![Fig. 1. Cell sorting strategy and purity of sorted fractions. / Stained cells were sorted according to CD34 and CD38 expression (A) or DNA/RNA staining (B) by using a Coulter Elite flow cytometer. For cell sorting, immunomagnetic-purified CD34+ cells were gated on a first R1 region by selecting lymphomononuclear cells and excluding dead cells (FSC/SSC dot plot). A second region R2 corresponding to CD34+ cells was drawn on a second dot plot (CD34/SSC) gated on R1. (A) The CD34+CD38−fraction was arbitrarily defined according to the CD38 expression level as the 10% of CD34+ cells with the lowest CD38 labeling. Two gates corresponding to CD34+CD38− and to CD34+CD38+ fractions were defined (Ai and Aii, respectively). Five percent of cells at the limits between these populations were excluded from the sort. (B) CD34+ cells were also sorted according to simultaneous DNA/RNA staining with Hoechst 33342 and pyronin Y. This cell cycle fractionation allowed isolation of viable [G0] CD34+ cells from [G1+S+G2/M] cells. Cells residing in G0 exhibit a low RNA content and appear at the bottom of the Hoechst/pyronin Y dot plot identified by a low pyronin Y and a low Hoechst staining (Bi). Cells in G1 show a brighter pyronin Y signal associated with a low Hoechst staining and cells in S+G2/M display both high Hoechst and pyronin Y staining. Two gates were defined corresponding to [G0] CD34+cells and to [G1+S+G2/M] CD34+ cells (Bi and Bii, respectively). The purity of the CD34+CD38−, CD34+CD38+, [G0] CD34+, and [G1+S+G2/M] CD34+ sorted fractions was more than 99% as established by the flow cytometry analysis following sorting. A representative analysis of each sorted fraction cell purity was shown on histograms of CD38 and pyronin Y fluorescences (Ai, Aii and Bi, Bii).](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/99/4/10.1182_blood.v99.4.1117/6/h80422156001.jpeg?Expires=1725125972&Signature=Ppb0hDS2nSKHfr6DFP2AGDLnUKo4aDjTVUef0lZ~WDTRPQ2Z-G3MOFgk~1Fx17-ghh617lboAy8J1OM3wW1IOSiPJVhQ9atcXG0gug~n8XhdIxnH9xoOwphf-U9AYBnQb1eRu063hEF4cus7Z6~IEGqFmEG0~2M7gz5AH2aOoNWJ4lqu-xdz5hp4QMffgF5CsGdDH7e1XzMy42dmYKYswa7BEJcQnindZ4dR2FWP9Z8~nq8auoxEKbg~-jrzbqcQ~4TdkbtLEFRsvg1X5W16W5vUQxgsFK11kC4wDG4KzIEruBzYNGS3RYxJ20ZJeLEdF04sn8aM3U2XW89TRKakow__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
Cell sorting strategy and purity of sorted fractions.
Stained cells were sorted according to CD34 and CD38 expression (A) or DNA/RNA staining (B) by using a Coulter Elite flow cytometer. For cell sorting, immunomagnetic-purified CD34+ cells were gated on a first R1 region by selecting lymphomononuclear cells and excluding dead cells (FSC/SSC dot plot). A second region R2 corresponding to CD34+ cells was drawn on a second dot plot (CD34/SSC) gated on R1. (A) The CD34+CD38−fraction was arbitrarily defined according to the CD38 expression level as the 10% of CD34+ cells with the lowest CD38 labeling. Two gates corresponding to CD34+CD38− and to CD34+CD38+ fractions were defined (Ai and Aii, respectively). Five percent of cells at the limits between these populations were excluded from the sort. (B) CD34+ cells were also sorted according to simultaneous DNA/RNA staining with Hoechst 33342 and pyronin Y. This cell cycle fractionation allowed isolation of viable [G0] CD34+ cells from [G1+S+G2/M] cells. Cells residing in G0 exhibit a low RNA content and appear at the bottom of the Hoechst/pyronin Y dot plot identified by a low pyronin Y and a low Hoechst staining (Bi). Cells in G1 show a brighter pyronin Y signal associated with a low Hoechst staining and cells in S+G2/M display both high Hoechst and pyronin Y staining. Two gates were defined corresponding to [G0] CD34+cells and to [G1+S+G2/M] CD34+ cells (Bi and Bii, respectively). The purity of the CD34+CD38−, CD34+CD38+, [G0] CD34+, and [G1+S+G2/M] CD34+ sorted fractions was more than 99% as established by the flow cytometry analysis following sorting. A representative analysis of each sorted fraction cell purity was shown on histograms of CD38 and pyronin Y fluorescences (Ai, Aii and Bi, Bii).
