Over 20,000 human basic promoter regions for each unique target gene have been systematically analyzed by ASB's team and cloned in Renilla Luciferase based vector. This group of vector will be valuable reagents for quickly data validation when a specific TF interaction with various promoters has been obtained using GREMA technology. Co-transfection of TF full-length cDNA (make this superlink to full-length TF cDNA product section). and promoter-luciferase vector will help to rapidly validate TF/promoter interaction for up- or down regulating of gene transcription.

    One of the critical steps in Chromatin immunoprecipitation (ChIP) assay is a validation of TF specific binding promoter DNA in the pull-down complex using PCR based assay. Due to a high GC containing and rich repetitive elements in human promoter region, design of oligo for specific amplification of human promoter DNA fragment becomes a challenge job in the field. Currently, ASB has individually designed and PCR validated more than 20,000 human promoter using its unique in house developed "matrix selection" algorithm. In order to help our customer, this validated oligo design for each of human gene / promoter could be accessed by simple send your target accession number and received recommended oligo design in 24 hours in your email. Please click here for more information:

    After cloning more than 20,000 human promoters in report vector like Renilla luciferase, and DNA sequence validated for each of them. You can simple click search bar and access a specific promoter-report ready plasmids for your project.