REVIEW ARTICLE


Desiccation Tolerance of Adult Stem Cells in the Presence of Trehalose and Glycerol



Surbhi Mittal, Ram V. Devireddy*
Bioengineering Laboratory, Department of Mechanical Engineering, Louisiana State University, Baton Rouge, LA, USA

Article Information


Identifiers and Pagination:

Year: 2008
Volume: 2
First Page: 211
Last Page: 218
Publisher ID: TOBIOTJ-2-211
DOI: 10.2174/1874070700802010211

Article History:

Received Date: 14/03/2008
Revision Received Date: 08/07/2008
Acceptance Date: 09/07/2008
Electronic publication date: 25/7/2008
Collection year: 2008

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Creative Commons License
© 2008 Mittal and Devireddy

open-access license: This is an open access article distributed under the terms of the Creative Commons Attribution 4.0 International Public License (CC-BY 4.0), a copy of which is available at: (https://creativecommons.org/licenses/by/4.0/legalcode). This license permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.

* Address correspondence to this author at the Bioengineering Laboratory, Department of Mechanical Engineering, Louisiana State University, Baton Rouge, LA, USA; Tel: 1-225-578-5891; Fax: 1-225-578-5924; E-mail: devireddy@me.lsu.edu


Abstract

Development of protocols for storing desiccated cells at ambient temperatures offers tremendous economic and practical advantages over traditional storage procedures like cryopreservation and freeze-drying. As a first step for developing such procedures for adult stem cells, we have measured the post-rehydration membrane integrity (PRMI) of two passages, Passage-0 (P0) and Passage-1 (P1), of human adipose-derived stem cells (ASCs). ASCs were dried using a convective stage at three different drying rates (slow, moderate and rapid) in D-PBS with trehalose (50 mM) and glycerol (384 mM). ASCs were incubated in the drying media for 30 mins prior to drying at the prescribed rate on the convective stage for 30 mins. After drying, the ASCs were stored for 48 hrs in three different conditions: i) at ambient temperature, ii) in plastic bags at ambient temperature and iii) in vacuum sealed plastic bags at ambient temperature. PRMI was assessed after incubating the rehydrated ASCs with stromal medium for a further 48 hrs. Our measurements show that the PRMI of ASCs was: i) higher when ASCs were dried slowly; ii) increased when they were stored in vacuum as opposed to at ambient or in plastic bags; and iii) decreased with increasing passage of ASCs, i.e. under similar drying and storage conditions P0 ASCs had higher PRMI than P1 ASCs. Our results suggest that the best PRMI (37% for P0 ASCs and ~14% for P1 ASCs) can be achieved when the ASCs were dried slowly and stored in vacuum.