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The first step to model DTG-PCR Ji Youn Lee Cell and microbial engineering laboratory Seoul National University Basic concept • Make use of the math in published ones : Competitive PCR • Addition of the ssDNA distribution profile with temperature • Experimental part • Modeling and simulation part Competitive PCR • Originally introduced for the analysis of quantitative PCR • Target and various concentrations of internal standard • Efficiencies at each cycle eiT and eiS Ti = (1+ eiT ) Ti-1 Si = (1+ eiS ) Si-1 Tn = P i=1 n (1+ eiT ) T0 Sn = P i=1 n (1+ eiS ) S0 Our modeling ? • Factors affecting PCR – the concentrations of DNA polymerase, dNTPs, MgCl2, DNA and primers – the denaturing annealing and synthesis temperatures – the length and number of cycles – ramping times and the presence of contaminating DNA and inhibitors in the sample • Modeling – Exceptions Enzyme inactivation Substrate consumption High-tolerance of PCR to mismatches – All together~ Each steps • 1st step: denaturation dsDNA ssDNA Number of ssDNA molecules participating in the annealing reaction (melting curve or data table) • 2nd step: annealing ssDNA + primer heteroduplex • 3rd step: extension heteroduplex + polymerase enzyme-substrate complex [complex + dNTP elongated complex]repeat fully elongated complex dsDNA + polymerase enzyme kinetics 이용 (Michealis-Menten equation) Work to do.. • • • • Experiments Melting curve or melting data acquisition Equations Search the kinetic parameters