the intact spheroid. Here, we leverage UV photolithography to microfabricate PDMS (polydimethylsiloxane) stamps that allow for generation of high‐content, reproducible well‐like structures in multiple different imaging chambers. Addition of multicellular tumour spheroids into stamped collagen structures allows for precise positioning of spheroids in 3D space for reproducible high‐/super‐resolution imaging. Embedded spheroids can be imaged live or fixed and are amenable to immunostaining, allowing for greater flexibility of experimental approaches. We describe the use of these spheroid imaging chambers to analyse cell invasion, cell–ECM interaction, ECM alignment, force‐dependent intracellular protein dynamics and extension of fine actin‐based protrusions with a variety of commonly used inverted microscope platforms. This method enables reproducible, high‐/super‐resolution live imaging of multiple tumour spheroids, that can be potentially extended to visualise organoids and other more complex 3D in vitro systems.

Funder

Medical Research Council

Publisher

Wiley

Subject

Histology,Pathology and Forensic Medicine

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