Fig. 1.
Fig. 1. Primarsequence and cytogenetic location of 16 microsatellite markers used in the study. The distance in centimorgans between the markers is indicated. The PCR conditions included denaturation in 95° for 5 minutes. Denaturation temperature was always 94°C for 30 to 60 seconds. Annealing time was 30°C and the temperature is shown for every microsatelite marker. Elongation temperature was 72°C for 30 to 40 seconds. The number of cycles is shown for every marker. Amplification was always concluded with 10-minute final extension at 72°C. Marker D6S15433 and D6S1709, located between D6S468 and D6S283, and marker D6S434 and D6S1028, located between D6S283 and D6S301, are not shown in the figure.

Primarsequence and cytogenetic location of 16 microsatellite markers used in the study. The distance in centimorgans between the markers is indicated. The PCR conditions included denaturation in 95° for 5 minutes. Denaturation temperature was always 94°C for 30 to 60 seconds. Annealing time was 30°C and the temperature is shown for every microsatelite marker. Elongation temperature was 72°C for 30 to 40 seconds. The number of cycles is shown for every marker. Amplification was always concluded with 10-minute final extension at 72°C. Marker D6S15433 and D6S1709, located between D6S468 and D6S283, and marker D6S434 and D6S1028, located between D6S283 and D6S301, are not shown in the figure.

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