Department of Dermatology, University Hospital Zurich, Gloriastrasse 31, F floor, Zurich, 8091, Switzerland.
Department of Biology, Institute for Molecular Health Sciences, ETH Zürich, Otto-Stern-Weg 7, Zurich, 8093, Switzerland.
Cell Death Dis. 2018 Jan 18;9(2):24. doi: 10.1038/s41419-017-0009-4.
Inflammasomes are multimeric protein complexes that assemble upon sensing of a variety of stress factors. Their formation results in caspase-1-mediated activation and secretion of the pro-inflammatory cytokines pro-interleukin(IL)-1β and -18, which induce an inflammatory response. Inflammation is supported by a lytic form of cell death, termed pyroptosis. Innate immune cells, such as macrophages or dendritic cells, express and activate inflammasomes. However, it has also been demonstrated that human primary keratinocytes activate different types of inflammasomes in vitro, for example, upon UVB irradiation or viral infection. Keratinocytes are the main cell type of the epidermis, the outermost layer of the body, and form a protective barrier consisting of a stratified multi-layered epithelium. In human, gain-of-function mutations of the NLRP1 gene cause syndromes mediated by inflammasome activation in keratinocytes that are characterised by skin inflammation and skin cancer susceptibility. Here we demonstrate that murine keratinocytes do not activate inflammasomes in response to stimuli, which induce IL-1β and -18 secretion by human keratinocytes. Whereas murine keratinocytes produced caspase-1 and proIL-18, expression of the inflammasome proteins Nlrp1, Nlrp3, Aim2, Asc, and proIL-1β was, compared to human keratinocytes or murine dendritic cells, very low or even undetectable. Priming of murine keratinocytes with cytokines commonly used for induction of proIL-1β and inflammasome protein expression did not rescue inflammasome activation. Nevertheless, UVB-induced inflammation and neutrophil recruitment in murine skin was dependent on IL-1β and caspase-1. However, also under these conditions, we did not detect expression of proIL-1β by keratinocytes in murine skin, but by immune cells. These results demonstrate a higher immunological competence of human compared to murine keratinocytes, which is reflected by stress-induced IL-1β secretion that is mediated by inflammasomes. Therefore, keratinocytes in human skin can exert immune functions, which are carried out by professional immune cells in murine skin.
炎症小体是一种多聚体蛋白复合物,在感知多种应激因子时会组装。它们的形成导致半胱天冬酶-1 介导的前炎症细胞因子白细胞介素(IL)-1β 和 -18 的激活和分泌,从而引发炎症反应。炎症由一种称为细胞焦亡的裂解形式的细胞死亡支持。先天免疫细胞,如巨噬细胞或树突状细胞,表达和激活炎症小体。然而,已经证明人原代角质形成细胞在体外也可以激活不同类型的炎症小体,例如,在 UVB 照射或病毒感染时。角质形成细胞是表皮(身体最外层)的主要细胞类型,形成由分层的多层上皮组成的保护性屏障。在人类中,NLRP1 基因的获得功能突变导致炎症小体激活介导的综合征,其特征是皮肤炎症和皮肤癌易感性。在这里,我们证明了小鼠角质形成细胞不会对诱导人角质形成细胞产生 IL-1β 和 -18 分泌的刺激物激活炎症小体。虽然小鼠角质形成细胞产生了半胱天冬酶-1 和前 IL-18,但与人类角质形成细胞或小鼠树突状细胞相比,炎症小体蛋白 NLRP1、NLRP3、Aim2、Asc 和前 IL-1β 的表达非常低甚至无法检测到。用通常用于诱导前 IL-1β 和炎症小体蛋白表达的细胞因子对小鼠角质形成细胞进行预处理并不能挽救炎症小体的激活。然而,UVB 诱导的小鼠皮肤炎症和中性粒细胞募集依赖于 IL-1β 和半胱天冬酶-1。然而,即使在这些条件下,我们也没有在小鼠皮肤的角质形成细胞中检测到前 IL-1β 的表达,而是在免疫细胞中检测到。这些结果表明,与人相比,小鼠角质形成细胞具有更高的免疫能力,这反映在应激诱导的 IL-1β 分泌上,该分泌由炎症小体介导。因此,人类皮肤中的角质形成细胞可以发挥免疫功能,而这些功能是由小鼠皮肤中的专业免疫细胞执行的。
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