早孕滋养细胞膜型及可溶性趋化因子CXCL16表达调控

目的 探讨趋化因子CXCL16在人早孕滋养细胞表达和释放的调控机制.方法 原代培养人早孕滋养细胞,实时定量RT-PCR、免疫化学和ELISA方法分析CXCL16的表达和分泌;ELISA方法分析细胞因子IFN-γ、TNF-α、IL-4刺激前后滋养细胞CXCL16的表达和分泌水平;ELISA方法分析ADAM10治疗前后滋养细胞CXCL16的表达及分泌水平.结果 滋养细胞表达并分泌趋化因子CXCL16;IFN-γ治疗后滋养细胞表达和分泌CXCL16水平均显著上升(P<0.01),但TNF-α和IL-4并不影响CXCL16的表达或分泌;ADAM10可以加速CXCL16自滋养细胞的脱落,但并不上调CXCL16的合成.结论 IFN-γ和ADAM10参与调控母胎界面滋养细胞趋化因子CXCL16的合成和分泌.

The synthesis and shedding of transmembrane CXCL16 in first-trimester human trophoblast

Objective To detect the regulation of CXCL16 synthesis and shedding in first-trimester human trophoblasts. Methods Firstly, we analyzed the expression and secretion of chemokine CXCL16 in primary cultured trophoblasts by immunochemical staining and ELISA. Then we determined the soluble and cell-associated CXCLI6 respectively with and without treatments of cytokine IFN-γ, TNF-α, IL-4 and ADAM10 by ELISA. Results Trophoblast expressed and secreted CXCL16 in a stable level. Cytokine IFN-γ induced both synthesis and secretion of CXCL16 significantly ( P <0. 01 ) in trophoblasts. ADAM10 increased the shedding of chemokine domain of CXCL16 from trophoblasts but didn't influence the synthesis of CXCL16 protein in trophoblast. Conclusion IFN-γ and ADAM10 play important roles in production and shedding of transmembrane CXCL16 in first-trimester trophublasts.