A cryoembedding method for cutting ultrathin cryosections from small frozen specimens

1 October 1984

journal article
research article
Published by Wiley in Journal of Microscopy

Vol. 136 (1) , 69-75
https://doi.org/10.1111/j.1365-2818.1984.tb02546.x

Abstract

A technique is described which allows one to embed small frozen specimens for easy sectioning in a cryoultramicrotome. n‐Heptane is recommended as a cryoembedding medium due to its suitable melting point (182.4 K), high vapour pressure, chemical inertia, and good sectioning properties when solid. Freeze dried cryosections of cultured muscle cells, slime moulds, insect antennae and unicellular algae are presented as examples. There is no evidence that the preparation disturbs the distribution of soluble elements in the specimen, since X‐ray spectra of muscle cells exposed to heptane do not differ from those of samples not exposed.

Keywords

This publication has 9 references indexed in Scilit:

Pheromone receptors in Bombyx mori and Antheraea pernyi
Cell and tissue research, 1984
Preparation of biological cryosections for analytical electron microscopy
Ultramicroscopy, 1982
Experiments on freezing damage with freeze substitution using moth antennae as test objects
Journal of Microscopy, 1982
Cryoultramicrotomy: evidence against melting and the use of a low temperature cement for specimen orientation
Journal of Microscopy, 1982
Cryofixation: A Tool In Biological Ultrastructural Research
Published by Elsevier ,1982
Cryofixation without cryoprotectants. Freeze substitution and freeze etching of an insect olfactory receptor
Tissue and Cell, 1980
X-ray microanalysis of receptor lymph in a cuticular arthropod sensillum
Journal of comparative physiology, 1976
The Sex-Attractant Receptor of Moths
Scientific American, 1974
Improved Cryofixation Applicable to Freeze Etching
Proceedings of the National Academy of Sciences, 1971