DOI: 10.1083/jcb.104.4.875. Rapid analytical and preparative isolation of functional endosomes by free flow electrophoresis

Rapid analytical and preparative isolation of functional endosomes by free flow electrophoresis

10.1083/jcb.104.4.875

Crossref journal-article

Rockefeller University Press

The Journal of cell biology (291)

Abstract

Endosomes are prelysosomal organelles that serve as an intracellular site for the sorting, distribution, and processing of receptors, ligands, fluid phase components, and membrane proteins internalized by endocytosis. Whereas the overall functions of endosomes are increasingly understood, little is known about endosome structure, composition, or biogenesis. In this paper, we describe a rapid procedure that permits analytical and preparative isolation of endosomes from a variety of tissue culture cells. The procedure relies on a combination of density gradient centrifugation and free flow electrophoresis. It yields a fraction of highly purified, functionally intact organelles. As markers for endosomes in Chinese hamster ovary cells, we used endocytosed horseradish peroxidase, FITC-conjugated dextran, and [35S]methionine-labeled Semliki Forest virus. Total postnuclear supernatants, crude microsomal pellets, or partially purified Golgi fractions were subjected to free flow electrophoresis. Endosomes and lysosomes migrated together as a single anodally deflected peak separated from most other organelles (plasma membrane, mitochondria, endoplasmic reticulum, and Golgi). The endosomes and lysosomes were then resolved by centrifugation in Percoll density gradients. Endosomes prepared in this way were enriched up to 70-fold relative to the initial homogenate and were still capable of ATP-dependent acidification. By electron microscopy, the isolated organelles were found to consist of electron lucent vacuoles and tubules, many of which could be shown to contain an endocytic tracer (e.g., horseradish peroxidase). SDS PAGE analysis of integral and peripheral membrane proteins (separated from each other by condensation in Triton X-114) revealed a unique and restricted subset of proteins when compared with lysosomes, the unshifted free flow electrophoresis peak, and total cell protein. Altogether, the purification procedure takes 5-6 h and yields amounts of endosomes (150-200 micrograms protein) sufficient for biochemical, immunological, and functional analysis.

Bibliography

Marsh, M., Schmid, S., Kern, H., Harms, E., Male, P., Mellman, I., & Helenius, A. (1987). Rapid analytical and preparative isolation of functional endosomes by free flow electrophoresis. The Journal of Cell Biology, 104(4), 875â886.

Authors 7

M Marsh (first)
S Schmid (additional)
H Kern (additional)
E Harms (additional)
P Male (additional)
I Mellman (additional)
A Helenius (additional)

References 0 Referenced 157

None

Dates

Type	When
Created	21 years, 3 months ago (May 14, 2004, 8:18 p.m.)
Deposited	2 years, 1 month ago (July 21, 2023, 8:10 p.m.)
Indexed	4 months, 2 weeks ago (April 5, 2025, 2:07 p.m.)
Issued	38 years, 4 months ago (April 1, 1987)
Published	38 years, 4 months ago (April 1, 1987)
Published Online	38 years, 4 months ago (April 1, 1987)
Published Print	38 years, 4 months ago (April 1, 1987)

Funders 0

None

BibTeX

@article{Marsh_1987, title={Rapid analytical and preparative isolation of functional endosomes by free flow electrophoresis}, volume={104}, ISSN={1540-8140}, url={http://dx.doi.org/10.1083/jcb.104.4.875}, DOI={10.1083/jcb.104.4.875}, number={4}, journal={The Journal of cell biology}, publisher={Rockefeller University Press}, author={Marsh, M and Schmid, S and Kern, H and Harms, E and Male, P and Mellman, I and Helenius, A}, year={1987}, month=apr, pages={875–886} }

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