No significant reduction in cervical cell viability was observed

No significant reduction in cervical cell viability was observed in the samples that were subjected to a delayed processing compared to those processed immediately ( Table 2). Because of the low yield of cells that can be recovered by cytobrush from the female genital tract (Nkwanyana et al., 2009), few studies have evaluated the feasibility and impact of cryopreservation on cell recovery and viability. We compared the number of CD3+

T cells isolated from the cervical cytobrushes of 13 HIV-infected women before and after storage in liquid nitrogen. In these samples, the median CD3+ T cell number obtained ex vivo was 75 280 (IQR 37 240–90 560), while Microbiology inhibitor a significantly lower median of 22 664 [(IQR 13 968–44 672); 48.7% recovery; p = 0.005] was recovered after thawing. Measurements of CD3+ event counts after ICS or CD3+ T cell numbers by Guava similarly showed that T cell numbers were relatively stable over the 24 h period at 37 °C, 4 °C and room temperature but

that there was a significantly lower T cell yield after cryopreservation. Annexin V and PI staining were used to evaluate the viability of CD3+ T cells before freezing and after thawing (Fig. 1). Fig. 1A shows a representative plot of Annexin V versus PI staining of CD3+ T cells from a cervical cytobrush sample. A median value of 99.5% (IQR 96.16–100.0%) of cervical cytobrush-derived CD3+ cells were viable ex vivo; of which, 18.3% co-expressed the late apoptotic markers Annexin V and PI (IQR 6.5–44.3%), 9.8% expressed Annexin V only and not PI indicating early apoptosis (IQR 3.3–15.7%; Annexin + PI−), while 61.4% were not apoptotic and lacked Epacadostat supplier expression of either marker ( Fig. 1B; IQR 39.3–82.60%). We found that only a small proportion of the cervical T cells were dead [1.0% Annexin V-PI+; IQR 0–3.2%; Fig. 1B]. After thawing cervical cytobrush cells taken from HIV-infected women, we found that 96.9% (IQR 89.3–99.4) Thiamine-diphosphate kinase of CD3+ cells recovered were viable and a comparable proportion of thawed cells expressed early or late apoptotic markers Annexin V and PI as found on ex vivo T cells ( Fig. 1B).

If thawed cells were rested overnight (as is a common practise with thawed PBMCs prior to functional analysis), we found that the majority of CD3+ T cells were co-expressing late apoptotic markers Annexin V and PI (78.5% IQR 78.3–78.6) indicating that they were in the process of undergoing apoptosis. When we compared the impact of thawing and resting on cervical cytobrush cell viability from women who were not infected with HIV ( Fig. 1B; n = 2), we found that viability of thawed cells was comparable to HIV-infected women but that CD3+ T cells from uninfected women did not exhibit the massive increase in expression of apoptotic markers after resting as was noted in cytobrush samples from HIV-infected women. From this data, conducting analyses on HIV-infected samples is best performed immediately after thawing.

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