Fig. 1.
Fig. 1. Competitive PCR method for residual disease quantification. / A competitor was constructed by PCR using genomic DNA from the malignant clone as template together with a clone-specific primer and primer-XhoI to introduce a restriction site. The first amplification in the seminested PCR was done with the clone-specific primer and primer-1 and the second amplification with the clone-specific primer and primer-2. The PCR products from the competitor are cleaved by the restriction enzyme XhoI; the PCR products from the malignant clone remain uncleaved. The MRD level can be determined from the lanes with equal amplification of the competitor and malignant clone.14

Competitive PCR method for residual disease quantification.

A competitor was constructed by PCR using genomic DNA from the malignant clone as template together with a clone-specific primer and primer-XhoI to introduce a restriction site. The first amplification in the seminested PCR was done with the clone-specific primer and primer-1 and the second amplification with the clone-specific primer and primer-2. The PCR products from the competitor are cleaved by the restriction enzyme XhoI; the PCR products from the malignant clone remain uncleaved. The MRD level can be determined from the lanes with equal amplification of the competitor and malignant clone.14 

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