Fig. 8.
Fig. 8. The effect of PKC- and PKC-β2 ribozymes on CD34+ cells cultured with EPO and SCF. / The CD34+ cells were incubated at 30 000 cells/well in flat-bottomed, 96 well plates with PKC-α ribozyme (2 μmol/L), PKC-β2 ribozyme (2 μmol/L), or medium for 24 hours and then stimulated with EPO (5 U/mL) and SCF (50 ng/mL.). (A) Cells were stained with the indicated mAbs 8 days after transfection with ribozymes. (B) Cytosolic proteins were prepared from cells cultured for 6 days after transfection. (C) Cytosolic proteins were prepared from cells cultured for 6 days after transfection. Control cells were transfected with a PKC-ε ribozyme that was not catalytic active. (D) RT-PCR was performed on RNA prepared from cells cultured for 6 days after transfection. PKC-α, 320 bp; actin, 620 bp.

The effect of PKC- and PKC-β2 ribozymes on CD34+ cells cultured with EPO and SCF.

The CD34+ cells were incubated at 30 000 cells/well in flat-bottomed, 96 well plates with PKC-α ribozyme (2 μmol/L), PKC-β2 ribozyme (2 μmol/L), or medium for 24 hours and then stimulated with EPO (5 U/mL) and SCF (50 ng/mL.). (A) Cells were stained with the indicated mAbs 8 days after transfection with ribozymes. (B) Cytosolic proteins were prepared from cells cultured for 6 days after transfection. (C) Cytosolic proteins were prepared from cells cultured for 6 days after transfection. Control cells were transfected with a PKC-ε ribozyme that was not catalytic active. (D) RT-PCR was performed on RNA prepared from cells cultured for 6 days after transfection. PKC-α, 320 bp; actin, 620 bp.

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