Fig. 3.
Fig. 3. Determination of the linkage between nt 19911 and nt 20210 by simultaneous HindIII and EcoNI digestion of a 345-bp amplified fragment spanning both sites. (A) Schematic illustration of 4 possible alleles and specific fragment sizes in basepairs after cleavage at the indicated sites (X). (B) Electrophoretic separation of the following observed genotypes: 3 normal homozygotes for 20210G (lanes 1 through 3) who were GG, GA, and AA for the 19911 polymorphism, respectively; 2 homozygotes for 20210A (lanes 4 and 5) who were AA and AG for the 19911 polymorphism, respectively; and 2 heterozygotes for G20210A who were AA (lane 6) and AG (lane 7) for the 19911 polymorphism. The additional band in lane 7 between the 345- and 303-bp bands represents a heteroduplex (H.D). This was proved by the following two mixing experiments. (1) When 345-bp PCR fragments from a homozygote for 20210G and 19911G and a homozygote for 20210A and 19911A were mixed and digested with HindIII andEcoNI, an uncut 345-bp fragment and a 303-bp fragment were obtained (lane 8). (2) When DNA samples from the same 2 individuals were mixed and then amplified by PCR, followed by digestion and electrophoresis, a pattern representing heteroduplex bands was obtained (lane 9) that is identical to the one shown in lane 7. Numbers alongside the gel indicate the size (in basepairs) of the bands.

Determination of the linkage between nt 19911 and nt 20210 by simultaneous HindIII and EcoNI digestion of a 345-bp amplified fragment spanning both sites. (A) Schematic illustration of 4 possible alleles and specific fragment sizes in basepairs after cleavage at the indicated sites (X). (B) Electrophoretic separation of the following observed genotypes: 3 normal homozygotes for 20210G (lanes 1 through 3) who were GG, GA, and AA for the 19911 polymorphism, respectively; 2 homozygotes for 20210A (lanes 4 and 5) who were AA and AG for the 19911 polymorphism, respectively; and 2 heterozygotes for G20210A who were AA (lane 6) and AG (lane 7) for the 19911 polymorphism. The additional band in lane 7 between the 345- and 303-bp bands represents a heteroduplex (H.D). This was proved by the following two mixing experiments. (1) When 345-bp PCR fragments from a homozygote for 20210G and 19911G and a homozygote for 20210A and 19911A were mixed and digested with HindIII andEcoNI, an uncut 345-bp fragment and a 303-bp fragment were obtained (lane 8). (2) When DNA samples from the same 2 individuals were mixed and then amplified by PCR, followed by digestion and electrophoresis, a pattern representing heteroduplex bands was obtained (lane 9) that is identical to the one shown in lane 7. Numbers alongside the gel indicate the size (in basepairs) of the bands.

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