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Journal of Cell Science 115, 2485-2495 (2002)
© 2002 The Company of Biologists Limited


Research Article

Involvement of ASIP/PAR-3 in the promotion of epithelial tight junction formation

Tomonori Hirose1, Yasushi Izumi1, Yoji Nagashima2, Yoko Tamai-Nagai1, Hidetake Kurihara3, Tatsuo Sakai3, Yukari Suzuki1, Tomoyuki Yamanaka1, Atsushi Suzuki1, Keiko Mizuno1 and Shigeo Ohno1,*

1 Department of Molecular Biology, Yokohama City University School of Medicine, Kanazawa-ku, Yokohama 236-0004, Japan
2 Department of Pathology, Yokohama City University School of Medicine, Kanazawa-ku, Yokohama 236-0004, Japan
3 Department of Anatomy, Juntendo University School of Medicine, Bunkyo-ku, Tokyo 113-8421, Japan

* Author for correspondence (e-mail: ohnos{at}med.yokohama-cu.ac.jp )

Accepted 10 April 2002

The mammalian protein ASIP/PAR-3 interacts with atypical protein kinase C isotypes (aPKC) and shows overall sequence similarity to the invertebrate proteins C. elegans PAR-3 and Drosophila Bazooka, which are crucial for the establishment of polarity in various cells. The physical interaction between ASIP/PAR-3 and aPKC is also conserved in C. elegans PAR-3 and PKC-3 and in Drosophila Bazooka and DaPKC. In mammals, ASIP/PAR-3 colocalizes with aPKC and concentrates at the tight junctions of epithelial cells, but the biological meaning of ASIP/PAR-3 in tight junctions remains to be clarified. In the present study, we show that ASIP/PAR-3 staining distributes to the subapical domain of epithelial cell-cell junctions, including epithelial cells with less-developed tight junctions, in clear contrast with ZO-1, another tight-junction-associated protein, the staining of which is stronger in cells with well-developed tight junctions. Consistently, immunogold electron microscopy revealed that ASIP/PAR-3 concentrates at the apical edge of tight junctions, whereas ZO-1 distributes alongside tight junctions. To clarify the meaning of this characteristic localization of ASIP, we analyzed the effects of overexpressed ASIP/PAR-3 on tight junction formation in cultured epithelial MDCK cells. The induced overexpression of ASIP/PAR-3, but not its deletion mutant lacking the aPKC-binding sequence, promotes cell-cell contact-induced tight junction formation in MDCK cells when evaluated on the basis of transepithelial electrical resistance and occludin insolubilization. The significance of the aPKC-binding sequence in tight junction formation is also supported by the finding that the conserved PKC-phosphorylation site within this sequence, ASIP-Ser827, is phosphorylated at the most apical tip of cell-cell contacts during the initial phase of tight junction formation in MDCK cells. Together, our present data suggest that ASIP/PAR-3 regulates epithelial tight junction formation positively through interaction with aPKC.

Key words: ASIP/PAR-3, Atypical PKC, Epithelial tight junction, Epithelial cell polarity


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