hnRNP A1-丝氨酸 199 的磷酸化不是 T 细胞分化和功能所必需的。

Q3 Medicine ImmunoHorizons Pub Date : 2024-02-01 DOI:10.4049/immunohorizons.2300074
Tristan L A White, Ye Jin, Sean D A Roberts, Matthew J Gable, Penelope A Morel
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引用次数: 0

摘要

hnRNP A1 是一种重要的 RNA 结合蛋白,它影响 RNA 处理的许多阶段,包括转录、替代剪接、mRNA 核输出和 RNA 稳定性。然而,hnRNP A1 在免疫细胞(尤其是 CD4+ T 细胞)中的作用仍不清楚。我们以前的研究表明,hnRNP A1 的 Akt 磷酸化依赖于 TCR 信号强度,并与 Treg 分化有关。为了探索 Akt 磷酸化 hnRNP A1 对 CD4+ T 细胞分化的影响,我们实验室利用 CRISPR Cas9 技术生成了一个突变小鼠模型 hnRNP A1-S199A(A1-MUT),其中 hnRNP A1 上的主要 Akt 磷酸化位点被突变为丙氨酸。A1-MUT小鼠的免疫图谱显示肠系膜淋巴结中Tregs的数量发生了变化。我们发现,在体外,幼稚 CD4+ T 细胞向 Th1、Th2、Th17 或 T 调节细胞(Tregs)分化方面没有明显差异。在体内,使用暴露于 OVA 食物的 OTII-A1 突变 CD4+ T 细胞进行的 Treg 分化试验显示,A1-MUT 存在迁移和归巢缺陷,但在 Treg 诱导方面没有变化。用 NP- 锁孔帽状血蓝蛋白免疫 A1-MUT 小鼠,观察到生殖中心发育正常,NP 特异性 B 细胞数量正常,Tfh 数量无变化。总之,在测试的模型中,hnRNP A1 S199 的 Akt 磷酸化对 CD4+ T 细胞的命运或功能不起作用。这种 hnRNP A1-S199A 小鼠模型应该是研究 hnRNP A1-S199 的 Akt 磷酸化在不同细胞类型或其他人类疾病小鼠模型中的作用的重要工具。
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Phosphorylation of hnRNP A1-Serine 199 Is Not Required for T Cell Differentiation and Function.

hnRNP A1 is an important RNA-binding protein that influences many stages of RNA processing, including transcription, alternative splicing, mRNA nuclear export, and RNA stability. However, the role of hnRNP A1 in immune cells, specifically CD4+ T cells, remains unclear. We previously showed that Akt phosphorylation of hnRNP A1 was dependent on TCR signal strength and was associated with Treg differentiation. To explore the impact of hnRNP A1 phosphorylation by Akt on CD4+ T cell differentiation, our laboratory generated a mutant mouse model, hnRNP A1-S199A (A1-MUT) in which the major Akt phosphorylation site on hnRNP A1 was mutated to alanine using CRISPR Cas9 technology. Immune profiling of A1-MUT mice revealed changes in the numbers of Tregs in the mesenteric lymph node. We found no significant differences in naive CD4+ T cell differentiation into Th1, Th2, Th17, or T regulatory cells (Tregs) in vitro. In vivo, Treg differentiation assays using OTII-A1-Mut CD4+ T cells exposed to OVA food revealed migration and homing defects in the A1-MUT but no change in Treg induction. A1-MUT mice were immunized with NP- keyhole limpet hemocyanin, and normal germinal center development, normal numbers of NP-specific B cells, and no change in Tfh numbers were observed. In conclusion, Akt phosphorylation of hnRNP A1 S199 does not play a role in CD4+ T cell fate or function in the models tested. This hnRNP A1-S199A mouse model should be a valuable tool to study the role of Akt phosphorylation of hnRNP A1-S199 in different cell types or other mouse models of human disease.

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