Fig. 3.
Fig. 3. Introducing the constitutively active mutant of EpoR into the endogenous EpoR locus. / (A) Targeting of EpoRR129C mutation into the endogenous EpoR locus was performed using a double replacement. In the first step, pEpoR-M2 construct was used to replace the WT allele of the EpoR to generate EpoRhytk/− ES cells. For the second step, pEpoRR129C construct was electroporated into the EpoRhytk/− ES to replace the EpoRhytk allele. Predicted restriction fragments by EcoRV digestion were indicated. (B) Southern blot analysis for knock-in event. Genomic DNA was isolated and digested with EcoRV. Southern blot was probed with an external probe A.

Introducing the constitutively active mutant of EpoR into the endogenous EpoR locus.

(A) Targeting of EpoRR129C mutation into the endogenous EpoR locus was performed using a double replacement. In the first step, pEpoR-M2 construct was used to replace the WT allele of the EpoR to generate EpoRhytk/− ES cells. For the second step, pEpoRR129C construct was electroporated into the EpoRhytk/− ES to replace the EpoRhytk allele. Predicted restriction fragments by EcoRV digestion were indicated. (B) Southern blot analysis for knock-in event. Genomic DNA was isolated and digested with EcoRV. Southern blot was probed with an external probe A.

Close Modal
This Feature Is Available To Subscribers Only

or Create an Account

Close Modal
Close Modal