The non-ELR CXC chemokine encoded by human cytomegalovirus UL146 genotype 5 contains a C-terminal β-hairpin and induces neutrophil migration as a selective CXCR2 agonist

• Published in: PLoS pathogens Vol. 18; no. 3; p. e1010355
• Main Authors: Berg, Christian, Wedemeyer, Michael J, Melynis, Motiejus, Schlimgen, Roman R, Hansen, Lasse H, Våbenø, Jon, Peterson, Francis C, Volkman, Brian F, Rosenkilde, Mette M, Lüttichau, Hans R
• Format: Journal Article
• Language: English
• Published: United States Public Library of Science 01.03.2022; Public Library of Science (PLoS)
• Subjects: Acquired immune deficiency syndrome; Agonists; AIDS; Arrestin; Assaying; Biology and Life Sciences; Cell Movement; Chemokine receptors; Chemokines; Chemokines, CXC - genetics; Chemotaxis; Clinical isolates; CXC chemokines; CXCR2 protein; Cytomegalovirus; Cytomegalovirus - genetics; Destabilization; Genes; Genotype; Genotype & phenotype; Genotypes; Humans; Immunocompromised hosts; Infections; Interleukin-8; Leukocyte migration; Leukocytes (neutrophilic); Ligands; Mass spectrometry; Medicine and Health Sciences; Neutrophils; Neutrophils - cytology; NMR; Nuclear magnetic resonance; Peptides; Physical Sciences; Proteins; Receptors; Receptors, Interleukin-8A - genetics; Receptors, Interleukin-8B - agonists; Receptors, Interleukin-8B - genetics; Research and Analysis Methods; Scientific imaging; Signaling; Tryptophan
• ISSN: 1553-7374; 1553-7366; 1553-7374
• DOI: 10.1371/journal.ppat.1010355

Human cytomegalovirus (HCMV) is a major pathogen in immunocompromised patients. The UL146 gene exists as 14 diverse genotypes among clinical isolates, which encode 14 different CXC chemokines. One genotype (vCXCL1GT1) is a known agonist for CXCR1 and CXCR2, while two others (vCXCL1GT5 and vCXCL1GT6) lack the ELR motif considered crucial for CXCR1 and CXCR2 binding, thus suggesting another receptor targeting profile. To determine the receptor target for vCXCL1GT5, the chemokine was probed in a G protein signaling assay on all 18 classical human chemokine receptors, where CXCR2 was the only receptor being activated. In addition, vCXCL1GT5 recruited β-arrestin in a BRET-based assay and induced migration in a chemotaxis assay through CXCR2, but not CXCR1. In contrast, vCXCL1GT1 stimulated G protein signaling, recruited β-arrestin and induced migration through both CXCR1 and CXCR2. Both vCXCL1GT1 and vCXCL1GT5 induced equally potent and efficacious migration of neutrophils, and ELR vCXCL1GT4 and non-ELR vCXCL1GT6 activated only CXCR2. In contrast to most human chemokines, the 14 UL146 genotypes have remarkably long C-termini. Comparative modeling using Rosetta showed that each genotype could adopt the classic chemokine core structure, and predicted that the extended C-terminal tail of several genotypes (including vCXCL1GT1, vCXCL1GT4, vCXCL1GT5, and vCXCL1GT6) forms a novel β-hairpin not found in human chemokines. Secondary NMR shift and TALOS+ analysis of vCXCL1GT1 supported the existence of two stable β-strands. C-terminal deletion of vCXCL1GT1 resulted in a non-functional protein and in a shift to solvent exposure for tryptophan residues likely due to destabilization of the chemokine fold. The results demonstrate that non-ELR chemokines can activate CXCR2 and suggest that the UL146 chemokines have unique C-terminal structures that stabilize the chemokine fold. Increased knowledge of the structure and interaction partners of the chemokine variants encoded by UL146 is key to understanding why circulating HCMV strains sustain 14 stable genotypes.