Study of cellular heterogeneity and differential dynamics of autophagy in human embryonic kidney development by single-cell RNA sequencing

Chen Wen-jin; Pan Xiu-wu; Chu Jian; Xu Da; Chen Jia-xin; Chen Wei-jie; Wang Lin-hui; Cui Xin-gang

doi:10.1186/s12935-021-02154-w

Cancer Cell International (Aug 2021)

Study of cellular heterogeneity and differential dynamics of autophagy in human embryonic kidney development by single-cell RNA sequencing

Chen Wen-jin,
Pan Xiu-wu,
Chu Jian,
Xu Da,
Chen Jia-xin,
Chen Wei-jie,
Wang Lin-hui,
Cui Xin-gang

Affiliations

Chen Wen-jin: Department of Urology, The Third Affiliated Hospital of Second Military Medical University
Pan Xiu-wu: Department of Urology, The Third Affiliated Hospital of Second Military Medical University
Chu Jian: Department of Urology, The Third Affiliated Hospital of Second Military Medical University
Xu Da: Department of Urology, The Third Affiliated Hospital of Second Military Medical University
Chen Jia-xin: Department of Urology, The Third Affiliated Hospital of Second Military Medical University
Chen Wei-jie: Department of Urology, The Third Affiliated Hospital of Second Military Medical University
Wang Lin-hui: Department of Urology, Changzheng Hospital of Second Military Medical University
Cui Xin-gang: Department of Urology, The Third Affiliated Hospital of Second Military Medical University

DOI: https://doi.org/10.1186/s12935-021-02154-w
Journal volume & issue: Vol. 21, no. 1
pp. 1 – 16

Abstract

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Abstract Background Autophagy is believed to participate in embryonic development, but whether the expression of autophagy-associated genes undergoes changes during the development of human embryonic kidneys remains unknown. Methods In this work, we identified 36,151 human renal cells from embryonic kidneys of 9–18 gestational weeks in 16 major clusters by single-cell RNA sequencing (scRNA-seq), and detected 1350 autophagy-related genes in all fetal renal cells. The abundance of each cell cluster in Wilms tumor samples from scRNA-seq and GDC TARGET WT datasets was detected by CIBERSORTx. R package Monocle 3 was used to determine differentiation trajectories. Cyclone tool of R package scran was applied to calculate the cell cycle scores. R package SCENIC was used to investigate the transcriptional regulons. The FindMarkers tool from Seurat was used to calculate DEGs. GSVA was used to perform gene set enrichment analyses. CellphoneDB was utilized to analyze intercellular communication. Results It was found that cells in the 13th gestational week showed the lowest transcriptional level in each cluster in all stages. Nephron progenitors could be divided into four subgroups with diverse levels of autophagy corresponding to different SIX2 expressions. SSBpod (podocyte precursors) could differentiate into four types of podocytes (Pod), and autophagy-related regulation was involved in this process. Pseudotime analysis showed that interstitial progenitor cells (IPCs) potentially possessed two primitive directions of differentiation to interstitial cells with different expressions of autophagy. It was found that NPCs, pretubular aggregates and interstitial cell clusters had high abundance in Wilms tumor as compared with para-tumor samples with active intercellular communication. Conclusions All these findings suggest that autophagy may be involved in the development and cellular heterogeneity of early human fetal kidneys. In addition, part of Wilms tumor cancer cells possess the characteristics of some fetal renal cell clusters. Graphical abstract

Published in Cancer Cell International

ISSN: 1475-2867 (Online)
Publisher: BMC
Country of publisher: United Kingdom
LCC subjects: Medicine: Internal medicine: Neoplasms. Tumors. Oncology. Including cancer and carcinogens; Science: Biology (General): Cytology
Website: https://cancerci.biomedcentral.com

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