Fig. 6.
Fig. 6. Detection of RAG-2 after culture with FL, supplemental cytokines, and SCM. CD34+Lin−DR− cells were cultured in the presence of supplemental cytokines (IL-2, IL-3, IL-7, and KL) with or without SCM and FL. After 7 or 14 days, cells were harvested and mRNA amplified using RAG-2 primers. Five replicate samples for each culture condition are shown. Jurkat T-cell mRNA was used as a positive control (+C), and a template-free PCR reaction served as a negative control (−C). Shown is an autoradiograph after hybridization with a RAG-2 sequence-specific probe. The absence of genomic RAG-2 sequences was confirmed by amplification of mRNA without prior reverse transcription. Transcripts for β-actin were simultaneously amplified to confirm the presence of intact mRNA.

Detection of RAG-2 after culture with FL, supplemental cytokines, and SCM. CD34+LinDR cells were cultured in the presence of supplemental cytokines (IL-2, IL-3, IL-7, and KL) with or without SCM and FL. After 7 or 14 days, cells were harvested and mRNA amplified using RAG-2 primers. Five replicate samples for each culture condition are shown. Jurkat T-cell mRNA was used as a positive control (+C), and a template-free PCR reaction served as a negative control (−C). Shown is an autoradiograph after hybridization with a RAG-2 sequence-specific probe. The absence of genomic RAG-2 sequences was confirmed by amplification of mRNA without prior reverse transcription. Transcripts for β-actin were simultaneously amplified to confirm the presence of intact mRNA.

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