Table_2.xlsx

Abstract

Objectives: Alterations in natural killer (NK) cells activity cause damage to pancreatic islets in type 1 diabetes mellitus (T1DM). The aim of this study is to identify T1DM ketosis or ketoacidosis related genes in activated CD56+CD16+ NK cells. Methods: Microarray datasets were downloaded from Gene Expression Omnibus (GEO) database. Differentially expressed genes (DEGs) were analyzed using GEO2R tool. Enrichment analyses were performed using Metascape online database and GSEA software. Cell-specific gene coexpression network was built using NetworkAnalyst tools. Cytoscape software was used to identify hub genes and construct co-expressed networks. Target miRNAs were predicted based on the DIANA-micro T, miRDB and miRWalk online databases. Results: A total of 70 DEGs were identified between T1DM patients recovered from ketosis or ketoacidosis and healthy control blood samples in GSE44314. Among the DEGs, 10 hub gene were screened out. The mature NK cell-specific gene coexpression network for DEGs in T1DM was built using NetworkAnalyst tools. DEGs between activated CD56+CD16+ NK cells and CD56brightCD16- NK cells were identified from GSE1511. After intersection, 13 overlapping genes between GSE44314 and GSE1511 microarray datasets were screened out, in which 7 hub genes were identified. Additionally, 59 target miRNAs were predicted according to the 7 hub genes. After validated with miRNA expression profile dataset of GSE97123, 7 differentially expressed miRNAs (DEmiRNAs) in plasma-derived exosome were selected. Finally, a mRNA-miRNA network was constructed, which involved in T1DM ketosis or ketoacidosis process. Conclusion: This work identified 7 hub genes in activated CD56+CD16+ NK cells and 7 miRNAs in plasma-derived exosome as potential predictors of T1DM ketoacidosis, which provided novel insight for the pathogenesis at transcriptome level.