Spatial organization of cellulose microfibrils and matrix polysaccharides in primary plant cell walls as imaged by multichannel atomic force microscopy

被引:177
作者
Zhang, Tian [1 ,2 ]
Zheng, Yunzhen [1 ,2 ]
Cosgrove, Daniel J. [1 ,2 ]
机构
[1] Penn State Univ, Dept Biol, 208 Mueller Lab, University Pk, PA 16802 USA
[2] Penn State Univ, Ctr Lignocellulose Struct & Format, 208 Mueller Lab, University Pk, PA 16802 USA
关键词
atomic force microscopy; electron microscopy; cell wall models; cellulose microfibrils; nanomechanical mapping; pectin; primary cell wall architecture; MOLECULAR-DYNAMICS SIMULATION; NUCLEAR-MAGNETIC-RESONANCE; SOLID-STATE NMR; ONION EPIDERMIS; ARABIDOPSIS HYPOCOTYL; MECHANICAL-PROPERTIES; SYNTHASE COMPLEX; GROWTH; MODELS; ARCHITECTURE;
D O I
10.1111/tpj.13102
中图分类号
Q94 [植物学];
学科分类号
071001 ;
摘要
We used atomic force microscopy (AFM), complemented with electron microscopy, to characterize the nanoscale and mesoscale structure of the outer (periclinal) cell wall of onion scale epidermis - a model system for relating wall structure to cell wall mechanics. The epidermal wall contains similar to 100 lamellae, each similar to 40 nm thick, containing 3.5-nm wide cellulose microfibrils oriented in a common direction within a lamella but varying by similar to 30 to 90 degrees between adjacent lamellae. The wall thus has a crossed polylamellate, not helicoidal, wall structure. Montages of high-resolution AFM images of the newly deposited wall surface showed that single microfibrils merge into and out of short regions of microfibril bundles, thereby forming a reticulated network. Microfibril direction within a lamella did not change gradually or abruptly across the whole face of the cell, indicating continuity of the lamella across the outer wall. A layer of pectin at the wall surface obscured the underlying cellulose microfibrils when imaged by FESEM, but not by AFM. The AFM thus preferentially detects cellulose microfibrils by probing through the soft matrix in these hydrated walls. AFM-based nanomechanical maps revealed significant heterogeneity in cell wall stiffness and adhesiveness at the nm scale. By color coding and merging these maps, the spatial distribution of soft and rigid matrix polymers could be visualized in the context of the stiffer microfibrils. Without chemical extraction and dehydration, our results provide multiscale structural details of the primary cell wall in its near-native state, with implications for microfibrils motions in different lamellae during uniaxial and biaxial extensions.
引用
收藏
页码:179 / 192
页数:14
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