Pure suspensions of human lymphocytes were separated from peripheral blood by means of nylon wool, homogenized in 0.34 M sucrose-0.01 M EDTA solution, and fractionated by differential centrifugation. The bulk of acid hydrolase activity was found to be concentrated in a 20,000 g x 20 min granular fraction, whereas nuclear, debris, and supernatant fractions contained lesser concentrations of hydrolases. Acid hydrolase activity present in the granular fraction showed appropriate "latency" as judged by its dose-dependent release into the 20,000 g x 20 min supernatant after exposure to membrane-disruptive agents such as streptolysin S, filipin, and lysolecithin. Heparin proved to be necessary in the suspending medium so that reproducible homogenization and cell fractionation could be obtained. Even excessive contamination of lymphocyte suspensions with platelets did not appreciably alter the acid hydrolase activity of lymphocyte homogenates or the distribution of enzymes in subcellular fractions. Discontinuous density-gradient centrifugation of a 500 g x 10 min supernatant, containing both acid hydrolase-rich organelles and mitochondria, resulted in partial resolution of hydrolase-rich organelles from mitochondria. Fine structural studies of the intact lymphocytes showed the presence of acid phosphatase-positive, membrane-bounded organelles. Electron microscopy of the "large granule" (20,000 g x 20 min) fraction of such lymphocytes demonstrated 80–90% mitochondria, 5–10% platelets, and 5–10% membrane-bounded acid phosphatase-positive structures. The data indicate the presence in human peripheral blood lymphocytes of acid hydrolase-rich granules which possess many of the biochemical and structural characteristics of lysosomes in other tissues.
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1 May 1968
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May 01 1968
STUDIES ON LYSOSOMES : XI. Characterization of a Hydrolase-Rich Fraction from Human Lymphocytes
Günter Brittinger,
Günter Brittinger
From the Department of Medicine, the New York University School of Medicine, New York 10016 and the Department of Medicine, the University of California Medical School, San Francisco, California
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Rochelle Hirschhorn,
Rochelle Hirschhorn
From the Department of Medicine, the New York University School of Medicine, New York 10016 and the Department of Medicine, the University of California Medical School, San Francisco, California
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Steven D. Douglas,
Steven D. Douglas
From the Department of Medicine, the New York University School of Medicine, New York 10016 and the Department of Medicine, the University of California Medical School, San Francisco, California
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Gerald Weissmann
Gerald Weissmann
From the Department of Medicine, the New York University School of Medicine, New York 10016 and the Department of Medicine, the University of California Medical School, San Francisco, California
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Günter Brittinger
From the Department of Medicine, the New York University School of Medicine, New York 10016 and the Department of Medicine, the University of California Medical School, San Francisco, California
Rochelle Hirschhorn
From the Department of Medicine, the New York University School of Medicine, New York 10016 and the Department of Medicine, the University of California Medical School, San Francisco, California
Steven D. Douglas
From the Department of Medicine, the New York University School of Medicine, New York 10016 and the Department of Medicine, the University of California Medical School, San Francisco, California
Gerald Weissmann
From the Department of Medicine, the New York University School of Medicine, New York 10016 and the Department of Medicine, the University of California Medical School, San Francisco, California
Received:
October 24 1967
Revision Received:
January 10 1968
Online ISSN: 1540-8140
Print ISSN: 0021-9525
1968
J Cell Biol (1968) 37 (2): 394–411.
Article history
Received:
October 24 1967
Revision Received:
January 10 1968
Citation
Günter Brittinger, Rochelle Hirschhorn, Steven D. Douglas, Gerald Weissmann; STUDIES ON LYSOSOMES : XI. Characterization of a Hydrolase-Rich Fraction from Human Lymphocytes . J Cell Biol 1 May 1968; 37 (2): 394–411. doi: https://doi.org/10.1083/jcb.37.2.394
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