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在人胎盘绒毛滋养层细胞中合成无β2-微球蛋白、二硫键连接的HLA-G5同型二聚体。

Synthesis of beta(2)-microglobulin-free, disulphide-linked HLA-G5 homodimers in human placental villous cytotrophoblast cells.

作者信息

Morales Pedro J, Pace Judith L, Platt Jeralyn Sue, Langat Daudi K, Hunt Joan S

机构信息

Department of Anatomy and Cell Biology, University of Kansas Medical Center, Kansas City, KS 66160-7400, USA.

出版信息

Immunology. 2007 Oct;122(2):179-88. doi: 10.1111/j.1365-2567.2007.02623.x. Epub 2007 May 2.

Abstract

Human leucocyte antigen-G (HLA-G) is a natural immunosuppressant produced in human placentas that binds differently to the inhibitory leucocyte immunoglobulin-like receptors LILRB1 (ILT2) and LILRB2 (ILT4) according to its biochemical structure. To predict the binding functions of the HLA-G5 soluble isoform synthesized in placental villous cytotrophoblast (vCTB) cells, we investigated structural features of this protein. Biochemical and immunological studies showed that vCTB cell HLA-G5 heavy (H)-chain proteins are disulphide-bonded homodimers unassociated with beta(2)-microglobulin (beta2m) light-chain proteins. Although comparatively low levels of beta2m messenger RNA (mRNA) were identified by real-time reverse transcription-polymerase chain reaction, immunoprecipitation studies failed to detect beta2m protein even when specific mRNA was doubled by transduction of a lentivirus-beta2m complementary DNA into vCTB cells. No abnormalities were identified in the translational start codon of vCTB cell beta2m mRNA and differentiation into syncytium did not promote beta2m synthesis. The failure of vCTB cells to exhibit beta2m in vitro was paralleled by a lack of detectable beta2m in vCTB cells in vivo. Lack of the beta2m protein could be the result of low levels of beta2m transcripts or of as yet unidentified translational defects. Experiments with recombinant ectodomains of LILRB indicate that beta2m-free HLA-G binds strongly to LILRB2, a receptor that is expressed by macrophages. This potentially immunosuppressive cell type is abundant in the pregnant uterus. Thus, our findings are consistent with the postulate that the natural beta2m-free homodimeric form of HLA-G5 synthesized in primary vCTB cells could comprise a particularly effective tolerogenic molecule at the maternal-fetal interface.

摘要

人类白细胞抗原G(HLA - G)是一种在人胎盘中产生的天然免疫抑制剂,根据其生化结构,它与抑制性白细胞免疫球蛋白样受体LILRB1(ILT2)和LILRB2(ILT4)的结合方式不同。为了预测在胎盘绒毛细胞滋养层(vCTB)细胞中合成的HLA - G5可溶性异构体的结合功能,我们研究了该蛋白的结构特征。生化和免疫学研究表明,vCTB细胞的HLA - G5重链(H)蛋白是通过二硫键结合的同型二聚体,与β2 - 微球蛋白(β2m)轻链蛋白不相关。尽管通过实时逆转录 - 聚合酶链反应鉴定出相对较低水平的β2m信使核糖核酸(mRNA),但免疫沉淀研究未能检测到β2m蛋白,即使通过将慢病毒 - β2m互补DNA转导到vCTB细胞中使特定mRNA加倍时也是如此。在vCTB细胞β2m mRNA的翻译起始密码子中未发现异常,并且向合体滋养层的分化并未促进β2m的合成。vCTB细胞在体外未能表现出β2m,在体内vCTB细胞中也缺乏可检测到的β2m。β2m蛋白的缺失可能是β2m转录本水平低或尚未确定的翻译缺陷的结果。用LILRB的重组胞外域进行的实验表明,不含β2m的HLA - G与巨噬细胞表达的受体LILRB2强烈结合。这种具有潜在免疫抑制作用的细胞类型在妊娠子宫中大量存在。因此,我们的研究结果与以下假设一致:在原代vCTB细胞中合成的天然不含β2m的HLA - G5同型二聚体形式可能是母胎界面处一种特别有效的致耐受性分子。

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