The phenylpropanoid pathway in plants is responsible for the biosynthesis of a huge amount of secondary metabolites derived from phenylalanine and tyrosine. Both flavonoids and lignins are synthesized at the end of this very diverse metabolic pathway, as well as many intermediate molecules whose precise biological functions remain largely unknown. The diversity of these molecules can be further increased under the action of UDP-glycosyltransferases (UGTs) leading to the production of glycosylated hydroxycinnamates and related aldehydes, alcohols and esters. Glycosylation can change phenylpropanoid solubility, stability and toxic potential, as well as influencing compartmentalization and biological activity. (De)-glycosylation therefore represents an extremely important regulation point in phenylpropanoid homeostasis. In this article we review recent knowledge on the enzymes involved in regulating phenylpropanoid glycosylation status and availability in different subcellular compartments. We also examine the potential link between monolignol glycosylation and lignification by exploring co-expression of lignin biosynthesis genes and phenolic (de)glycosylation genes. Of the different biological roles linked with their particular chemical properties, phenylpropanoids are often correlated with the plant's stress management strategies that are also regulated by glycosylation. UGTs can for instance influence the resistance of plants during infection by microorganisms and be involved in the mechanisms related to environmental changes. The impact of flavonoid glycosylation on the color of flowers, leaves, seeds and fruits will also be discussed. Altogether this paper underlies the fact that glycosylation and deglycosylation are powerful mechanisms allowing plants to regulate phenylpropanoid localisation, availability and biological activity.
Fresh weight (FW), dry weight (DW), carbon and nitrogen content were measured for specimens of Laminaria saccharina (Heterokontophyta: Phaeophyceae) sampled in the eastern English Channel in order to conduct a biometrical study. The aim was to relate carbon and nitrogen masses of the algae to a simple and rapid morphological measurement of the total length of the sporophyte. These relationships were highly significant and appeared very useful to express the standing biomass of L. saccharina in terms of carbon or nitrogen and then to consider dynamic processes such as primary production. Variations in tissue carbon (C) and nitrogen (N) were examined over a complete seasonal cycle. Average carbon and nitrogen content ranged from 23·9 to 31·4% and 2·23 to 3·42% of the total dry weight, respectively. Variations in C/N ratio showed a clear seasonal pattern with an increase in the early spring corresponding to strong photosynthesis and growth.
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