Table 1.

PCR primer sequences used in ChIP

Forward primer
Reverse primer
hTERT Buffer G*  GGTTACCCCACAGCCTAGGCCGATTC   CAGGGCTTCCCACGTGCGCAGCAGGACGCAGC  
C17 Buffer L   CTGTGCAGAAAGAAATTTCTTG   CATGGTGCCAGGCGCTGGTG  
c-Myc Buffer A   ACCCTCCCCACCCTCCCCATAAG   GCCTCTGAGAAGCCCTGCCCTTC  
hTERT control Buffer A  GGTAATGAAGTGGTGTGCAGGAAA   TGGCTGAAAGCAGCCTCATCTCTC  
C17 control Buffer E   CTTTAACTTGGCTGCTTAGAC   CATAGTTTAGAGGGGACTCC  
c-Myc control Buffer A
 		 ACATCAACCCCATGAAGGAGATAC
 		 GCCTGACCAGGCTTAGATGTTGAG
 
Forward primer
Reverse primer
hTERT Buffer G*  GGTTACCCCACAGCCTAGGCCGATTC   CAGGGCTTCCCACGTGCGCAGCAGGACGCAGC  
C17 Buffer L   CTGTGCAGAAAGAAATTTCTTG   CATGGTGCCAGGCGCTGGTG  
c-Myc Buffer A   ACCCTCCCCACCCTCCCCATAAG   GCCTCTGAGAAGCCCTGCCCTTC  
hTERT control Buffer A  GGTAATGAAGTGGTGTGCAGGAAA   TGGCTGAAAGCAGCCTCATCTCTC  
C17 control Buffer E   CTTTAACTTGGCTGCTTAGAC   CATAGTTTAGAGGGGACTCC  
c-Myc control Buffer A
 		 ACATCAACCCCATGAAGGAGATAC
 		 GCCTGACCAGGCTTAGATGTTGAG
 
*

Fail-safe buffers were used, as indicated in “Materials and methods”

Control indicates a DNA region 5 to 6 kb away from the promoter

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