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内皮炎症:N-脱乙酰酶/N-磺基转移酶差异表达在硫酸乙酰肝素免疫特性改变中的作用

Endothelial inflammation: the role of differential expression of N-deacetylase/N-sulphotransferase enzymes in alteration of the immunological properties of heparan sulphate.

作者信息

Carter Noel M, Ali Simi, Kirby John A

机构信息

Institute of Pharmacy, Chemistry and Biomedical Science, University of Sunderland, Sunderland SR1 3SD, UK.

出版信息

J Cell Sci. 2003 Sep 1;116(Pt 17):3591-600. doi: 10.1242/jcs.00662. Epub 2003 Jul 22.

DOI:10.1242/jcs.00662
PMID:12876215
Abstract

Heparan sulphate N-deacetylase/N-sulphotransferase (NDST) enzymes catalyse the reaction that initiates sulphation and subsequent modification of the oligosaccharide, heparan sulphate (HS). The extent and distribution of sulphate substitution on HS plays a vital role in regulation of the binding of a range of proteins, including IFN-gamma, several interleukins and most chemokines. In this study, the expression of NDST transcripts was found to be non-uniform between a range of cell types, suggesting that different cells produce characteristic HS species. It was found that stimulation of the HMEC-1 microvascular endothelial cell line with the pro-inflammatory cytokines IFN-gamma and TNF-alpha caused a transient decrease in the level of NDST-1 and -2 transcripts after 4 hours (P < 0.05 and P < 0.01 respectively), but the expression of NDST-1 increased above control levels after 16 hours (P < 0.01). The change in NDST expression was concurrent with an increase in the abundance of sulphated HS epitopes on the cell surface; this was not caused by variation in the expression of proteoglycans or by changes in the rate of GAG turnover. Cytokine-stimulated endothelial cells also showed an increase in their potential to bind RANTES (CCL5); this was abrogated by chlorate blockade of sulphotransferase activity or by heparitinase cleavage of cell surface HS. Monolayers of cytokine-stimulated HMEC-1 also supported an enhanced leukocyte chemotactic response towards RANTES. This study demonstrated that pro-inflammatory cytokines can increase NDST expression leading to increased sulphation of HS and a corresponding increase in sequestration of functional RANTES at the apical surface of endothelial cells. This may enhance leukocyte extravasation at sites of inflammation.

摘要

硫酸乙酰肝素N - 脱乙酰酶/N - 硫酸转移酶(NDST)催化启动硫酸化反应及随后对硫酸乙酰肝素(HS)寡糖进行修饰的过程。HS上硫酸取代的程度和分布在一系列蛋白质(包括干扰素 - γ、多种白细胞介素和大多数趋化因子)的结合调节中起着至关重要的作用。在本研究中,发现NDST转录本在一系列细胞类型中的表达并不均匀,这表明不同细胞产生具有特征性的HS种类。研究发现,用促炎细胞因子干扰素 - γ和肿瘤坏死因子 - α刺激HMEC - 1微血管内皮细胞系4小时后,NDST - 1和 - 2转录本水平短暂下降(分别为P < 0.05和P < 0.01),但16小时后NDST - 1的表达高于对照水平(P < 0.01)。NDST表达的变化与细胞表面硫酸化HS表位丰度的增加同时发生;这不是由蛋白聚糖表达的变化或糖胺聚糖周转率的改变引起的。细胞因子刺激的内皮细胞结合RANTES(CCL5)的能力也有所增加;通过氯酸盐阻断硫酸转移酶活性或通过肝素酶切割细胞表面HS可消除这种增加。细胞因子刺激的HMEC - 1单层细胞对RANTES的白细胞趋化反应也增强。本研究表明,促炎细胞因子可增加NDST表达,导致HS硫酸化增加以及在内皮细胞顶端表面功能性RANTES的隔离相应增加。这可能会增强炎症部位的白细胞外渗。

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