Figure 1
Figure 1. Validation of ChIP-chip–identified SALL4-binding sites by Q-RT-PCR. Chromatin immunoprecipitation experiments were performed in NB4 cells with antibodies raised against SALL4. Forty-three randomly selected promoters identified as SALL4 targets with ChIP-chip arrays were analyzed by Q-RT-PCR. ChIP-Q-RT-PCR identified 39 targets having more than 2-fold enrichment versus the input control. The fold change of SALL4 immunoprecipitated DNA over the input is presented on a log2 scale. Negative control primers were designed based on the genomic regions surrounding the peak as shown in Figure S2.

Validation of ChIP-chip–identified SALL4-binding sites by Q-RT-PCR. Chromatin immunoprecipitation experiments were performed in NB4 cells with antibodies raised against SALL4. Forty-three randomly selected promoters identified as SALL4 targets with ChIP-chip arrays were analyzed by Q-RT-PCR. ChIP-Q-RT-PCR identified 39 targets having more than 2-fold enrichment versus the input control. The fold change of SALL4 immunoprecipitated DNA over the input is presented on a log2 scale. Negative control primers were designed based on the genomic regions surrounding the peak as shown in Figure S2.

Close Modal
This Feature Is Available To Subscribers Only

or Create an Account

Close Modal
Close Modal