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Identification of new mitochondrial genome organizations in wheat plants regenerated from somatic tissue cultures
Authors:C Hartmann  Y Henry  J De Buyser  C Aubry  A Rode
Institution:(1) Laboratoire de Biologie Moléculaire Végétale, Bâtiment 430, UA CNRS 1128, Université Paris XI, F-91405 Orsay, France;(2) Laboratoire d'Amélioration des Plantes, Bâtiment 360, UA CNRS 115, Université Paris XI, F-91405 Orsay, France
Abstract:Summary Plants have been regenerated from short-and long-term in vitro somatic tissue cultures made from immature embryos of the hexaploid wheat cultivar ldquoChinese Springrdquo. The mitochondrial genome organization of each regenerated plantlet was studied, after one selfing, by probing Sal I-restricted total DNA with cloned Sal I fragments of wheat mitochondrial DNA derived from a segment of the genome, which displays marked structural changes in response to in vitro culture. Short-term in vitro cultures give rise to regenerated plants whose mitochondrial genome organization is either close to that of the parental cultivar or to that of embryogenic callus cultures, except for a single plant which has an organization resembling that of short-term non-embryogenic cultures. In contrast, all but one of the plants regenerated from long-term cultures exhibited a mitochondrial genome organization similar to that of long-term nonembryogenic cultures. In addition, extra labelled bands were detected in some of the regenerated plants with two of the probes used. These results emphasize the importance of the duration of the in vitro step preceding the regeneration process: the longer it is, the higher the probability is of obtaining mitochondrial DNA variability in regenerated plants. Furthermore, since increasing the duration of the in vitro stetp results in the production of regenerated plants with a mitochondrial genome organization resembling that of non-embryogenic tissue cultures, the question is thus raised as to whether regeneration from long-term cultures is suitable for use in plant breeding.
Keywords:Mitochondrial DNA  Chondriome variability  In vitro culture  Plant regeneration  Wheat
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