Cathepsin D and its newly identified transport receptor Sez6l2 can modulate neurite outgrowth

Author:

Boonen Marielle1,Staudt Catherine1,Gilis Florentine1,Oorschot Viola2,Klumperman Judith2,Jadot Michel1

Affiliation:

1. URPhyM-Laboratoire de Chimie Physiologique, University of Namur, 61 rue de Bruxelles, 5000 Namur, Belgium

2. Department of Cell Biology, University Medical Center Utrecht, Heidelberglaan 100, 3584 CX Utrecht, The Netherlands

Abstract

How, in the absence of a functional mannose 6-phosphate (Man-6-P) signal-dependent transport pathway, some acid hydrolases remain sorted to endosomes/lysosomes in the brain is poorly understood. We demonstrate that cathepsin D binds to mouse Sez6l2, a type 1 transmembrane protein predominantly expressed in brain. Studies of the subcellular trafficking of Sez6l2, and its silencing in a mouse neuroblastoma cell line reveal that Sez6l2 is involved in the trafficking of cathepsin D to endosomes. Moreover, Sez6l2 can partially correct the cathepsin D hypersecretion resulting from the knock-down of GlcNAc-1-phosphotransferase in HeLa cells (i.e. unable to synthesize Man-6-P signals). Interestingly, cleavage of Sez6l2 by cathepsin D generates a N-terminal soluble fragment that induces neurite outgrowth, while its membrane counterpart prevents this. Taken together, our findings highlight that Sez6l2 can serve as receptor to mediate the sorting of cathepsin D to endosomes, and suggest that proteolytic cleavage of Sez6l2 by cathepsin D modulates neuronal differentiation.

Funder

F.R.S.-FNRS

Publisher

The Company of Biologists

Subject

Cell Biology

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