PHAGOCYTOSIS OF LATEX BEADS BY ACANTHAMOEBA CASTELLANII (NEFF): III. Isolation of the Phagocytic Vesicles and Their Membranes

doi:10.1083/jcb.43.1.90

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ARTICLE

PHAGOCYTOSIS OF LATEX BEADS BY ACANTHAMOEBA CASTELLANII (NEFF)

: III. Isolation of the Phagocytic Vesicles and Their Membranes

Mary G. Wetzel ¹ and Edward D. Korn ¹

¹ From the Section on Cellular Physiology, Laboratory of Biochemistry, National Heart Institute, National Institutes of Health, Bethesda, Maryland 20014

A method is described for the rapid and efficient isolationof phagocytic vesicles from large scale cultures of Acanthamoebacastellanii (Neff) that have been incubated with polystyrenelatex beads. Cells were allowed to phagocytose latex beads for30 min and then were homogenized, and the phagocytic vesicleswere isolated by one centrifugation through several layers ofsucrose. Identity and purity of the phagocytic vesicles weredetermined by electron microscopy, chemical analyses, and assaysof acid phosphatase, $alpha$ - and ß-glucosidase, and reduced nicotinamideadenine dinucleotide dehydrogenase. When phagocytosis was allowedto occur for longer periods the phagocytic vesicles appearedto fuse with each other and perhaps with digestive vacuoles.The resultant vesicles which contained many beads were heavierthan those which consisted of only one bead or a few beads witha closely applied membrane. Ultrasonication ruptured the isolatedvesicles, and the membranes could then be isolated in 30–50%yield based on phospholipid analysis. These membranes were essentiallyfree of acid hydrolases and, presumably, other soluble proteins,as was also indicated by their low ratio of protein to phospholipid.The membranes have been prepared both as closed vesicles andas open sheets.

Submitted on March 10, 1969
Revised on April 29, 1969

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