We have investigated the regulation of sucrose storage in cell-suspension cultures of sugarcane. When grown in batch culture, sucrose accumulation commences after about 5 d, when the nitrogen supply is exhausted. Sucrose storage is also induced by decreasing the nitrogen supply to cells growing in a chemostat. The measured activity of sucrose-phosphate synthase is high enough to account for the rate of sucrose accumulation, provided precautions are taken to avoid the hydrolysis of UDP during the assay. The cells contained high sucrose-synthase activity but pulsing experiments with [(14)C]glucose and unlabelled fructose indicated that this enzyme did not contribute substantially to the synthesis of sucrose, because the glucosyl and fructosyl moieties of sucrose were equally labelled. Several lines of evidence demonstrate the presence of a cycle in which sucrose is synthesized and degraded simultaneously; sucrosephosphate-synthase activity doubles during the phase when the cells are actively storing sucrose but activity is also high after storage has ceased, or when the sucrose is being remobilised; pulse experiments with [(14)C]fructose also showed that sucrose synthesis occurs not only during the storage phase, but also after storage has stopped and during the rapid mobilisation of sucrose; the cells contain high activities of sucrose synthase and alkaline invertase and these are both at a maximum when sucrose storage is occurring; even during the storage phase. [(14)C]fructose pulses lead to labelling of free glucose which is evidence for rapid synthesis and degradation of sucrose. It is proposed that the rate and extent of sucrose storage is regulated by this cycle of synthesis and degradation. Measurements of enzyme activities and metabolite levels are presented, and it is discussed which factors could contribute to the regulation of these two opposing fluxes and, hence, the rate of net sucrose storage and mobilisation.
We have investigated whether sucrose accumulation in heterotrophic cell-suspension cultures of Chenopodium rubrum L. is regulated by a cycle in which sucrose is simultaneously synthesised and degraded. Net sucrose accumulation was measured by monitoring the sucrose content, unidirectional synthesis was monitored by supplying pulses of [(14)C] glucose, and unidirectional degradation was estimated from the difference between unidirectional synthesis and net accumulation. When 50 mM glucose was supplied to carbohydrate-depleted cells there was a rapid net accumulation of sucrose, which stopped after 24 h. The incorporation of (14)C into sucrose was similar to the initial rate of net sucrose accumulation, but rapid (14)C incorporation continued after the cells had stopped accumulating sucrose. A method was developed to rapidly separate sucrose-phosphate synthase (SPS) from uridine-diphosphate-hydrolysing activities which interfered with the assay. The cells contained enough SPS activity to catalyse the observed rate of sucrose synthesis. SPS activity increased in cells which had stopped accumulating sucrose, and the enzyme became less sensitive to inhibition by inorganic phosphate. Sucrose synthase and alkaline invertase activity were four- and twofold higher than SPS activity, and both degradative enzymes increased in cells which had stopped accumulating sucrose. Sucrose synthase is strongly modulated by the concentration of sucrose and by competitive feedback regulation by fructose in these cells. It is concluded that sucrose accumulation ceases in these cells because the rate of degradation of sucrose increases until it matches the rate of synthesis. It is discussed how this cycle is regulated, and how it may interact with the substrate cycle between triose-phosphates and hexose-phosphates (Hatzfeld and Stitt, 1990, Planta 180, 198-204). These cycles allow sucrose turnover to respond in a highly sensitive manner to small changes in the balance between the supply of sucrose and the demand for carbon for respiration and biosynthesis in the cell.
Summary• Several pesticide classes have been used for control of the notorious plant pathogen, Phytophthora infestans . Some of these alter lipids, suggesting that lipid metabolism may be a target site. Here, we investigate the action of a new, active, mandelamide compound, SX 623509 ( N -2 ′ -(4 ′′ -ethoxy-3 ′′ -methoxy) phenylethyl-3, 4-dichloromandelamide), on lipid metabolism.• Phytophthora infestans cultured in pea-broth or minimal media was exposed to different concentrations of SX 623509. Lipid metabolism was followed with radiolabelled acetate, choline or ethanolamine. Products were analysed following separation by thin-layer chromatography and gas-liquid chromatography.• SX 623509 reduced growth and lipid labelling from [ 14 C]acetate in both media. The inhibition in lipid labelling was not caused merely by a reduction in uptake of the radiolabelled precursor. There were changes in labelling patterns, particularly reductions in phosphatidylcholine and triacylglycerol and increases in phosphatidate and diacylglycerol. The effect of SX 623509 on phosphatidylcholine labelling was followed in more detail.• We conclude that the mandelamide pesticide SX 623509 reduces lipid synthesis at concentrations similar to those inhibiting growth. Specific effects on lipid labelling patterns are probably caused by inhibition of cholinephosphotransferase, which may be a future target site for pesticide development.
The isolation of carbocyclic coformycin as the herbicidally active component from a fermentation of Saccharothrix species was described previously (B.D. Bush, G.V. Fitchett, D.A. Gates, D. Langley [1993] Phytochemistry 32: 737-739). Here we report that the primary mode of action of carbocyclic coformycin has been identified as inhibition of the enzyme AMP deaminase (EC 3.5.4.6) following phosphorylation at the 5' hydroxyl on the carbocyclic ring in vivo. When pea (Pisum sativum L. var Onward) seedlings are treated with carbocyclic coformycin, there is a very rapid and dramatic increase in ATP levels, indicating a perturbation in purine metabolism. Investigation of the enzymes of purine metabolism showed a decrease in the extractable activity of AMP deaminase that correlates with a strong, noncovalent association of the phosphorylated natural product with the protein. The 5'-phosphate analog of the carbocyclic coformycin was synthesized and shown to be a potent, tight binding inhibitor of AMP deaminase isolated from pea seedlings. Through the use of a synthetic radiolabeled marker, rapid conversion of carbocyclic coformycin to the 5'-phosphate analog could be demonstrated in vivo. It is proposed that inhibition of AMP deaminase leads to the death of the plant through perturbation of the intracellular ATP pool.
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