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拟杆菌属水相苯酚提取脂多糖复合物诱导肿瘤坏死因子

Tumor necrosis factor induction by an aqueous phenol-extracted lipopolysaccharide complex from Bacteroides species.

作者信息

Delahooke D M, Barclay G R, Poxton I R

机构信息

Department of Medical Microbiology, University of Edinburgh Medical School, Scotland.

出版信息

Infect Immun. 1995 Mar;63(3):840-6. doi: 10.1128/iai.63.3.840-846.1995.

Abstract

The stimulation of macrophages and monocytes by lipopolysaccharide (LPS) results in the secretion of tumor necrosis factor (TNF), a cytokine which is thought to play a pivotal role in subsequent host responses. Its induction is thought to be facilitated by the binding of complexes of LPS and LPS-binding protein to CD14. The LPS of Bacteroides species was considered a weak endotoxin; however, in a recent study we have shown that the biological activity and chemical composition of the LPS from Bacteroides species are dependent on the extraction method. The present study determines the capacity of LPS extracted by aqueous phenol (the method for producing an LPS of high endotoxic activity) from four species of Bacteroides to induce TNF. Induction was investigated from human mononuclear leukocytes (MNL), THP-1 cells (with and without enhancement by vitamin D2 for CD14), and peritoneal macrophages from C3H/HeJ (LPS nonresponder) and C3H/HeN (LPS responder) mice. Escherichia coli O18K- LPS, a typical smooth LPS of heterogeneous molecular mass, was used as a control throughout. The stimulation of TNF production by E. coli LPS was between two- and fourfold more than that by Bacteroides LPS in MNL, in THP-1 cells (with enhancement for CD14), and in peritoneal macrophages from C3H/HeN mice. In THP-1 cells (without enhancement for CD14), there was no significant difference in TNF production between E. coli and Bacteroides LPSs. In peritoneal macrophages from C3H/HeJ mice, E. coli LPS stimulated no TNF production, but there was no significant difference in TNF production from peritoneal macrophages from C3H/HeJ and C3H/HeN mice by Bacteroides LPS. In all cell populations, there was a peak of TNF production after approximately 4 h of stimulation with all LPSs tested. However, other peaks of TNF production were seen in MNL and THP-1 cells (with enhancement for CD14) after stimulation with E. coli LPS only. In stimulation assays in which Bacteroides LPS was together with but in excess of E. coli LPS, it was found that TNF production from MNL and THP-1 cells (with and without enhancement for CD14) was comparable to that of Bacteroides LPS alone and not E. coli LPS alone. An anti-CD14 monoclonal antibody did not inhibit Bacteroides LPS-stimulated TNF production. However, E. coli LPS-stimulated TNF release was inhibited by an anti-CD14 monoclonal antibody, most noticeably in MNL and THP-1 cells (with enhancement for CD14).(ABSTRACT TRUNCATED AT 400 WORDS)

摘要

脂多糖(LPS)对巨噬细胞和单核细胞的刺激会导致肿瘤坏死因子(TNF)的分泌,TNF是一种细胞因子,被认为在随后的宿主反应中起关键作用。人们认为LPS与LPS结合蛋白的复合物与CD14的结合促进了TNF的诱导。拟杆菌属的LPS曾被认为是一种弱内毒素;然而,在最近的一项研究中我们发现,拟杆菌属LPS的生物学活性和化学组成取决于提取方法。本研究测定了用酚水法(一种产生高内毒素活性LPS的方法)从四种拟杆菌中提取的LPS诱导TNF的能力。我们从人单核白细胞(MNL)、THP-1细胞(添加和不添加维生素D2增强CD14)以及C3H/HeJ(LPS无反应者)和C3H/HeN(LPS反应者)小鼠的腹腔巨噬细胞中研究了TNF的诱导情况。在整个实验中,均使用大肠杆菌O18K-LPS作为对照,它是一种典型的具有异质分子量的光滑LPS。在MNL、THP-1细胞(添加CD14增强剂)以及C3H/HeN小鼠的腹腔巨噬细胞中,大肠杆菌LPS对TNF产生的刺激作用比拟杆菌属LPS强2至4倍。在THP-1细胞(不添加CD14增强剂)中,大肠杆菌LPS和拟杆菌属LPS在TNF产生方面没有显著差异。在C3H/HeJ小鼠的腹腔巨噬细胞中,大肠杆菌LPS未刺激TNF产生,但拟杆菌属LPS刺激C3H/HeJ和C3H/HeN小鼠腹腔巨噬细胞产生的TNF没有显著差异。在所有测试的细胞群体中,用所有LPS刺激约4小时后,TNF产生均出现峰值。然而,仅用大肠杆菌LPS刺激后,在MNL和THP-1细胞(添加CD14增强剂)中还出现了其他TNF产生峰值。在用拟杆菌属LPS与过量大肠杆菌LPS共同进行的刺激试验中,发现MNL和THP-1细胞(添加和不添加CD14增强剂)产生的TNF与单独使用拟杆菌属LPS时相当,而与单独使用大肠杆菌LPS时不同。抗CD14单克隆抗体不抑制拟杆菌属LPS刺激的TNF产生。然而,抗CD14单克隆抗体抑制大肠杆菌LPS刺激的TNF释放,在MNL和THP-1细胞(添加CD14增强剂)中最为明显。(摘要截选至400字)

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