RESUMO
Interest in hemp (Cannabis sativa L.) is increasing due to the development of a new range of industrial applications based on bast fibers. However the variability of bast fiber yield and quality represents an important barrier to further exploitation. Primary and secondary fiber content was examined in two commercial hemp varieties (Fedora 17, Santhica 27) grown under contrasted sowing density and irrigation conditions. Both growing conditions and hemp varieties impact stem tissue architecture with a large effect on the proportion of secondary fibers but not primary fibers. Attenuated total reflectance infrared spectroscopy allowed the discrimination of manually-isolated native primary fibers and secondary fibers but did not reveal any clustering according to growing conditions and variety. Infrared data were confirmed by wet chemistry analyses that revealed slight but significant differences between primary and secondary fiber cell wall composition. Infrared spectroscopy of technical fibers obtained after mechanical defibering revealed differences with native primary, but not secondary fibers and also discriminated samples obtained from plants grown under different conditions. Altogether the results suggested that the observed variability of hemp technical fibers could be partially explained by i) differences in secondary fiber production and ii) differential behavior during mechanical defibering resulting in unequal separation of primary and secondary fibers.
Assuntos
Cannabis/química , Cannabis/metabolismo , Espectroscopia de Infravermelho com Transformada de Fourier , Floema/metabolismoRESUMO
BACKGROUND: Owing to the complexity of soil composition, accurate predictions of both apoplastic systemicity of lipophilic xenobiotics and their leaching from the soil are made difficult. Therefore, a non-destructive method to assess directly these two components of the spatial behaviour of soil-applied phytochemicals is needed. RESULTS: The plant selected was a dwarf tomato, which can exude an abundant apoplastic fluid through large stomata for several months. The feasibility and reliability of the method were assayed using three triazoles exhibiting different log D values. HPLC-MS analyses indicated that triadimenol (log D = 2.97) was clearly the most mobile compound within the apoplast, especially its diastereoisomer A. Propiconazole (log D = 3.65) and penconazole (log D = 4.64) exhibited a similar low systemicity. The data remained the same when the three fungicides were applied together on the soil. Long time-course studies (1.5 months) of penconazole behaviour indicated that, in contrast to leaching, which decrease sharply, root-to-shoot translocation remained almost unchanged during the whole experiment, in spite of the high lipophilicity of this fungicide. CONCLUSION: This method must contribute to a better knowledge of the behaviour of commercial soil-applied phytochemicals. It can also be used to screen new xenobiotics within strategies to satisfy environmental requirements.
Assuntos
Agroquímicos/química , Agroquímicos/metabolismo , Bioensaio/métodos , Solo/química , Fungicidas Industriais/química , Fungicidas Industriais/metabolismo , Interações Hidrofóbicas e Hidrofílicas , Solanum lycopersicum/citologia , Solanum lycopersicum/metabolismo , Raízes de Plantas/citologia , Raízes de Plantas/metabolismo , Estômatos de Plantas/citologia , Estômatos de Plantas/metabolismo , Fatores de Tempo , Triazóis/química , Triazóis/metabolismo , Xenobióticos/química , Xenobióticos/metabolismoRESUMO
Despite its important functions in plant physiology and defense, the membrane transport mechanism of salicylic acid (SA) is poorly documented due to the general assumption that SA is taken up by plant cells via the ion trap mechanism. Using Ricinus communis seedlings and modeling tools (ACD LogD and Vega ZZ softwares), we show that phloem accumulation of SA and hydroxylated analogs is completely uncorrelated with the physicochemical parameters suitable for diffusion (number of hydrogen bond donors, polar surface area, and, especially, LogD values at apoplastic pHs and Delta LogD between apoplast and phloem sap pH values). These and other data (such as accumulation in phloem sap of the poorly permeant dissociated form of monohalogen derivatives from apoplast and inhibition of SA transport by the thiol reagent p-chloromercuribenzenesulfonic acid [pCMBS]) lead to the following conclusions. As in intestinal cells, SA transport in Ricinus involves a pH-dependent carrier system sensitive to pCMBS; this carrier can translocate monohalogen analogs in the anionic form; the efficiency of phloem transport of hydroxylated benzoic acid derivatives is tightly dependent on the position of the hydroxyl group on the aromatic ring (SA corresponds to the optimal position) but moderately affected by halogen addition in position 5, which is known to increase plant defense. Furthermore, combining time-course experiments and pCMBS used as a tool, we give information about the localization of the SA carrier. SA uptake by epidermal cells (i.e. the step preceding the symplastic transport to veins) insensitive to pCMBS occurs via the ion-trap mechanism, whereas apoplastic vein loading involves a carrier-mediated mechanism (which is targeted by pCMBS) in addition to diffusion.
