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膜结合型和可溶性树突状细胞特异性细胞间黏附分子3抓取非整合素1(DC-SIGN1)和DC-SIGN2亚型的丰富 repertoire。DC-SIGN转录本表达的个体间差异。

Extensive repertoire of membrane-bound and soluble dendritic cell-specific ICAM-3-grabbing nonintegrin 1 (DC-SIGN1) and DC-SIGN2 isoforms. Inter-individual variation in expression of DC-SIGN transcripts.

作者信息

Mummidi S, Catano G, Lam L, Hoefle A, Telles V, Begum K, Jimenez F, Ahuja S S, Ahuja S K

机构信息

South Texas Veterans Health Care System, Audie L. Murphy Division, San Antonio, Texas 78229-4404, USA.

出版信息

J Biol Chem. 2001 Aug 31;276(35):33196-212. doi: 10.1074/jbc.M009807200. Epub 2001 May 3.

Abstract

Expression in dendritic cells (DCs) of DC-SIGN, a type II membrane protein with a C-type lectin ectodomain, is thought to play an important role in establishing the initial contact between DCs and resting T cells. DC-SIGN is also a unique type of human immunodeficiency virus-1 (HIV-1) attachment factor and promotes efficient infection in trans of cells that express CD4 and chemokine receptors. We have identified another gene, designated here as DC-SIGN2, that exhibits high sequence homology with DC-SIGN. Here we demonstrate that alternative splicing of DC-SIGN1 (original version) and DC-SIGN2 pre-mRNA generates a large repertoire of DC-SIGN-like transcripts that are predicted to encode membrane-associated and soluble isoforms. The range of DC-SIGN1 mRNA expression was significantly broader than previously reported and included THP-1 monocytic cells, placenta, and peripheral blood mononuclear cells (PBMCs), and there was cell maturation/activation-induced differences in mRNA expression levels. Immunostaining of term placenta with a DC-SIGN1-specific antiserum showed that DC-SIGN1 is expressed on endothelial cells and CC chemokine receptor 5 (CCR5)-positive macrophage-like cells in the villi. DC-SIGN2 mRNA expression was high in the placenta and not detectable in PBMCs. In DCs, the expression of DC-SIGN2 transcripts was significantly lower than that of DC-SIGN1. Notably, there was significant inter-individual heterogeneity in the repertoire of DC-SIGN1 and DC-SIGN2 transcripts expressed. The genes for DC-SIGN1, DC-SIGN2, and CD23, another Type II lectin, colocalize to an approximately 85 kilobase pair region on chromosome 19p13.3, forming a cluster of related genes that undergo highly complex alternative splicing events. The molecular diversity of DC-SIGN-1 and -2 is reminiscent of that observed for certain other adhesive cell surface proteins involved in cell-cell connectivity. The generation of this large collection of polymorphic cell surface and soluble variants that exhibit inter-individual variation in expression levels has important implications for the pathogenesis of HIV-1 infection, as well as for the molecular code required to establish complex interactions between antigen-presenting cells and T cells, i.e. the immunological synapse.

摘要

DC-SIGN是一种具有C型凝集素胞外结构域的II型膜蛋白,其在树突状细胞(DC)中的表达被认为在DC与静止T细胞建立初始接触中起重要作用。DC-SIGN也是一种独特的人类免疫缺陷病毒1型(HIV-1)附着因子,可促进表达CD4和趋化因子受体的细胞发生高效的反式感染。我们鉴定出了另一个基因,在此命名为DC-SIGN2,它与DC-SIGN具有高度的序列同源性。在此我们证明,DC-SIGN1(原始版本)和DC-SIGN2前体mRNA的可变剪接产生了大量类似DC-SIGN的转录本,预计这些转录本可编码膜相关和可溶性异构体。DC-SIGN1 mRNA的表达范围比先前报道的要广泛得多,包括THP-1单核细胞、胎盘和外周血单核细胞(PBMC),并且在细胞成熟/激活过程中mRNA表达水平存在差异。用DC-SIGN1特异性抗血清对足月胎盘进行免疫染色显示,DC-SIGN1在绒毛中的内皮细胞和CC趋化因子受体5(CCR5)阳性巨噬样细胞上表达。DC-SIGN2 mRNA在胎盘中表达较高,而在PBMC中未检测到。在DC中,DC-SIGN2转录本的表达明显低于DC-SIGN1。值得注意的是,所表达的DC-SIGN1和DC-SIGN2转录本库存在显著的个体间异质性。DC-SIGN1、DC-SIGN2和另一种II型凝集素CD23的基因共定位于19号染色体p13.3上一个约85千碱基对的区域,形成了一组经历高度复杂可变剪接事件的相关基因簇。DC-SIGN-1和-2的分子多样性让人联想到在某些其他参与细胞间连接的粘附性细胞表面蛋白中所观察到的情况。这种大量多态性细胞表面和可溶性变体的产生,其表达水平存在个体间差异,这对HIV-1感染的发病机制以及建立抗原呈递细胞与T细胞之间复杂相互作用所需的分子编码(即免疫突触)具有重要意义。

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