Beef liver catalase was injected intravenously into mice, and its distribution in the kidney, myocardium, and liver was studied with the electron microscope. A specific and relatively sensitive method was developed for its ultrastructural localization, based on the peroxidatic activity of catalase and employing a modified Graham and Karnovsky incubation medium. The main features of the medium were a higher concentration of diaminobenzidine, barium peroxide as the source of peroxide, and pH of 8.5. Ultrastructurally, the enzyme was seen to permeate the endothelial fenestrae and basement membranes of tubular and glomerular capillaries of the kidney. The urinary space and tubular lumina contained no reaction product. In the myocardial capillaries, the tracer filled the pinocytotic vesicles but did not diffuse across the intercellular clefts of the endothelium. In liver, uptake of catalase was seen both in hepatocytes and in Kupffer cells.
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1 August 1969
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August 01 1969
THE USE OF BEEF LIVER CATALASE AS A PROTEIN TRACER FOR ELECTRON MICROSCOPY
M. A. Venkatachalam,
M. A. Venkatachalam
From the Harvard Pathology Unit, Mallory Institute of Pathology, Boston City Hospital, Boston, Massachusetts 02118
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H. Dariush Fahimi
H. Dariush Fahimi
From the Harvard Pathology Unit, Mallory Institute of Pathology, Boston City Hospital, Boston, Massachusetts 02118
Search for other works by this author on:
M. A. Venkatachalam
From the Harvard Pathology Unit, Mallory Institute of Pathology, Boston City Hospital, Boston, Massachusetts 02118
H. Dariush Fahimi
From the Harvard Pathology Unit, Mallory Institute of Pathology, Boston City Hospital, Boston, Massachusetts 02118
Received:
February 03 1969
Revision Received:
April 04 1969
Online ISSN: 1540-8140
Print ISSN: 0021-9525
Copyright © 1969 by The Rockefeller University Press.
1969
J Cell Biol (1969) 42 (2): 480–489.
Article history
Received:
February 03 1969
Revision Received:
April 04 1969
Citation
M. A. Venkatachalam, H. Dariush Fahimi; THE USE OF BEEF LIVER CATALASE AS A PROTEIN TRACER FOR ELECTRON MICROSCOPY . J Cell Biol 1 August 1969; 42 (2): 480–489. doi: https://doi.org/10.1083/jcb.42.2.480
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