Genes & Human Disease Research Program, Oklahoma Medical Research Foundation, Oklahoma City, OK, USA.
Genes & Human Disease Research Program, Oklahoma Medical Research Foundation, Oklahoma City, OK, USA.
Exp Eye Res. 2024 Nov;248:110101. doi: 10.1016/j.exer.2024.110101. Epub 2024 Sep 18.
Endothelial cells (ECs) display organ- and tissue-specific heterogeneity. In the eye, the retinal and choroidal vascular beds are distinct networks with different molecular and morphological properties that serve location-specific functions, i.e., the former maintaining a tight barrier and the latter, a permeable fenestrated vasculature. Given that retinal health critically relies on the function of these vascular beds and that their dysfunction is implicated in a variety of retinal diseases, a molecular understanding of both physiological and pathophysiological characteristics of these distinct vasculatures is critical. Given their interspersed anatomic distribution among parenchymal cells, the study of EC gene expression, in vivo, has been hampered by the challenge of isolating pure populations of ocular ECs in sufficient quantities for large-scale transcriptomics. To address this challenge, we present a methodological and analytical workflow to facilitate inter-tissue comparisons of the in vivo EC translatome isolated from choroid, retina, and brain using the Cre-inducible NuTRAP flox construct and two widely-used endothelial Cre mouse lines: constitutive Tie2-Cre and tamoxifen-inducible Cdh5-CreERT2. For each Cre line, inter-tissue comparison of TRAP-RNAseq enrichment (TRAP-isolated translatome vs input transcriptome) showed tissue-specific gene enrichments with differential pathway representation. For each mouse model, inter-tissue comparison of the EC translatome (choroid vs brain, choroid vs retina, and brain vs retina) showed over 50% overlap of differentially expressed genes (DEGs) between the three paired comparisons, with differential pathway representation for each tissue. Pathway analysis of DEGs in the Cdh5-NuTRAP vs Tie2-NuTRAP comparison for retina, choroid, and brain predicted inhibition of processes related to myeloid cell function and activation, consistent with more specific targeting of ECs in the Cdh5-NuTRAP than in the Tie2-NuTRAP model which also targets hematopoietic progenitors giving rise to immune cells. Indeed, while TRAP enriches for EC transcripts in both models, myeloid transcripts were also captured in the Tie2-NuTRAP model which was confirmed using cell sorting. We suggest experimental/analytical considerations should be taken when selecting Cre-lines to target ECs.
内皮细胞(ECs)表现出器官和组织特异性的异质性。在眼睛中,视网膜和脉络膜血管床是具有不同分子和形态特性的独特网络,它们具有特定位置的功能,即前者维持紧密的屏障,后者则具有可渗透的有窗孔的血管系统。鉴于视网膜的健康严重依赖于这些血管床的功能,并且它们的功能障碍与多种视网膜疾病有关,因此对这些不同血管系统的生理和病理生理特征的分子理解至关重要。鉴于它们在实质细胞之间的穿插解剖分布,体内研究 EC 基因表达受到挑战,因为难以分离足够数量的纯眼部 EC 群体用于大规模转录组学。为了解决这一挑战,我们提出了一种方法学和分析工作流程,以使用 Cre 诱导型 NuTRAP flox 构建体和两种广泛使用的内皮 Cre 小鼠品系(组成型 Tie2-Cre 和他莫昔芬诱导型 Cdh5-CreERT2)从脉络膜、视网膜和大脑中分离的体内 EC 翻译组进行组织间比较。对于每条 Cre 线,TRAP-RNAseq 富集的组织间比较(TRAP 分离的翻译组与输入转录组)显示出具有不同途径表示的组织特异性基因富集。对于每种小鼠模型,EC 翻译组的组织间比较(脉络膜与大脑、脉络膜与视网膜和大脑与视网膜)显示出三个配对比较之间超过 50%的差异表达基因(DEG)重叠,每个组织的差异途径表示。Cdh5-NuTRAP 与 Tie2-NuTRAP 比较中视网膜、脉络膜和大脑的 DEG 的通路分析预测与髓样细胞功能和激活相关的过程被抑制,这与 Cdh5-NuTRAP 中对 EC 的更特异性靶向一致,而 Tie2-NuTRAP 模型也靶向造血祖细胞产生免疫细胞。事实上,虽然 TRAP 在两种模型中都富集了 EC 转录本,但在 Tie2-NuTRAP 模型中也捕获了髓样转录本,这一点通过细胞分选得到了证实。我们建议在选择靶向 EC 的 Cre 线时应考虑实验/分析因素。
