Microbial contamination of cord blood stem cells

Background and Objectives After storage, low levels of contaminating bacteria in standard blood components can reach bacteraemic levels, causing severe transfusion‐associated sepsis. For cord blood (CB), the significance of low levels of contaminating bacteria and the optimal detection method is unknown and not supported by available guidelines. Materials and Methods Spiking experiments and testing of various subfractions of CB units were used to determine the behaviour of bacteria during centrifugation, freezing and thawing. For routine testing of CB, different volumes were compared for the detection of potential pathogens and micro‐organisms of low pathogenicity. Results Centrifugation, as applied to CB fractionation, does not show concentration of bacteria in any particular fraction and supports the possibility of culture of waste fractions. Dimethylsulphoxide (DMSO) and freezing does not affect the viability of bacteria under the conditions used in this study. Owing to the low contamination level, a large sample volume of 20 ml was more sensitive than a 10‐ml sample volume. Eighty five per cent of the isolated strains can be considered to be of low pathogenicity. Conclusion When an optimal waste fraction sample volume of 20 ml was cultured, the contamination rate of CB was found to be ≈ 13%, with low levels of < 1 colony‐forming unit (CFU)/ml. Such levels of bacteria of low pathogenicity are expected to be of clinical importance only when CB is expanded in vitro for a prolonged period of time.