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Expression of tumour necrosis factor receptor and Toll-like receptor 2 and 4 on peripheral blood leucocytes of human volunteers after endotoxin challenge: a comparison of flow cytometric light scatter and immunofluorescence gating

机译:内毒素攻击后人类志愿者外周血白细胞上肿瘤坏死因子受体和Toll样受体2和4的表达:流式细胞仪光散射和免疫荧光门控的比较

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摘要

Toll-like receptors (TLRs) are involved in the recognition of bacterial products and thus participate in the induction of the inflammatory cascade. However, much less is known about the evolution of leucocyte TLR expression during human inflammatory stress. We hypothesized that a decrease in leucocyte TLRs could account for the so-called tolerance or hyporesponsiveness state to subsequent stimulation with bacteria-derived products. Because of the profound monocytopenia that ensues after in vivo lipopolysaccharide (LPS) challenge, we also compared monocyte TLR expression using two different techniques of flow cytometric gating. In a first set of experiments, 17 healthy volunteers underwent LPS challenge. Blood was drawn at different time-points and analysed by flow cytometry using light scatter gating and one-colour analysis to assess the expression of the tumour necrosis factor receptor (TNFR) and TLR2 and TLR4 on both monocytes and granulocytes. In a second set of experiments, the assessment of those receptors was made using a more specific gating method that utilized light scatter and CD14 immunofluorescence in a two-colour analysis. This was performed using whole blood drawn from five healthy volunteers and incubated ex vivo for different time periods with or without LPS and in 12 volunteers who underwent LPS challenge in vivo. The pattern of expression for monocyte TNFR was similar for both types of gating. Using only the light scatter gating, an initial drop of TLR 2 and 4 was observed on monocytes. By contrast, when using light scatter × immunofluorescence gating, an up-regulation of these two receptors following both in vivo and in vitro LPS exposure was observed. LPS up-regulates the expression of TLRs on monocytes and granulocytes. Depending upon the methodology utilized, contrasting results were obtained with respect to TLR2 and TLR4 expression. The flow cytometric gating technique used is of importance in determining cellular TLR2 and TLR4 expression, especially in blood samples exhibiting significant monocytopenia.
机译:Toll样受体(TLR)参与细菌产物的识别,因此参与了炎症级联反应的诱导。然而,关于人类炎性应激期间白细胞TLR表达的进化知之甚少。我们假设白细胞TLR的减少可以解释所谓的耐受性或低反应性状态,这种状态是随后对细菌衍生产物的刺激。由于体内脂多糖(LPS)攻击后会发生深层的单核细胞减少症,因此我们还使用两种不同的流式细胞术门控技术比较了单核细胞TLR表达。在第一组实验中,有17名健康志愿者接受了LPS挑战。在不同的时间点抽取血液,并使用光散射门控和单色分析通过流式细胞术进行分析,以评估肿瘤坏死因子受体(TNFR)以及TLR2和TLR4在单核细胞和粒细胞上的表达。在第二组实验中,使用更特定的门控方法对这些受体进行了评估,该方法在两种颜色的分析中利用了光散射和CD14免疫荧光。这是使用从五名健康志愿者那里抽取的全血进行的,并在有或没有LPS的情况下在不同时间段进行离体温育,并在12位接受LPS体内挑战的志愿者中进行。两种门控类型的单核细胞TNFR表达模式均相似。仅使用光散射门控,在单核细胞上观察到了TLR 2和4的初始下降。相比之下,当使用光散射x免疫荧光门控时,在体内和体外LPS暴露后都观察到这两个受体的上调。 LPS上调单核细胞和粒细胞上TLR的表达。根据所使用的方法,就TLR2和TLR4表达获得了相反的结果。所用的流式细胞术门控技术对确定细胞TLR2和TLR4的表达非常重要,特别是在血液样本中表现出明显的单核细胞减少症。

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