Fig. 1.
Fig. 1. Bone marrow-CD34+ and CD34− cells were sorted for their CD19 respective subsets using CD34 FITC- and CD19 PE-conjugated antibodies. To increase the sensitivity of our PCR method at the lymphoid progenitor cell level, only cells with a lymphoblastoid appearance were sorted. The FACS setting of one representative patient (K.A.) is shown. Isotype control for CD34+ cells (A) and for CD34− cells (C) were included. Sorting gates for CD34+ cells (B) and CD34− cells (D) were set to clearly separate between CD19+ and CD19− cells.

Bone marrow-CD34+ and CD34 cells were sorted for their CD19 respective subsets using CD34 FITC- and CD19 PE-conjugated antibodies. To increase the sensitivity of our PCR method at the lymphoid progenitor cell level, only cells with a lymphoblastoid appearance were sorted. The FACS setting of one representative patient (K.A.) is shown. Isotype control for CD34+ cells (A) and for CD34 cells (C) were included. Sorting gates for CD34+ cells (B) and CD34 cells (D) were set to clearly separate between CD19+ and CD19 cells.

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