New insights on Laminaria digitata ultrastructure through combined conventional chemical fixation and cryofixation

Author:

Katsaros Christos1,Le Panse Sophie2,Milne Gillian3,Carrano Carl J.4,Küpper Frithjof Christian456

Affiliation:

1. Department of Biology , National and Kapodistrian University of Athens, Panepistimiopolis , Athens , 157 84 , Greece

2. Plateforme d’Imagerie Merimage, FR2424, Centre National de la Recherche Scientifique, Station Biologique de Roscoff , Roscoff , 29680 , France

3. Microscopy and Histology Facility, University of Aberdeen, Institute of Medical Sciences , Foresterhill , Aberdeen , AB32 2ZD , SC , UK

4. Department of Chemistry and Biochemistry , San Diego State University , San Diego , CA , 92182-1030 , USA

5. School of Biological Sciences, University of Aberdeen , Cruickshank Building , St Machar Drive , Aberdeen , AB24 3UU , SC , UK

6. Department of Chemistry , Marine Biodiscovery Centre, University of Aberdeen , Aberdeen , AB24 3UE , SC , UK

Abstract

Abstract The objective of the present study is to examine the fine structure of vegetative cells of Laminaria digitata using both chemical fixation and cryofixation. Laminaria digitata was chosen due to its importance as a model organism in a wide range of biological studies, as a keystone species on rocky shores of the North Atlantic, its use of iodide as a unique inorganic antioxidant, and its significance as a raw material for the production of alginate. Details of the fine structural features of vegetative cells are described, with particular emphasis on the differences between the two methods used, i.e. conventional chemical fixation and freeze-fixation. The general structure of the cells was similar to that already described, with minor differences between the different cell types. An intense activity of the Golgi system was found associated with the thick external cell wall, with large dictyosomes from which numerous vesicles and cisternae are released. An interesting type of cisternae was found in the cryofixed material, which was not visible with the chemical fixation. These are elongated structures, in sections appearing tubule-like, close to the external cell wall or to young internal walls. An increased number of these structures was observed near the plasmodesmata of the pit fields. They are similar to the “flat cisternae” found associated with the forming cytokinetic diaphragm of brown algae. Their possible role is discussed. The new findings of this work underline the importance of such combined studies which reveal new data not known until now using the old conventional methods. The main conclusion of the present study is that cryofixation is the method of choice for studying Laminaria cytology by transmission electron microscopy.

Publisher

Walter de Gruyter GmbH

Subject

Plant Science,Aquatic Science,Ecology, Evolution, Behavior and Systematics

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