A. General consideration for primer selection for bisulfite-conversion based PCR methods Because the two strands are no longer complementary after bisulfite modification, strand-specific primers are used for PCR amplification. Usually the sense strand is chosen for primer design.Primers should be designed according to the guidelines prescribed by Clark and colleagues, and under the assumption that all cytosines had been converted to uracil. The important parameters to be considered when selecting PCR primers are the ability of the primer to form a stable duplex with the specific site on the target DNA and no duplex formation with another primer molecule or no hybridization at any other target site. Despite variations among bisulfite-conversion based methylation mapping methods, they all share the same procedure of modifying DNA with sodium bisulfite as the first step and subsequently PCR amplification with primers specific for modified DNA. The following criteria are common to both methylation specific PCR and bisulfite genomic sequencing PCR. B. Bisulfite sequencing PCR or restriction PCR. C. Methylation-Specific PCR (MSP) Reference Li, LC and Dahiya, R. Bioinformatics, 2002; 18(11):1427.Author: Long-Cheng Li Source: Protocol Online Abstract: Primer design rules for MSP and bisulfite sequencing PCR.
C" in their sequence to amplify only bisulfite modified DNA. Primers with more no-CpG "C"s are preferred.