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EMILIN1是决定人类滋养层细胞侵入子宫壁的主要基质成分。

EMILIN1 represents a major stromal element determining human trophoblast invasion of the uterine wall.

作者信息

Spessotto Paola, Bulla Roberta, Danussi Carla, Radillo Oriano, Cervi Marta, Monami Giada, Bossi Fleur, Tedesco Francesco, Doliana Roberto, Colombatti Alfonso

机构信息

Divisione di Oncologia Sperimentale 2, CRO-IRCCS, 33081 Aviano, Italy.

出版信息

J Cell Sci. 2006 Nov 1;119(Pt 21):4574-84. doi: 10.1242/jcs.03232.

Abstract

The detection of EMILIN1, a connective tissue glycoprotein associated with elastic fibers, at the level of the ectoplacental cone and trophoblast giant cells of developing mouse embryos (Braghetta et al., 2002) favored the idea of a structural as well as a functional role for this protein in the process of placentation. During the establishment of human placenta, a highly migratory subpopulation of extravillous trophoblasts (EVT), originating from anchoring chorionic villi, penetrate and invade the uterine wall. In this study we show that EMILIN1, produced by decidual stromal and smooth muscle uterine cells, is expressed in the stroma and in some instances as a gradient of increasing concentration in the perivascular region of modified vessels. This distribution pattern is consistent with the haptotactic directional migration observed in in vitro functional studies of freshly isolated EVT and of the immortalized HTR-8/SVneo cell line of trophoblasts. Function-blocking monoclonal antibodies against alpha4-integrin chain and against EMILIN1 as well as the use of EMILIN1-specific short interfering RNA confirmed that trophoblasts interact with EMILIN1 and/or its functional gC1q1 domain via alpha4beta1 integrin. Finally, membrane type I-matrix metalloproteinase (MT1-MMP) and MMP-2 were upregulated in co-cultures of trophoblast cells and stromal cells, suggesting a contributing role in the haptotactic process towards EMILIN1.

摘要

在发育中小鼠胚胎的外胎盘锥和滋养层巨细胞水平检测到与弹性纤维相关的结缔组织糖蛋白埃米林1(EMILIN1)(Braghetta等人,2002年),这支持了该蛋白在胎盘形成过程中具有结构和功能作用的观点。在人类胎盘建立过程中,源自锚定绒毛膜绒毛的高迁移性绒毛外滋养层细胞(EVT)亚群会穿透并侵入子宫壁。在本研究中,我们表明,由蜕膜基质和子宫平滑肌细胞产生的EMILIN1,在基质中表达,并且在某些情况下,在改良血管的血管周围区域以浓度递增的梯度形式表达。这种分布模式与在新鲜分离的EVT和永生化滋养层细胞系HTR-8/SVneo的体外功能研究中观察到的趋触性定向迁移一致。针对α4整合素链和EMILIN1的功能阻断单克隆抗体以及使用EMILIN1特异性短干扰RNA证实,滋养层细胞通过α4β1整合素与EMILIN1和/或其功能性gC1q1结构域相互作用。最后,在滋养层细胞与基质细胞的共培养中,膜型I基质金属蛋白酶(MT1-MMP)和MMP-2上调,表明在朝向EMILIN1的趋触性过程中发挥作用。

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