4.5 Article

Composition and Structure of Sugarcane Cell Wall Polysaccharides: Implications for Second-Generation Bioethanol Production

Journal

BIOENERGY RESEARCH
Volume 6, Issue 2, Pages 564-579

Publisher

SPRINGER
DOI: 10.1007/s12155-012-9268-1

Keywords

Bioenergy; Cellulosic ethanol; Hemicelluloses; Cell wall composition; Cell wall structure; Sugarcane

Funding

  1. Instituto Nacional de Ciencia e Tecnologia do Bioetanol-INCT do Bioetanol [FAPESP 2008/57908-6, CNPq 574002/2008-1]
  2. Centro de Processos Biologicos e Industriais para Biocombustiveis-CeProBIO [FAPESP 2009/52840-7, CNPq 490022/2009-0]
  3. Office of Biological and Environmental Research, Office of Science, United States, Department of Energy [DE-AC05-00OR22725]
  4. NSF Plant Genome Program [DBI-0421683]

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The structure and fine structure of leaf and culm cell walls of sugarcane plants were analyzed using a combination of microscopic, chemical, biochemical, and immunological approaches. Fluorescence microscopy revealed that leaves and culm display autofluorescence and lignin distributed differently through different cell types, the former resulting from phenylpropanoids associated with vascular bundles and the latter distributed throughout all cell walls in the tissue sections. Polysaccharides in leaf and culm walls are quite similar, but differ in the proportions of xyloglucan and arabinoxylan in some fractions. In both cases, xyloglucan (XG) and arabinoxylan (AX) are closely associated with cellulose, whereas pectins, mixed-linkage-beta-glucan (BG), and less branched xylans are strongly bound to cellulose. Accessibility to hydrolases of cell wall fraction increased after fractionation, suggesting that acetyl and phenolic linkages, as well as polysaccharide-polysaccharide interactions, prevented enzyme action when cell walls are assembled in its native architecture. Differently from other hemicelluloses, BG was shown to be readily accessible to lichenase when in intact walls. These results indicate that wall architecture has important implications for the development of more efficient industrial processes for second-generation bioethanol production. Considering that pretreatments such as steam explosion and alkali may lead to loss of more soluble fractions of the cell walls (BG and pectins), second-generation bioethanol, as currently proposed for sugarcane feedstock, might lead to loss of a substantial proportion of the cell wall polysaccharides, therefore decreasing the potential of sugarcane for bioethanol production in the future.

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