Direct fluorescence imaging of lignocellulosic and suberized cell walls in roots and stems

被引:46
作者
Kitin, Peter [1 ,2 ]
Nakaba, Satoshi [2 ,3 ]
Hunt, Christopher G. [4 ]
Lim, Sierin [5 ]
Funada, Ryo [2 ,3 ]
机构
[1] Univ Washington, Sch Environm & Forest Sci, Box 352100, Seattle, WA 98195 USA
[2] Tokyo Univ Agr & Technol, Inst Global Innovat Res, Fuchu, Tokyo 1838538, Japan
[3] Tokyo Univ Agr & Technol, Fac Agr, Fuchu, Tokyo 1838509, Japan
[4] USDA, Forest Prod Lab, Madison, WI 53726 USA
[5] Nanyang Technol Univ, Sch Chem & Biomed Engn, 70 Nanyang Dr,Block N1-3, Singapore 637457, Singapore
关键词
3D imaging; autofluorescence; cellulosic wall; Congo red; fluorol yellow; glycerol clearing; histochemistry; lignin; lipids; suberin; MANDSHURICA VAR JAPONICA; RING-POROUS HARDWOOD; WOOD FORMATION; CONGO-RED; CONFOCAL MICROSCOPY; LIGNIN DISTRIBUTION; EARLYWOOD VESSELS; LIGHT-MICROSCOPY; CHEMICAL-CHARACTERIZATION; TRACHEARY ELEMENTS;
D O I
10.1093/aobpla/plaa032
中图分类号
Q94 [植物学];
学科分类号
071001 ;
摘要
Investigating plant structure is fundamental in botanical science and provides crucial knowledge for the theories of plant evolution, ecophysiology and for the biotechnological practices. Modern plant anatomy often targets the formation, localization and characterization of cellulosic, lignified or suberized cell walls. While classical methods developed in the 1960s are still popular, recent innovations in tissue preparation, fluorescence staining and microscopy equipment offer advantages to the traditional practices for investigation of the complex lignocellulosic walls. Our goal is to enhance the productivity and quality of microscopy work by focusing on quick and cost-effective preparation of thick sections or plant specimen surfaces and efficient use of direct fluorescent stains. We discuss popular histochemical microscopy techniques for visualization of cell walls, such as autofluorescence or staining with calcofluor, Congo red (CR), fluorol yellow (FY) and safranin, and provide detailed descriptions of our own approaches and protocols. Autofluorescence of lignin in combination with CR and FY staining can clearly differentiate between lignified, suberized and unlignified cell walls in root and stem tissues. Glycerol can serve as an effective clearing medium as well as the carrier of FY for staining of suberin and lipids allowing for observation of thick histological preparations. Three-dimensional (3D) imaging of all cell types together with chemical information by wide-field fluorescence or confocal laser scanning microscopy (CLSM) was achieved.
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页数:19
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