LILRB1 polymorphisms influence posttransplant HCMV susceptibility and ligand interactions
Kang Yu, … , Swiss Transplant Cohort Study, Deborah N. Burshtyn
Kang Yu, … , Swiss Transplant Cohort Study, Deborah N. Burshtyn
Published March 12, 2018
Citation Information: J Clin Invest. 2018;128(4):1523-1537. https://doi.org/10.1172/JCI96174.
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Research Article Immunology Infectious disease

LILRB1 polymorphisms influence posttransplant HCMV susceptibility and ligand interactions

Abstract

UL18 is a human CMV (HCMV) MHC class I (MHCI) homolog that efficiently inhibits leukocyte immunoglobulin-like receptor subfamily B member 1 (LILRB1)+ NK cells. We found an association of LILRB1 polymorphisms in the regulatory regions and ligand-binding domains with control of HCMV in transplant patients. Naturally occurring LILRB1 variants expressed in model NK cells showed functional differences with UL18 and classical MHCI, but not with HLA-G. The altered functional recognition was recapitulated in binding assays with the binding domains of LILRB1. Each of 4 nonsynonymous substitutions in the first 2 LILRB1 immunoglobulin domains contributed to binding with UL18, classical MHCI, and HLA-G. One of the polymorphisms controlled addition of an N-linked glycan, and that mutation of the glycosylation site altered binding to all ligands tested, including enhancing binding to UL18. Together, these findings indicate that specific LILRB1 alleles that allow for superior immune evasion by HCMV are restricted by mutations that limit LILRB1 expression selectively on NK cells. The polymorphisms also maintained an appropriate interaction with HLA-G, fitting with a principal role of LILRB1 in fetal tolerance.

Authors

Kang Yu, Chelsea L. Davidson, Agnieszka Wójtowicz, Luiz Lisboa, Ting Wang, Adriana M. Airo, Jean Villard, Jeremie Buratto, Tatyana Sandalova, Adnane Achour, Atul Humar, Katia Boggian, Alexia Cusini, Christian van Delden, Adrian Egli, Oriol Manuel, Nicolas Mueller, Pierre-Yves Bochud, Swiss Transplant Cohort Study, Deborah N. Burshtyn

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Figure 3

Functional activity of LILRB1-PTTI and -LAIS variants.

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Functional activity of LILRB1-PTTI and -LAIS variants. (A) Expression of...
(A) Expression of HA–UL18-YFP on transduced 721.221 cells (left). MFIs are corrected for background staining in each case. (B) Surface expression of LILRB1 on YTS cells and LILRB1-transduced YTS cells detected with α-HA or α-LILRB1 (HPF1). (C) Surface expression of MHCI on transduced 721.221 cells detected with W6/32. (D) Specific lysis of 721.221 cells; 721.221 cells presenting HLA-Cw15, HLA-G, and UL18 by YTS; and YTS cells expressing LILRB1. Upper panel: representative result from 6 independent assays with 3 E/T ratios. Lower panel: aggregated result of 6 experiments at an E/T of 10:1; error bars indicate SD. *P < 0.05 determined by paired samples t test. (E) Lysis was determined in the presence of 10 μg/ml α-LILRB1 (HPF1) or isotype control IgG1κ at an E/T of 10:1. Results are aggregated from 3 independent tests. Error bars indicate SD. *P < 0.05 as determined by paired samples t test.