Literature DB >> 24501197

Three tapasin docking sites in TAP cooperate to facilitate transporter stabilization and heterodimerization.

Ralf M Leonhardt1, Parwiz Abrahimi, Susan M Mitchell, Peter Cresswell.   

Abstract

The TAP translocates peptide Ags into the lumen of the endoplasmic reticulum for loading onto MHC class I molecules. MHC class I acquires its peptide cargo in the peptide loading complex, an oligomeric complex that the chaperone tapasin organizes by bridging TAP to MHC class I and recruiting accessory molecules such as ERp57 and calreticulin. Three tapasin binding sites on TAP have been described, two of which are located in the N-terminal domains of TAP1 and TAP2. The third binding site is present in the core transmembrane (TM) domain of TAP1 and is used only by the unassembled subunits. Tapasin is required to promote TAP stability, but through which binding site(s) it is acting is unknown. In particular, the role of tapasin binding to the core TM domain of TAP1 single chains is mysterious because this interaction is lost upon TAP2 association. In this study, we map the respective binding site in TAP1 to the polar face of the amphipathic TM helix TM9 and identify key residues that are essential to establish the interaction. We find that this interaction is dispensable for the peptide transport function but essential to achieve full stability of human TAP1. The interaction is also required for proper heterodimerization of the transporter. Based on similar results obtained using TAP mutants that lack tapasin binding to either N-terminal domain, we conclude that all three tapasin-binding sites in TAP cooperate to achieve high transporter stability and efficient heterodimerization.

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Year:  2014        PMID: 24501197      PMCID: PMC3943870          DOI: 10.4049/jimmunol.1302637

Source DB:  PubMed          Journal:  J Immunol        ISSN: 0022-1767            Impact factor:   5.422


  50 in total

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5.  Critical role for the tapasin-docking site of TAP2 in the functional integrity of the MHC class I-peptide-loading complex.

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2.  Cytosolic Processing Governs TAP-Independent Presentation of a Critical Melanoma Antigen.

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Review 3.  A personal retrospective on the mechanisms of antigen processing.

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5.  Melanosomal formation of PMEL core amyloid is driven by aromatic residues.

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6.  Repeat domain-associated O-glycans govern PMEL fibrillar sheet architecture.

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7.  Identification of critical amino acid residues in the regulatory N-terminal domain of PMEL.

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8.  Modular transcriptional repertoire and MicroRNA target analyses characterize genomic dysregulation in the thymus of Down syndrome infants.

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Review 9.  Moving the Cellular Peptidome by Transporters.

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