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Suitable transfection methods for single particle tracing in plant suspension cells
Authors:Göhring  Janett  Fulcher  Nick  Schilcher  Kurt  Barta  Andrea  Jacak  Jaroslaw
Affiliation:1. Institute for Building Materials, ETH Zurich, Zurich, Switzerland
2. Applied Wood Research Laboratory, Empa - Swiss Federal Laboratories for Material Testing and Research, Duebendorf, Switzerland
3. Department of Materials Science and Process Engineering, BOKU-University of Natural Resources and Life Science, Konrad Lorenz Strasse 24, A-3430, Tulln, Vienna, Austria
4. INRA-UMR-614 Fractionnement des Agro-Ressources et Environnement (FARE), F-51686, Reims, France
5. Université de Reims Champagne-Ardenne, UMR614 Fractionnement des Agro-Ressources et Environnement (FARE), F-51686, Reims, France
Abstract:

Background

Besides classical utilization of wood and paper, lignocellulosic biomass has become increasingly important with regard to biorefinery, biofuel production and novel biomaterials. For these new applications the macromolecular assembly of cell walls is of utmost importance and therefore further insights into the arrangement of the molecules on the nanolevel have to be gained. Cell wall recalcitrance against enzymatic degradation is one of the key issues, since an efficient degradation of lignocellulosic plant material is probably the most crucial step in plant conversion to energy. A limiting factor for in-depth analysis is that high resolution characterization techniques provide structural but hardly chemical information (e.g. Transmission Electron Microscopy (TEM), Atomic Force Microscopy (AFM)), while chemical characterization leads to a disassembly of the cell wall components or does not reach the required nanoscale resolution (Fourier Tranform Infrared Spectroscopy (FT-IR), Raman Spectroscopy).

Results

Here we use for the first time Scanning Near-Field Optical Microscopy (SNOM in reflection mode) on secondary plant cell walls and reveal a segmented circumferential nanostructure. This pattern in the 100 nm range was found in the secondary cell walls of a softwood (spruce), a hardwood (beech) and a grass (bamboo) and is thus concluded to be consistent among various plant species. As the nanostructural pattern is not visible in classical AFM height and phase images it is proven that the contrast is not due to changes in surfaces topography, but due to differences in the molecular structure.

Conclusions

Comparative analysis of model substances of casted cellulose nanocrystals and spin coated lignin indicate, that the SNOM signal is clearly influenced by changes in lignin distribution or composition. Therefore and based on the known interaction of lignin and visible light (e.g. fluorescence and resonance effects), we assume the elucidated nanoscale structure to reflect variations in lignification within the secondary cell wall.
Keywords:
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