par Bosi, Emanuele;Marselli, Lorella;De Luca, Carmela;Suleiman, Mara;Tesi, Marta;Ibberson, Mark;Eizirik, Decio L. ;Cnop, Miriam ;Marchetti, Piero
Référence NAR Genomics and Bioinformatics, 3, 2, page (1)
Publication Publié, 2021-06
Référence NAR Genomics and Bioinformatics, 3, 2, page (1)
Publication Publié, 2021-06
Article révisé par les pairs
Résumé : | Pancreatic islet β-cell failure is key to the onset and progression of type 2 diabetes (T2D). The advent of single-cell RNA sequencing (scRNA-seq) has opened the possibility to determine transcriptional signatures specifically relevant for T2D at the β-cell level. Yet, applications of this technique have been underwhelming, as three independent studies failed to show shared differentially expressed genes in T2D β-cells. We performed an integrative analysis of the available datasets from these studies to overcome confounding sources of variability and better highlight common T2D β-cell transcriptomic signatures. After removing low-quality transcriptomes, we retained 3046 single cells expressing 27 931 genes. Cells were integrated to attenuate dataset-specific biases, and clustered into cell type groups. In T2D β-cells (n = 801), we found 210 upregulated and 16 downregulated genes, identifying key pathways for T2D pathogenesis, including defective insulin secretion, SREBP signaling and oxidative stress. We also compared these results with previous data of human T2D β-cells from laser capture microdissection and diabetic rat islets, revealing shared β-cell genes. Overall, the present study encourages the pursuit of single β-cell RNA-seq analysis, preventing presently identified sources of variability, to identify transcriptomic changes associated with human T2D and underscores specific traits of dysfunctional β- cells across different models and techniques. |