Figure 1

TILLING strategy for rice. After seed mutagenesis, chimeric M1 plants are allowed to self-pollinate and a single M2 plant is grown to provide DNA for mutation discovery and seed for banking. DNAs are pooled eightfold and arrayed in a two-dimensional format on 96-well plates. After PCR amplification of target genes, heteroduplexes are formed upon heating and annealing, and then digested using crude celery juice extract containing the CEL I nuclease. Cut strands are separated by denaturing polyacrylamide gel electrophoresis, and visualized by fluorescence detection using a Li-Cor DNA analyzer. The presence of cut products in two pools identifies the individual harboring the polymorphism.