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Plant Physiology 94:826-832 (1990)
© 1990 American Society of Plant Biologists

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Metabolism and Enzymology

Malate Metabolism in the Dark After 13CO2 Fixation in the Crassulacean Plant Kalanchoë tubiflora1

Willy Kalt2, C. Barry Osmond and James N. Siedow

Botany Department, Duke University, Durham, North Carolina 27706

The metabolism of [13C]malate was studied in the Crassulacean plant Kalanchoë tubiflora following exposure to 13CO2 for 2 hour intervals during a 16 hour dark cycle. Nuclear magnetic resonance spectroscopy of [13C]malate extracted from labeled tissue revealed that the transient flux of malate to the mitochondria, estimated by the randomization of [4-13C]malate to [1- 13C]malate by fumarase, varied substantially during the dark period. At both 15 and 25°C, the extent of malate label randomization in the mitochondria was greatest during the early and late parts of the dark period and was least during the middle of the night, when the rate of 13CO2 uptake was highest. Randomization of labeled malate continued for many hours after malate synthesis had initially occurred. Internally respired 12CO2 also served as a source of carbon for malate formation. At 15°C, 15% of the total malate was formed from respired 12CO2, while at 25°C, 49% of the accumulated malate was derived from respired 12CO2. Some of the malate synthesized from external 13CO2 was also respired during the night. The proportion of the total [13C]malate respired during the dark period was similar at 15 and 25°C, and respiration of newly formed [13C]malate increased as the night period progressed. These data are discussed with regard to the relative fluxes of malate to the mitochondria and the vacuole during dark CO2 fixation.


2 Present address: Agriculture Canada, Kentville Research Station, Kentville, Nova Scotia, Canada B4N 1J5.

1 This research was supported by a grant from the National Science Foundation to J.N.S. (CHE 86-07250).




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