Characterization of Aldosterone-producing Cell Cluster (APCC) at Single-cell Resolution

醛固酮合酶 醛固酮 肾小球带 甾体11β-羟化酶 肾上腺皮质 束状带 背景(考古学) 原发性醛固酮增多症 醛固酮增多症 内科学 内分泌学 生物 医学 肾素-血管紧张素系统 血管紧张素II 类固醇 古生物学 激素 血压
作者
Norifusa Iwahashi,Hironobu Umakoshi,Tsugio Seki,Celso E. Gómez-Sánchez,Kuniaki Mukai,Makoto Suematsu,Yuta Umezawa,Mototsugu Oya,Takeo Kosaka,Masahide Seki,Yutaka Suzuki,Yutaka Horiuchi,Yoshihiro Ogawa,Koshiro Nishimoto
出处
期刊:The Journal of Clinical Endocrinology and Metabolism [Oxford University Press]
卷期号:107 (9): 2439-2448 被引量:17
标识
DOI:10.1210/clinem/dgac394
摘要

Abstract Context The adrenal cortex consists of zona glomerulosa (ZG), fasciculata (ZF), and reticularis. Aldosterone-producing cell clusters (APCCs) that strongly express aldosterone synthase (CYP11B2) are frequently found in adult adrenals and harbor somatic mutations that are also detected in aldosterone-producing adenomas (APAs). Primary aldosteronism is mainly caused by APAs or idiopathic hyperaldosteronism (IHA). We presume that APCCs are causing IHA and are precursors of APAs. However, the gene expression characteristics and especially the development of APCCs are not well understood. Objective This study aimed to analyze the transcriptome of APCCs at single-cell resolution and infer the developmental trajectory. Methods Single-cell RNA sequencing (scRNA-seq) of 2 adult adrenals was performed. Results Immunohistochemical analyses confirmed the 2 adrenals had APCCs. scRNA-seq data of 2928 adrenal cells were obtained and 1765 adrenocortical cells were identified based on unsupervised clustering and the marker gene expression. The adrenocortical cells were divided into 6 clusters, of which 3 clusters (923 cells) were composed of APCC/ZG cells. By further subclustering, the APCC/ZG cells were divided into 3 clusters (clusters C1, C2, and C3), we finally identified APCC cluster (C3) and ZG cluster (C1). Cluster C2 seemed to be ZG-to-ZF transitional cells. RNA velocity analysis inferred the developmental direction from cluster ZG-cluster-C1 to APCC-cluster-C3. The scRNA-seq additionally revealed that many CYP11B2-positive cells were positive for CYP11B1 and/or CYP17A1, which were essential for cortisol but not for aldosterone production. Conclusions Our results revealed the gene expression characteristics of APCC at single-cell resolution and show that some ZG cells remodel to APCC.
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