肺损伤中鞘氨醇激酶1和2的差异调节
Differential regulation of sphingosine kinases 1 and 2 in lung injury.
作者信息
Wadgaonkar Raj, Patel Vipul, Grinkina Natalia, Romano Carol, Liu Jing, Zhao Yutong, Sammani Saad, Garcia Joe G N, Natarajan Viswanathan
机构信息
Department of Medicine, SUNY Downstate Medical Center, Brooklyn, NY 11203, USA.
出版信息
Am J Physiol Lung Cell Mol Physiol. 2009 Apr;296(4):L603-13. doi: 10.1152/ajplung.90357.2008. Epub 2009 Jan 23.
Two mammalian sphingosine kinase (SphK) isoforms, SphK1 and SphK2, possess identical kinase domains but have distinct kinetic properties and subcellular localizations, suggesting each has one or more specific roles in sphingosine-1-phosphate (S1P) generation. Although both kinases use sphingosine as a substrate to generate S1P, the mechanisms controlling SphK activation and subsequent S1P generation during lung injury are not fully understood. In this study, we established a murine lung injury model to investigate LPS-induced lung injury in SphK1 knockout (SphK1(-/-)) and wild-type (WT) mice. We found that SphK1(-/-) mice were much more susceptible to LPS-induced lung injury compared with their WT counterparts, quantified by multiple parameters including cytokine induction. Intriguingly, overexpression of WT SphK1 delivered by adenoviral vector to the lungs protected SphK1(-/-) mice from lung injury and attenuated the severity of the response to LPS. However, adenoviral overexpression of a SphK1 kinase-dead mutant (SphKKD) in SphK1(-/-) mouse lungs further exacerbated the response to LPS as well as the extent of lung injury. WT SphK2 adenoviral overexpression also failed to provide protection and, in fact, augmented the degree of LPS-induced lung injury. This suggested that, in vascular injury, S1P generated by SphK2 activation plays a distinctly separate role compared with SphK1-dependent S1P generation and survival signaling. Microarray and real-time RT-PCR analysis of SphK1 and SphK2 expression levels during lung injury revealed that, in WT mice, LPS treatment caused significantly enhanced SphK1 expression ( approximately 5x) levels within 6 h, which declined back to baseline levels by 24 h posttreatment. In contrast, expression of SphK2 was gradually induced following LPS treatment and was elevated within 24 h. Collectively, our results for the first time demonstrate distinct functional roles of the two SphK isoforms in the regulation of LPS-induced lung injury.
两种哺乳动物鞘氨醇激酶(SphK)亚型,即SphK1和SphK2,具有相同的激酶结构域,但动力学特性和亚细胞定位不同,这表明它们在鞘氨醇-1-磷酸(S1P)生成过程中各自具有一个或多个特定作用。尽管两种激酶都利用鞘氨醇作为底物来生成S1P,但在肺损伤期间控制SphK激活及随后S1P生成的机制尚未完全明了。在本研究中,我们建立了小鼠肺损伤模型,以研究脂多糖(LPS)诱导的SphK1基因敲除(SphK1(-/-))小鼠和野生型(WT)小鼠的肺损伤。我们发现,与野生型小鼠相比,SphK1(-/-)小鼠对LPS诱导的肺损伤更为敏感,这通过包括细胞因子诱导在内的多个参数得以量化。有趣的是,通过腺病毒载体将野生型SphK1导入肺中进行过表达,可保护SphK1(-/-)小鼠免受肺损伤,并减轻对LPS反应的严重程度。然而,在SphK1(-/-)小鼠肺中腺病毒过表达SphK1激酶失活突变体(SphKKD),进一步加剧了对LPS的反应以及肺损伤程度。野生型SphK2的腺病毒过表达也未能提供保护,实际上还增强了LPS诱导的肺损伤程度。这表明,在血管损伤中,与SphK1依赖性S1P生成和存活信号传导相比,SphK2激活所产生的S1P发挥着明显不同的作用。对肺损伤期间SphK1和SphK2表达水平进行的微阵列和实时逆转录-聚合酶链反应(RT-PCR)分析显示,在野生型小鼠中,LPS处理在6小时内导致SphK1表达水平显著增强(约5倍),在处理后24小时降至基线水平。相反,SphK2的表达在LPS处理后逐渐诱导,并在24小时内升高。总体而言,我们的结果首次证明了两种SphK亚型在调节LPS诱导的肺损伤中具有不同的功能作用。
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