Comparison of HTLV-I basal transcription and expression of CREB/ATF-1/CREM family members in peripheral blood mononuclear cells and Jurkat T cells.

G C Newbound, J P O'Rourke, N D Collins, J DeWille, M D Lairmore
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引用次数: 9

Abstract

HTLV-I is the etiologic agent of adult T-cell leukemia/lymphoma and is associated with tropical spastic paraparesis/HTLV-I-associated myelopathy. Following integration into the host cell genome, HTLV-I replication is regulated by both host and viral mechanisms that control transcription. Low levels of viral transcription (basal transcription) occur before expression of the virally encoded Tax protein (Tax-mediated transcription). Members of the cyclic adenosine monophosphate (cAMP) response element binding (CREB)/activating transcription factor 1 (ATF-1) family of transcription factors bind three 21-bp repeats (Tax-responsive element-1, or TRE-1) within the viral promoter and are important for basal and Tax-mediated transcription. Using mitogen stimulated and quiescent peripheral blood mononuclear cells (PBMC) and Jurkat cells, we compared differences in basal transcription and amounts and binding of transcription factors with TRE-1. We demonstrate that amounts of transcriptionally active phosphorylated CREB protein (P-CREB) differ between activated PBMC and Jurkat cells. Following stimulation, P-CREB levels remain elevated in PBMC for up to 24 hours whereas CREB is dephosphorylated in Jurkat cells within 4 hours following stimulation. The differences in P-CREB levels between PBMC and Jurkat cells were directly correlated with basal transcription of HTLV-I in the two cell types. Using electrophoretic mobility shift assays, we determined that the pattern of band migration differed between the two cell types. These data demonstrate that PBMC differentially regulate basal HTLV-I transcription compared with Jurkat T cells, and this differential regulation is due, in part to differential phosphorylation and binding of CREB/ATF-1 to TRE-1 in the HTLV-I promoter. We demonstrate the utility of using primary lymphocyte models to study HTLV-I transcription in the context of cell signaling and suggest that activated PBMC maintain elevated levels of P-CREB, which promote basal HTLV-I transcription and enhance viral persistence in vivo.

外周血单个核细胞与Jurkat T细胞HTLV-I基础转录及CREB/ATF-1/CREM家族成员表达的比较
htlv - 1是成人t细胞白血病/淋巴瘤的病因,并与热带痉挛性麻痹/ htlv - 1相关的脊髓病有关。在整合到宿主细胞基因组后,HTLV-I的复制受到宿主和病毒控制转录机制的调节。低水平的病毒转录(基础转录)发生在病毒编码的税收蛋白(税收介导转录)表达之前。环腺苷单磷酸(cAMP)反应元件结合(CREB)/激活转录因子1 (ATF-1)家族的成员在病毒启动子中结合3个21 bp重复序列(Tax-responsive element-1,或tre1),对基础转录和税收介导的转录很重要。利用丝裂原刺激和静止的外周血单核细胞(PBMC)和Jurkat细胞,我们比较了基础转录、转录因子与tre1结合的数量和数量的差异。我们证明了转录活性磷酸化CREB蛋白(P-CREB)的数量在活化的PBMC和Jurkat细胞之间存在差异。刺激后,PBMC中的P-CREB水平在24小时内保持升高,而Jurkat细胞中的CREB在刺激后4小时内被去磷酸化。PBMC和Jurkat细胞之间P-CREB水平的差异与两种细胞类型中HTLV-I的基础转录直接相关。利用电泳迁移率转移测定,我们确定了两种细胞类型之间的带迁移模式不同。这些数据表明,与Jurkat T细胞相比,PBMC对HTLV-I基础转录的调节存在差异,这种差异调节部分是由于HTLV-I启动子中CREB/ATF-1与tre1的磷酸化和结合存在差异。我们证明了使用原代淋巴细胞模型在细胞信号传导背景下研究HTLV-I转录的实用性,并表明激活的PBMC维持高水平的P-CREB,从而促进HTLV-I的基础转录并增强病毒在体内的持久性。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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