CYTOCHEMISTRY AND ELECTRON MICROSCOPY: The Preservation of Cellular Ultrastructure and Enzymatic Activity by Aldehyde Fixation

doi:10.1083/jcb.17.1.19

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CYTOCHEMISTRY AND ELECTRON MICROSCOPY : The Preservation of Cellular Ultrastructure and Enzymatic Activity by Aldehyde Fixation

David D. Sabatini M.D.¹, Klaus Bensch M.D.¹, and Russell J. Barrnett M.D.¹

¹ From the Department of Anatomy, Yale University School of Medicine, New Haven.

Dr. Sabatini's present address is The Rockefeller Institute, New York. Dr. Bensch's address is Department of Pathology, Yale University School of Medicine

The aldehydes introduced in this paper and the more appropriateconcentrations for their general use as fixatives are: 4 to6.5 per cent glutaraldehyde, 4 per cent glyoxal, 12.5 per centhydroxyadipaldehyde, 10 per cent crotonaldehyde, 5 per centpyruvic aldehyde, 10 per cent acetaldehyde, and 5 per cent methacrolein.These were prepared as cacodylate- or phosphate-buffered solutions(0.1 to 0.2 M, pH 6.5 to 7.6) that, with the exception of glutaraldehyde,contained sucrose (0.22 to 0.55 M). After fixation of from 0.5hour to 24 hours, the blocks were stored in cold (4°C)buffer (0.1 M) plus sucrose (0.22 M). This material was usedfor enzyme histochemistry, for electron microscopy (both withand without a second fixation with 1 or 2 per cent osmium tetroxide)after Epon embedding, and for the combination of the two techniques.After fixation in aldehyde, membranous differentiations of thecell were not apparent and the nuclear structure differed fromthat commonly observed with osmium tetroxide. A postfixationin osmium tetroxide, even after long periods of storage, developedan image that—notable in the case of glutaraldehyde—waslargely indistinguishable from that of tissues fixed under optimalconditions with osmium tetroxide alone. Aliesterase, acetylcholinesterase,alkaline phosphatase, acid phosphatase, 5-nucleotidase, adenosinetriphosphatase, and DPNH and TPNH diaphorase activities weredemonstrable histochemically after most of the fixatives. Cytochromeoxidase, succinic dehydrogenase, and glucose-6-phosphatase wereretained after hydroxyaldipaldehyde and, to a lesser extent,after glyoxal fixation. The final product of the activity ofseveral of the above-mentioned enzymes was localized in relationto the fine structure. For this purpose the double fixationprocedure was used, selecting in each case the appropriate aldehyde.

Submitted on September 13, 1962

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