School of Biological Sciences, National Institute of Science Education and Research, HBNI, Bhubaneswar, India.
Infectious Disease Biology, Institute of Life Sciences, Bhubaneswar, India.
Front Immunol. 2019 Apr 12;10:786. doi: 10.3389/fimmu.2019.00786. eCollection 2019.
Chikungunya virus (CHIKV), a mosquito-borne Alphavirus, is endemic in different parts of the globe. The host macrophages are identified as the major cellular reservoirs of CHIKV during infection and this virus triggers robust TNF production in the host macrophages, which might be a key mediator of virus induced inflammation. However, the molecular mechanism underneath TNF induction is not understood yet. Accordingly, the Raw264.7 cells, a mouse macrophage cell line, were infected with CHIKV to address the above-mentioned question. It was observed that CHIKV induces both p38 and JNK phosphorylation in macrophages in a time-dependent manner and p-p38 inhibitor, SB203580 is effective in reducing infection even at lower concentration as compared to the p-JNK inhibitor, SP600125. However, inhibition of p-p38 and p-JNK decreased CHIKV induced TNF production in the host macrophages. Moreover, CHIKV induced macrophage derived TNF was found to facilitate TCR driven T cell activation. Additionally, it was noticed that the expressions of key transcription factors involved mainly in antiviral responses (p-IRF3) and TNF production (p-c-jun) were induced significantly in the CHIKV infected macrophages as compared to the corresponding mock cells. Further, it was demonstrated that CHIKV mediated TNF production in the macrophages is dependent on p38 and JNK MAPK pathways linking p-c-jun transcription factor. Interestingly, it was found that CHIKV nsP2 interacts with both p-p38 and p-JNK MAPKs in the macrophages. This observation was supported by the protein-protein docking analysis which illustrates the specific amino acids responsible for the nsP2-MAPKs interactions. A strong polar interaction was predicted between Thr-180 (within the phosphorylation lip) of p38 and Gln-273 of nsP2, whereas, no such polar interaction was predicted for the phosphorylation lip of JNK which indicates the differential roles of p-p38 and p-JNK during CHIKV infection in the host macrophages. In summary, for the first time it has been shown that CHIKV triggers robust TNF production in the host macrophages via both p-p38 and p-JNK/p-c-jun pathways and the interaction of viral protein, nsP2 with these MAPKs during infection. Hence, this information might shed light in rationale-based drug designing strategies toward a possible control measure of CHIKV infection in future.
基孔肯雅病毒(CHIKV)是一种虫媒黄病毒,在全球不同地区流行。宿主巨噬细胞被鉴定为 CHIKV 感染期间的主要细胞储库,该病毒在宿主巨噬细胞中引发强烈的 TNF 产生,这可能是病毒诱导炎症的关键介质。然而,诱导 TNF 产生的分子机制尚不清楚。因此,用 CHIKV 感染 Raw264.7 细胞(一种小鼠巨噬细胞系)来解决上述问题。结果观察到,CHIKV 以时间依赖性方式诱导巨噬细胞中 p38 和 JNK 的磷酸化,并且 p38 抑制剂 SB203580 比 JNK 抑制剂 SP600125 更有效,即使在较低浓度下也能抑制感染。然而,抑制 p38 和 JNK 降低了宿主巨噬细胞中 CHIKV 诱导的 TNF 产生。此外,发现 CHIKV 诱导的巨噬细胞衍生的 TNF 有利于 TCR 驱动的 T 细胞激活。此外,注意到与相应的 mock 细胞相比,CHIKV 感染的巨噬细胞中主要涉及抗病毒反应(p-IRF3)和 TNF 产生(p-c-jun)的关键转录因子的表达明显诱导。此外,证明 CHIKV 介导的巨噬细胞中的 TNF 产生依赖于 p38 和 JNK MAPK 途径,该途径连接 p-c-jun 转录因子。有趣的是,发现 CHIKV nsP2 与巨噬细胞中的 p-p38 和 p-JNK MAPKs 相互作用。蛋白质-蛋白质对接分析支持了这一观察结果,该分析说明了 nsP2-MAPKs 相互作用的特定氨基酸。预测 Thr-180(磷酸化唇内)与 nsP2 的 Gln-273 之间存在强烈的极性相互作用,而 JNK 的磷酸化唇内则没有预测到这种极性相互作用,这表明 p-p38 和 p-JNK 在 CHIKV 感染宿主巨噬细胞中的作用不同。总之,这是首次表明 CHIKV 通过 p-p38 和 p-JNK/p-c-jun 途径以及病毒蛋白 nsP2 与这些 MAPKs 在感染过程中的相互作用在宿主巨噬细胞中引发强烈的 TNF 产生。因此,这些信息可能为基于合理药物设计策略提供信息,以在未来控制 CHIKV 感染。
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