Missing a “Missing Self” Mechanism: Modeling and Detection of Ly49 Expression in Canine NK Cells

Author:

Gingrich Alicia A.1,Razmara Aryana M.1,Gingrich Phillip W.2,Rebhun Robert B.3ORCID,Murphy William J.4,Kent Michael S.3ORCID,Brown C. Titus5,Siegel Justin B.2,Canter Robert J.1ORCID

Affiliation:

1. *Department of Surgery, University of California, Davis School of Medicine, Sacramento, CA

2. †Department of Biochemistry and Molecular Medicine, University of California, Davis School of Medicine, Sacramento, CA

3. ‡Department of Surgical and Radiological Sciences, University of California, Davis School of Veterinary Medicine, Davis, CA

4. §Department of Dermatology, University of California, Davis School of Medicine, Sacramento, CA

5. ¶Department of Population Health and Reproduction, University of California, Davis School of Veterinary Medicine, Davis, CA

Abstract

Abstract NK cells are a key focus in immuno-oncology, based on their ability to eliminate malignant cells without prior sensitization. Dogs are valuable models for translational immunotherapy studies, especially for NK cells, where critical species differences exist between mice and humans. Given that the mechanism for recognition of “self” by canine NK cells is currently unknown, we sought to evaluate expression of Ly49 in canine NK cells using in silico and high-throughput techniques. We interrogated the identified polymorphism/mutation in canine Ly49 and assessed the potential impact on structure using computational modeling of three-dimensional protein structure and protein-protein docking of canine Ly49 with MHC class I (MHC-I). Bulk and single-cell RNA-sequencing analysis was performed to detect gene expression of Ly49/KLRA1 in resting and activated NK cells. Tertiary protein structure demonstrated significant structural similarity to the known murine system. Molecular docking of canine Ly49 with MHC-I was favorable, converging at a single low-energy conformation. RNA sequencing revealed expression of Ly49/KLRA1 in both resting and activated NK cells and demonstrated almost exclusive expression of the gene in the NK cluster at the single-cell level. Despite prior reports of a mutated, nonfunctional canine Ly49, our data support that the protein product is predicted to bind to MHC-I in a comparable conformation to the murine system and is expressed in canine NK cells with upregulation following activation. Taken together, these data suggest that Ly49 is capable of recognizing MHC-I and therefore regulating NK cell function in dogs.

Publisher

The American Association of Immunologists

Subject

Immunology and Allergy,General Medicine,Immunology

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