Figure 1
Figure 1. Procedure for determining 2H enrichments in CD38+ and CD38− CLL cells and time point selection in relation to 2H availability in body water. (A) Deuterium enrichment measured in plasma of body water compartment of a representative case (CLL 875). CLL cells were flow-sorted at the 3 time points indicated by arrows. Vertical dashed line indicates time when 2H2O intake was ended. (B) After gating CD19+CD3− cells, CD5+ cells were flow-sorted based on their expression of CD38. 2H in genomic DNA was then measured by GC/MS. (C) The ratio of CD38+/CD38− fractions (f) of labeled cells (Table 2) was averaged. Bars represent SEs of the 3 time points studied. Significant differences in 2H incorporation between the CD38− and CD38+ B-CLL subpopulations were achieved early and maintained during labeling period, whereas they disappeared during washout.

Procedure for determining 2H enrichments in CD38+ and CD38 CLL cells and time point selection in relation to 2H availability in body water. (A) Deuterium enrichment measured in plasma of body water compartment of a representative case (CLL 875). CLL cells were flow-sorted at the 3 time points indicated by arrows. Vertical dashed line indicates time when 2H2O intake was ended. (B) After gating CD19+CD3 cells, CD5+ cells were flow-sorted based on their expression of CD38. 2H in genomic DNA was then measured by GC/MS. (C) The ratio of CD38+/CD38 fractions (f) of labeled cells (Table 2) was averaged. Bars represent SEs of the 3 time points studied. Significant differences in 2H incorporation between the CD38 and CD38+ B-CLL subpopulations were achieved early and maintained during labeling period, whereas they disappeared during washout.

Close Modal
This Feature Is Available To Subscribers Only

or Create an Account

Close Modal
Close Modal