"Universal" vitrification of cells by ultra-fast cooling

Author:

Heo Yun Seok1,Nagrath Sunitha1,Moore Alessandra L.1,Zeinali Mahnaz1,Irimia Daniel1,Stott Shannon L.12,Toth Thomas L.3,Toner Mehmet1

Affiliation:

1. BioMEMS Resource Center, Massachusetts General Hospital, Harvard Medical School, and Shriners Hospital for Children, Boston, MA, USA

2. Massachusetts General Hospital, Cancer Center, Harvard Medical School, Boston, MA, USA

3. Massachusetts General Hospital, Obstetrics and Gynecology Services, Harvard Medical School, Boston, MA, USA

Abstract

Long-term preservation of live cells is critical for a broad range of clinical and research applications. With the increasing diversity of cells that need to be preserved (e.g. oocytes, stem and other primary cells, genetically modified cells), careful optimization of preservation protocols becomes tedious and poses significant limitations for all but the most expert users. To address the challenge of long-term storage of critical, heterogeneous cell types, we propose a universal protocol for cell vitrification that is independent of cell phenotype and uses only low concentrations of cryoprotectant (1.5 M PROH and 0.5 M trehalose). We employed industrial grade microcapillaries made of highly conductive fused silica, which are commonly used for analytical chemistry applications. The minimal mass and thermal inertia of the microcapillaries enabled us to achieve ultrafast cooling rates up to 4,000 K/s. Using the same low, non-toxic concentration of cryoprotectant, we demonstrate high recovery and viability rates after vitrification for human mammary epithelial cells, rat hepatocytes, tumor cells from pleural effusions, and multiple cancer cell lines.

Publisher

World Scientific Pub Co Pte Lt

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