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Zooming in on Cryopreservation of hiPSCs and Neural Derivatives: A Dual‐Center Study Using Adherent Vitrification

Human induced pluripotent stem cells (hiPSCs) are an important tool for research and regenerative medicine, but their efficient cryopreservation remains a major challenge. The current gold standard is slow‐rate freezing of dissociated colonies in suspension, but low recovery rates limit immediate po...

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Autores principales: Kaindl, Johanna, Meiser, Ina, Majer, Julia, Sommer, Annika, Krach, Florian, Katsen‐Globa, Alisa, Winkler, Jürgen, Zimmermann, Heiko, Neubauer, Julia C., Winner, Beate
Formato: Online Artículo Texto
Lenguaje:English
Publicado: John Wiley & Sons, Inc. 2018
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6392398/
https://www.ncbi.nlm.nih.gov/pubmed/30456912
http://dx.doi.org/10.1002/sctm.18-0121
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author Kaindl, Johanna
Meiser, Ina
Majer, Julia
Sommer, Annika
Krach, Florian
Katsen‐Globa, Alisa
Winkler, Jürgen
Zimmermann, Heiko
Neubauer, Julia C.
Winner, Beate
author_facet Kaindl, Johanna
Meiser, Ina
Majer, Julia
Sommer, Annika
Krach, Florian
Katsen‐Globa, Alisa
Winkler, Jürgen
Zimmermann, Heiko
Neubauer, Julia C.
Winner, Beate
author_sort Kaindl, Johanna
collection PubMed
description Human induced pluripotent stem cells (hiPSCs) are an important tool for research and regenerative medicine, but their efficient cryopreservation remains a major challenge. The current gold standard is slow‐rate freezing of dissociated colonies in suspension, but low recovery rates limit immediate post‐thawing applicability. We tested whether ultrafast cooling by adherent vitrification improves post‐thawing survival in a selection of hiPSCs and small molecule neural precursor cells (smNPCs) from Parkinson's disease and controls. In a dual‐center study, we compared the results by immunocytochemistry (ICC), fluorescence‐activated cell sorting analysis, and RNA‐sequencing (RNA‐seq). Adherent vitrification was achieved in the so‐called TWIST substrate, a device combining cultivation, vitrification, storage, and post‐thawing cultivation. Adherent vitrification resulted in preserved confluency and significantly higher cell numbers, and viability at day 1 after thawing, while results were not significantly different at day 4 after thawing. RNA‐seq and ICC of hiPSCs revealed no change in gene expression and pluripotency markers, indicating that physical damage of slow‐rate freezing disrupts cellular membranes. Scanning electron microscopy showed preserved colony integrity by adherent vitrification. Experiments using smNPCs demonstrated that adherent vitrification is also applicable to neural derivatives of hiPSCs. Our data suggest that, compared to the state‐of‐the‐art slow‐rate freezing in suspension, adherent vitrification is an improved cryopreservation technique for hiPSCs and derivatives. stem cells translational medicine 2019;8:247&259
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spelling pubmed-63923982019-03-07 Zooming in on Cryopreservation of hiPSCs and Neural Derivatives: A Dual‐Center Study Using Adherent Vitrification Kaindl, Johanna Meiser, Ina Majer, Julia Sommer, Annika Krach, Florian Katsen‐Globa, Alisa Winkler, Jürgen Zimmermann, Heiko Neubauer, Julia C. Winner, Beate Stem Cells Transl Med Enabling Technologies for Cell‐Based Clinical Translation Human induced pluripotent stem cells (hiPSCs) are an important tool for research and regenerative medicine, but their efficient cryopreservation remains a major challenge. The current gold standard is slow‐rate freezing of dissociated colonies in suspension, but low recovery rates limit immediate post‐thawing applicability. We tested whether ultrafast cooling by adherent vitrification improves post‐thawing survival in a selection of hiPSCs and small molecule neural precursor cells (smNPCs) from Parkinson's disease and controls. In a dual‐center study, we compared the results by immunocytochemistry (ICC), fluorescence‐activated cell sorting analysis, and RNA‐sequencing (RNA‐seq). Adherent vitrification was achieved in the so‐called TWIST substrate, a device combining cultivation, vitrification, storage, and post‐thawing cultivation. Adherent vitrification resulted in preserved confluency and significantly higher cell numbers, and viability at day 1 after thawing, while results were not significantly different at day 4 after thawing. RNA‐seq and ICC of hiPSCs revealed no change in gene expression and pluripotency markers, indicating that physical damage of slow‐rate freezing disrupts cellular membranes. Scanning electron microscopy showed preserved colony integrity by adherent vitrification. Experiments using smNPCs demonstrated that adherent vitrification is also applicable to neural derivatives of hiPSCs. Our data suggest that, compared to the state‐of‐the‐art slow‐rate freezing in suspension, adherent vitrification is an improved cryopreservation technique for hiPSCs and derivatives. stem cells translational medicine 2019;8:247&259 John Wiley & Sons, Inc. 2018-11-19 /pmc/articles/PMC6392398/ /pubmed/30456912 http://dx.doi.org/10.1002/sctm.18-0121 Text en © 2018 The Authors stem cells translational medicine published by Wiley Periodicals, Inc. on behalf of AlphaMed Press This is an open access article under the terms of the http://creativecommons.org/licenses/by-nc-nd/4.0/ License, which permits use and distribution in any medium, provided the original work is properly cited, the use is non‐commercial and no modifications or adaptations are made.
spellingShingle Enabling Technologies for Cell‐Based Clinical Translation
Kaindl, Johanna
Meiser, Ina
Majer, Julia
Sommer, Annika
Krach, Florian
Katsen‐Globa, Alisa
Winkler, Jürgen
Zimmermann, Heiko
Neubauer, Julia C.
Winner, Beate
Zooming in on Cryopreservation of hiPSCs and Neural Derivatives: A Dual‐Center Study Using Adherent Vitrification
title Zooming in on Cryopreservation of hiPSCs and Neural Derivatives: A Dual‐Center Study Using Adherent Vitrification
title_full Zooming in on Cryopreservation of hiPSCs and Neural Derivatives: A Dual‐Center Study Using Adherent Vitrification
title_fullStr Zooming in on Cryopreservation of hiPSCs and Neural Derivatives: A Dual‐Center Study Using Adherent Vitrification
title_full_unstemmed Zooming in on Cryopreservation of hiPSCs and Neural Derivatives: A Dual‐Center Study Using Adherent Vitrification
title_short Zooming in on Cryopreservation of hiPSCs and Neural Derivatives: A Dual‐Center Study Using Adherent Vitrification
title_sort zooming in on cryopreservation of hipscs and neural derivatives: a dual‐center study using adherent vitrification
topic Enabling Technologies for Cell‐Based Clinical Translation
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6392398/
https://www.ncbi.nlm.nih.gov/pubmed/30456912
http://dx.doi.org/10.1002/sctm.18-0121
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