Polarized transport of the polymeric immunoglobulin receptor in transfected rabbit mammary epithelial cells.

Kraehenbuhl, J.P.

doi:10.1083/jcb.110.4.987

Titre

Polarized transport of the polymeric immunoglobulin receptor in transfected rabbit mammary epithelial cells.

Type

article

Institution

UNIL/CHUV/Unisanté + institutions partenaires

Périodique

Journal of Cell Biology

Auteur(s)

Schaerer, E.

Auteure/Auteur

Verrey, F.

Auteure/Auteur

Racine, L.

Auteure/Auteur

Tallichet, C.

Auteure/Auteur

Reinhardt, M.

Auteure/Auteur

Kraehenbuhl, J.P.

Auteure/Auteur

Liens vers les personnes

Kraehenbuhl, Jean-Pierre

Liens vers les unités

Inst. recherche Expériment. Cancer

ISSN

0021-9525

Statut éditorial

Publié

Date de publication

1990-04

Volume

110

Numéro

4

Première page

987

Dernière page/numéro d’article

998

Peer-reviewed

Oui

Langue

anglais

Notes

Publication types: Journal Article ; Research Support, Non-U.S. Gov't
Publication Status: ppublish

Résumé

A cDNA for the rabbit low Mr polymeric immunoglobulin (poly-Ig) receptor was expressed in an immortalized rabbit mammary cell line. The intracellular routing of the receptor and its cell surface expression was analyzed in stably transfected cells grown on permeable supports. Initially the cells formed a monolayer with no transmural electrical resistance. All monolayer cells expressed the poly-Ig receptor and cytokeratin 7 filaments characteristic of luminal mammary cells but absent in myoepithelial cells. Within 7 d in culture, the cells underwent cytodifferentiation and formed a bilayer with a transepithelial electrical resistance of approximately 500 omega x cm2. Upper layer cells formed tight junctions with adjacent cells and gap junctions with basal cells. Expression of the poly-Ig receptor and cytokeratin 7 was restricted to the cells from the upper layer. The kinetics of receptor biosynthesis and processing was similar to that reported for rabbit mammary gland and rat liver. The receptor was cleaved at the apical cell surface and release of secretory component into the apical medium occurred with a half-time of approximately 2 h. Selective cell surface trypsinization combined with pulse-chase experiments served to determine at which cell surface domain newly synthesized receptor appeared first. The receptor was digested with a half-time of approximately 60 min with trypsin present in the basolateral medium and 90 min with apical trypsin. These data are consistent with selective targeting of newly synthesized receptor to the basolateral surface. The results indicate that transcytosis of the receptor from basolateral to apical membrane in the presence or the absence of its ligand requires approximately 30 min. Cleavage of the receptor by endogenous protease is not concomitant with its appearance at the apical surface, but requires additional time, thus explaining the presence of intact receptor on the apical membrane.

PID Serval

serval:BIB_534D86EE1715

DOI

10.1083/jcb.110.4.987

PMID

1691196

WOS

A1990CX59200012

Permalien

https://iris.unil.ch/handle/iris/67575

Open Access

Oui

Date de création

2008-01-25T14:05:12.007Z

Date de création dans IRIS

2025-05-20T16:06:16Z

Fichier(s)

Nom

1691196_BIB_534D86EE1715.pdf

Version du manuscrit

published

Taille

3.08 MB

Format

Adobe PDF

PID Serval

serval:BIB_534D86EE1715.P001

Somme de contrôle

(MD5):b673a4e610cee3348e5b9f6c2ace39e9