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Recycling and LFA-1-Dependent Trafficking of ICAM-1 to the Immunological Synapse

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Abstract
Little is known about how adhesion molecules On APCs accumulate at immunological synapses. We show here that ICAM-1 on APCs is continuously internalized and rapidly recycled back to the interface after antigen-priming T-cell contact. The internalization rate is high in APCs, including Raji B cells and dendritic cells, but low in endothelial cells. Internalization is significantly reduced by inhibitors of Na+/H+ exchangers (NHEs), suggesting that members of the NHE-family regulate this process. Once internalized, ICAM-1 is co-localized with MHC class II in the polarized recycling compartment. Surprisingly, not only ICAM-1, but also MFIC class II, is targeted to the immunological synapse through LFA-1-dependent adhesion. Cytosolic ICAM-1 is highly mobile and forms a tubular structure. Inhibitors of microtubule or actin polymerization can reduce ICAM-1 mobility, and thereby block accumulation at immunological synapses. Membrane ICAM-1 also moves to the T-cell contact zone, presumably through an active, cytoskeleton-dependent mechanism. Collectively, these results demonstrate that ICAM-1 can be transported to the immunological synapse through the recycling compartment. Furthermore, the high-affinity state of LFA-1 on T cells is critical to induce targeted movements of both ICAM-1 and MHC class II to the immunological synapse on APCs. J. Cell. Biochem. 111: 1125-1137, 2010. (C) 2010 Wiley-Liss, Inc.
Author(s)
Jo, Jae-HyeokKwon, Min-SungChoi, Hyang-OkOh, Hyun-MeeKim, Hyang-JinJun, Chang-Duk
Issued Date
2010-12
Type
Article
DOI
10.1002/jcb.22798
URI
https://scholar.gist.ac.kr/handle/local/16546
Publisher
John Wiley & Sons Inc.
Citation
Journal of Cellular Biochemistry, v.111, no.5, pp.1125 - 1137
ISSN
0730-2312
Appears in Collections:
Department of Life Sciences > 1. Journal Articles
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