4.7 Article

The influence of aerated hydration seed treatment on seed longevity as assessed by the viability equations

Journal

JOURNAL OF EXPERIMENTAL BOTANY
Volume 51, Issue 353, Pages 2031-2043

Publisher

OXFORD UNIV PRESS
DOI: 10.1093/jexbot/51.353.2031

Keywords

Brassica oleracea var. botrytis; beta-tubulin; controlled deterioration germination; K-i; rate of deterioration (1/sigma); 4C DNA

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Aerated hydration (AH) treatments of cauliflower seeds for 12 h (12AH) and 28 h (28AH) at 20 degreesC resulted in improved or reduced storage potential of low or high vigour seeds, respectively, Seeds were stored at their initial seed moisture content (mean 5.5% me) or at 12% me at 10 degreesC for 12 months and at 20 degreesC for 4 months. The improved longevity of low vigour seeds was associated with increased K-i (initial seed viability) and a reduced rate of deterioration (1/sigma) whereas the K-i of high vigour seeds fell after 28AH and the rate of deterioration increased such that the time to lose one probit of viability decreased from 28.7 to 5.3 months at 10 degreesC and from 10.4 to 1.2 months at 20 C. The improved K-i of low vigour seeds could be explained by the reduction in the extent of deterioration after AH, as indicated by the increase in germination after cotrolled deterioration (CD), and the possible activation of metabolic repair during treatment. In contrast the reduced germination after CD of AH-treated high vigour seeds was indicative of deterioration as a result of treatment. Both high and low vigour seeds contained constitutive levels of beta -tubulin which increased during AH treatment, the increase being greater in high vigour seeds. High vigour seeds also showed an increase in the proportion of nuclear DNA present as 4C DNA, from 3% (untreated seeds) to 26% (28AH), indicative of germination advancement from the G(1) to G(2) phase of the cell cycle during treatment. This higher proportion of 4C DNA is correlated with the increased sensitivity of seeds to drying and/or storage after AH, leading to their reduced K-i and storage potential. In contrast, there was little change in %4C in low vigour seeds. Priming in polyethylene glycol (PEG, -1.0 MPa) for 5 d or 13 d also improved the longevity of low vigour seeds stored at their initial and 12% me at 10 degreesC for 8 months, as reflected in their laboratory and CD germination. In this case, however, the improved longevity of the low vigour seeds following 13 d priming was associated with an increase in 4C DNA from 4% (dry control) to 56% after treatment. The germination of both untreated and primed high vigour seeds remained high throughout the storage period. Increases in the rate of germination (decreased mean germination time) observed after all AH and PEG treatments were not consistently associated with an increase in the proportion of nuclei containing 4C DNA.

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