Biosynthesis and alternate targeting of the lysosomal cysteine protease cathepsin L.

J Collette, JP Bocock, K Ahn, RL Chapman… - International review of …, 2004 - europepmc.org
J Collette, JP Bocock, K Ahn, RL Chapman, G Godbold, S Yeyeodu, AH Erickson
International review of cytology, 2004europepmc.org
Upregulation of cathepsin L expression, whether during development or cell transformation,
or mediated by ectopic expression from a plasmid, alters the targeting of the protease and
thus its physiological function. Upregulated procathepsin L is targeted to small dense core
vesicles and to the dense cores of multivesicular bodies, as well as to lysosomes and to the
plasma membrane for selective secretion. The multivesicular vesicles resemble secretory
lysosomes characterized in specialized cell types in that they are endosomes that stably …
Upregulation of cathepsin L expression, whether during development or cell transformation, or mediated by ectopic expression from a plasmid, alters the targeting of the protease and thus its physiological function. Upregulated procathepsin L is targeted to small dense core vesicles and to the dense cores of multivesicular bodies, as well as to lysosomes and to the plasma membrane for selective secretion. The multivesicular vesicles resemble secretory lysosomes characterized in specialized cell types in that they are endosomes that stably store an upregulated protein and they possess the tetraspanin CD63. Morphologically the multivesicular endosomes also resemble late endosomes, but they store procathepsin L, not the active protease, and they are not the major site for LAMP-1 accumulation. Distinction between the lysosomal proenzyme and active protease thus identifies two populations of multivesicular endosomes in fibroblasts, one a storage compartment and one an enzymatically active compartment. A distinctive targeting pathway using aggregation is utilized to enrich the storage endosomes with a particular lysosomal protease that can potentially activate and be secreted.
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