ABSTRACT
Five types of cellular aggregates have been characterised in embryogenic cell suspensions of banana (Musa AAA Grande naine cv.). Type I corresponded to isolated cells or to small cell aggregates. Type II were composed of embryogenic cells. Type III can be distinguished from type II due to the presence of peripheral proliferation zones with embryonic cells. Type IV were composed of protodermic masses histologically comparable to proembryos. Type V were nodules composed of a central zone of meristematic cells and of an external zone of starchy cells. Each culture flask of a cell line contained a majority of one of the above-mentioned aggregate types. Histological studies of somatic embryo developement on semi-solid regeneration medium showed that there were close similarities between the initial steps of ontogenesis of the embryos and the different cell aggregates in liquid multiplication medium. It appeared that aggregates II-IV of the suspension belong to the same development continuum which reproduces the initial phases of somatic embryo ontogenesis on semi-solid medium. Type V resulted from the development of type IV, for which ontogenesis is hindered by direct contact with 2,4-dichlorophenoxyacetic acid and the shaken liquid multiplication medium. Type I aggregates probably do not belong to the development continuum but rather correspond to the degeneration of the other types of aggregates in the suspension. The presence of intermediate types in the liquid medium reinforces the hypothesis of a relationship between the aggregates. The aggregates tended to develop through time from a majority of type II or III at the beginning of their culture to types IV-V for older suspensions.
ABSTRACT
Photosynthesis and light O(2)-uptake of the aerial portion of the CAM plant Ananas comosus (L.) merr. were studied by CO(2) and O(2) gas exchange measurements. The amount of CO(2) which was fixed during a complete day-night cycle was equal to the amount of total net O(2) evolved. This finding justifies the assumption that in each time interval of the light period, the difference between the rates of net O(2)-evolution and of net light atmospheric CO(2)-uptake give the rates of malate-decarboxylation-dependent CO(2) assimilation. Based upon this hypothesis, the following photosynthetic characteristics were observed: (a) From the onset of the light to midphase IV of CAM, the photosynthetic quotient (net O(2) evolved/net CO(2) fixed) was higher than 1. This indicates that malate-decarboxylation supplied CO(2) for the photosynthetic carbon reduction cycle during this period. (b) In phase III and early phase IV, the rate of CO(2) assimilation deduced from net O(2)-evolution was 3 times higher than the maximum rate of atmospheric CO(2)-fixation during phase IV. A conceivable explanation for this stimulation of photosynthesis is that the intracellular CO(2)-concentration was high because of malate decarboxylation. (c) During the final hours of the light period, the photosynthetic quotient decreased below 1. This may be the result of CO(2)-fixation by phosphoenolpyruvate-carboxylase activity and malate accumulation. Based upon this hypothesis, the gas exchange data indicates that at least 50% of the CO(2) fixed during the last hour of the light period was stored as malate. Light O(2)-uptake determined with (18)O(2) showed two remarkable characteristics: from the onset of the light until midphase IV the rate of O(2)-uptake increased progressively; during the following part of the light period, the rate of O(2)-uptake was 3.5 times higher than the maximum rate of CO(2)-uptake. When malate decarboxylation was reduced or suppressed after a night in a CO(2)-free atmosphere or in continuous illumination, the rate of O(2)-uptake was higher than in the control. This supports the hypothesis that the low rate of O(2)-uptake in the first part of the light period is due to the inhibition of photorespiration by increased intracellular CO(2) concentration because of malate decarboxylation. In view of the law of gas diffusion and the kinetic properties of the ribulose-1,5-bisphosphate carboxylase/oxygenase, O(2) and CO(2) gas exchange suggest that at the end of the light period the intracellular CO(2) concentration was very low. We propose that the high ratio of O(2)-uptake/CO(2)-fixation is principally caused by the stimulation of photorespiration during this period.
