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TC-PTP 调节小鼠早期 T 细胞发育过程中的 IL-7 转录反应。

TC-PTP regulates the IL-7 transcriptional response during murine early T cell development.

机构信息

Rosalind and Morris Goodman Cancer Centre, McGill University, Montréal, QC H3A 1A3, Canada.

Division of Experimental Medicine, Department of Medicine, McGill University, Montréal, QC H3A 1A3, Canada.

出版信息

Sci Rep. 2017 Oct 16;7(1):13275. doi: 10.1038/s41598-017-13673-w.

Abstract

Cytokines play a critical role in directing the discrete and gradual transcriptional changes that define T cell development. The interleukin-7 receptor (IL-7R), via its activation of the JAK-STAT pathway, promotes gene programs that change dynamically as cells progress through T cell differentiation. The molecular mechanism(s) directing differential gene expression downstream of the IL-7R are not fully elucidated. Here, we have identified T cell protein tyrosine phosphatase (TC-PTP), also known as PTPN2, as a negative regulator of IL-7R-STAT signaling in T cell progenitors, contributing to both the quantitative and qualitative nature of STAT-gene targeting. Novel genetic strategies used to modulate TC-PTP expression demonstrate that depletion of TC-PTP expression heightens the phosphorylation of STAT family members, causing aberrant expression of an interferon-response gene profile. Such molecular re-programming results in deregulation of early development checkpoints culminating in inefficient differentiation of CD4CD8 double positive cells. TC-PTP is therefore shown to be required to safeguard the dynamic transcriptome necessary for efficient T cell differentiation.

摘要

细胞因子在指导 T 细胞发育过程中离散和逐步的转录变化中起着关键作用。白细胞介素-7 受体(IL-7R)通过其激活 JAK-STAT 途径,促进细胞在 T 细胞分化过程中动态变化的基因程序。指导 IL-7R 下游差异基因表达的分子机制尚未完全阐明。在这里,我们已经确定 T 细胞蛋白酪氨酸磷酸酶(TC-PTP),也称为 PTPN2,作为 T 细胞祖细胞中 IL-7R-STAT 信号的负调节剂,有助于 STAT 基因靶向的数量和质量性质。用于调节 TC-PTP 表达的新型遗传策略表明,TC-PTP 表达的耗竭会增加 STAT 家族成员的磷酸化,导致干扰素反应基因谱的异常表达。这种分子重编程导致早期发育检查点的失调,最终导致 CD4CD8 双阳性细胞的分化效率降低。因此,TC-PTP 被证明是为了保护高效 T 细胞分化所需的动态转录组所必需的。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/da59/5643372/d7561013c0d6/41598_2017_13673_Fig1_HTML.jpg

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