Autor: |
Radke TF; Institute of Transplantation Diagnostics and Cell Therapeutics, Heinrich Heine University Medical Center, Moorenstra β e 5, 40225 Düsseldorf, Germany., Barbosa D, Duggleby RC, Saccardi R, Querol S, Kögler G |
Jazyk: |
angličtina |
Zdroj: |
Stem cells international [Stem Cells Int] 2013; Vol. 2013, pp. 823912. Date of Electronic Publication: 2013 Mar 07. |
DOI: |
10.1155/2013/823912 |
Abstrakt: |
The assessment of nonviable haematopoietic cells by Annexin V staining method in flow cytometry has recently been published by Duggleby et al. Resulting in a better correlation with the observed colony formation in methylcellulose assays than the standard ISHAGE protocol, it presents a promising method to predict cord blood potency. Herein, we applied this method for examining the parameters during processing which potentially could affect cord blood viability. We could verify that the current standards regarding time and temperature are sufficient, since no significant difference was observed within 48 hours or in storage at 4°C up to 26°C. However, the addition of DMSO for cryopreservation alone leads to an inevitable increase in nonviable haematopoietic stem cells from initially 14.8% ± 4.3% to at least 30.6% ± 5.5%. Furthermore, CFU-assays with varied seeding density were performed in order to evaluate the applicability as a quantitative method. The results revealed that only in a narrow range reproducible clonogenic efficiency (ClonE) could be assessed, giving at least a semiquantitative estimation. We conclude that both Annexin V staining method and CFU-assays with defined seeding density are reliable means leading to a better prediction of the final potency. Especially Annexin V, due to its fast readout, is a practical tool for examining and optimising specific steps in processing, while CFU-assays add a functional confirmation. |
Databáze: |
MEDLINE |
Externí odkaz: |
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