Alternative splicing of FKBP5 gene exerts control over T lymphocyte expansion.

IF 3 3区 生物学 Q3 BIOCHEMISTRY & MOLECULAR BIOLOGY Journal of cellular biochemistry Pub Date : 2024-12-01 Epub Date: 2023-01-16 DOI:10.1002/jcb.30364
Laura Marrone, Massimo D'Agostino, Elena Cesaro, Valeria di Giacomo, Simona Urzini, Maria Fiammetta Romano, Simona Romano
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Abstract

FKBP51 is constitutively expressed by immune cells. As other FKBP family members, FKBP51 acts as a coreceptor for the natural products FK506 and rapamycin, which exhibit immunosuppressive effects. However, little is known about the intrinsic role of this large FKBP in the primary function of lymphocytes, that is, the adaptive immune response against foreign antigens, for example, pathogens. This paper aimed to investigate whether FKBP51 expression was modulated during lymphocyte activation. Moreover, as we recently identified a splicing isoform of FKBP51, namely FKBP51s, we also measured this splice protein, along with the canonical one, at different times of a peripheral blood mononuclear cell culture stimulated via T cell receptor. Our results show that the two FKBP51 isoforms were alternatively induced during the proliferative burst. Canonical FKBP51 increased in the time window between 48 and 96 h and its expression levels correlated with cyclin D levels. FKBP51s transiently increased earlier, at 24-36 h to reappearing later, at 120 h, when cyclin D expression returned at resting levels and proliferation ceased. Interestingly, within these two specific timeframes, FKBP51s accumulated in the nucleus. Here FKBP51s colocalized with the Foxp3 transcription factor at 36 h. Regulatory T cell (Treg) counts significantly decreased when FKBP51s was downmodulated. The coculture suppression assay suggested that FKBP51s supports the suppressive capability of Tregs. At 120 h, chromatin immunoprecipitation experiments found FKBP51s linked to CCND1 gene, suggesting a possible effect on gene transcription regulation, as previously demonstrated in melanoma. In conclusion, our study shows that FKBP5 isoforms are upregulated during lymphocyte activation, albeit on different timeframes. The activation of canonical FKBP51 coincides with proliferation hallmarks; FKBP5 splicing occurs early to sustain Treg development and late when proliferation ceases.

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FKBP5 基因的交替剪接控制着 T 淋巴细胞的扩增。
FKBP51 由免疫细胞组成表达。与 FKBP 家族的其他成员一样,FKBP51 也是天然产物 FK506 和雷帕霉素的核心受体,具有免疫抑制作用。然而,人们对这种大型 FKBP 在淋巴细胞主要功能(即对外来抗原(如病原体)的适应性免疫反应)中的内在作用知之甚少。本文旨在研究 FKBP51 的表达在淋巴细胞活化过程中是否受到调节。此外,由于我们最近发现了 FKBP51 的一种剪接异构体,即 FKBP51s,因此我们还测量了这种剪接蛋白和标准蛋白在通过 T 细胞受体刺激的外周血单核细胞培养的不同时期的表达情况。我们的结果表明,在增殖爆发过程中,两种 FKBP51 异构体被交替诱导。典型的 FKBP51 在 48 至 96 h 的时间窗口内增加,其表达水平与细胞周期蛋白 D 的水平相关。FKBP51s 在较早的 24-36 小时内短暂增加,在较晚的 120 小时内再次出现,此时细胞周期蛋白 D 的表达恢复到静息水平,增殖停止。有趣的是,在这两个特定的时间段内,FKBP51s在细胞核中积累。在 36 小时时,FKBP51s 与 Foxp3 转录因子共定位。当 FKBP51s 下调时,调节性 T 细胞(Treg)数量明显减少。共培养抑制试验表明,FKBP51s支持Tregs的抑制能力。在 120 h 染色质免疫沉淀实验中发现 FKBP51s 与 CCND1 基因相连,这表明 FKBP51s 可能对基因转录调控有影响,这与之前在黑色素瘤中的研究结果一致。总之,我们的研究表明,FKBP5同工酶在淋巴细胞活化过程中上调,尽管上调的时间框架不同。典型 FKBP51 的激活与增殖标志相吻合;FKBP5 的剪接发生在早期,以维持 Treg 的发育,而在增殖停止时则发生在晚期。
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来源期刊
Journal of cellular biochemistry
Journal of cellular biochemistry 生物-生化与分子生物学
CiteScore
9.90
自引率
0.00%
发文量
164
审稿时长
1 months
期刊介绍: The Journal of Cellular Biochemistry publishes descriptions of original research in which complex cellular, pathogenic, clinical, or animal model systems are studied by biochemical, molecular, genetic, epigenetic or quantitative ultrastructural approaches. Submission of papers reporting genomic, proteomic, bioinformatics and systems biology approaches to identify and characterize parameters of biological control in a cellular context are encouraged. The areas covered include, but are not restricted to, conditions, agents, regulatory networks, or differentiation states that influence structure, cell cycle & growth control, structure-function relationships.
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