Inhibition of Deoxyribonuclease Activity in the Medium Surrounding Plant Protoplasts

Abstract

After 1 h, exogenous DNA was degraded within a culture medium at 25.degree. C (pH 6) containing protoplasts of Daucus carota L. var. sativa. Low temperature incubation (1.degree. C) or the addition of 45 mM sodium citrate to the medium eliminated DNase activity for at least 4.5 h. This DNase activity was not reduced at pH 7 or 9, nor by addition of 200 mM ATP. Techniques were developed to ensure high protoplast plating efficiencies and high regenerative capabilities after low temperature treatment and the addition of sodium citrate to the medium. Results indicated citrate concentrations to 45 mM and 1.degree. C temperatures revealed little or no effect on protoplast regeneration capacities. Protoplast viability was 90-95% at the time of plating as determined by phenosafranin staining and an estimated 50-60% of these undergo cell division in the solid agar medium.