骨桥蛋白在子宫内膜细胞的多因素调节

目的:通过体外研究雌激素(E2)、孕激素(MPA)、肝素结合表皮生长因子(HB-EGF)对骨桥蛋白(OPN)在子宫内膜细胞中表达的调节,探讨OPN在子宫内膜表达的意义。方法:体外培养高分化子宫内膜癌细胞Ishikawa细胞株,按实验目的做空白对照(不加刺激因素)和加入E2(10-8mol/L),MPA(10-6mol/L),MPA(10-6mol/L)联合E2(10-8mmol/L),肝素结合表皮生长因子HB-EGF(10ng/mL)刺激48～72h后,采用免疫组化、WesternBlot方法测定各个处理因素下OPN的表达。结果:OPN表达于Ishikawa细胞胞浆,MPA、MPA联合E2和HB-EGF均可增加OPN的表达,E2对其表达无明显影响。结论:OPN在子宫内膜腺上皮细胞的表达同时受孕激素和生长因子的上调,是影响子宫内膜容受性的重要指标。

MMP-9/TIMP-1在子宫内膜细胞中的多因素调节

目的 通过体外实验研究E2、MPA、HB -EGF对Ishikawa细胞中MMP - 9/TIMP - 1mRNA表达的调节,探讨其在胚胎种植中的意义。方法 体外培养Ishikawa细胞,分别加入E2、MPA、E2 +MPA、E2 +MPA +RU4 86、HB -EGF刺激4 8h后,采用原位杂交、RT -PCR测定各种条件下MMP - 9、TIMP - 1mRNA的表达。结果 雌、孕激素单独或联合作用均可以显著降低TIMP - 1mRNA的表达(P <0 .0 5 ) ,同时加RU4 86后TIMP - 1mRNA的下降趋势减弱。相反HB -EGF使TIMP - 1mRNA的表达增高(P <0 .0 5 )。Ishikawa细胞中MMP - 9mRNA均没有阳性表达。结论 (1)雌、孕激素对TIMP - 1mRNA具有下调作用,RU4 86可以抑制孕激素的作用。(2 )HB -EGF对TIMP - 1mRNA的表达具有上调作用。(3)MMP - 9mRNA在Ishikawa细胞中没有表达。

高压交直流混联电网架空输电线路施工技术研究

为了提高高压交直流混联电网架空输电线路施工质量与线路抗干扰能力,进行了高压交直流混联电网架空输电线路施工技术研究。构建输电线路施工约束参数模型,采用混合MMC电容电压波动调节方法进行输电线路输出载荷的稳定性调节;结合电网混合拓扑结构进行输电线路的组网设计,采用多因素反馈调节方法进行负电平输出稳定性调节;结合模块投切输出转换控制方法进行高压交直流混联电网的负载均衡控制;采用排序方法均衡输出输电线路子模块之间的电容电压,实现高压交直流混联电网架空输电线路施工技术优化。仿真结果表明,负载均衡性较好,抗干扰能力较强,提高了高压交直流混联电网架空输电线路的稳定性和可靠性。

Is the iron regulatory hormone hepcidin a risk factor for alcoholic liver disease?

Despite heavy consumption over a long period of time, only a small number of alcoholics develop alcoholic liver disease. This alludes to the possibility that other factors, besides alcohol, may be involved in the progression of the disease. Over the years, many such factors have indeed been identified, including iron. Despite being crucial for various important biological processes, iron can also be harmful due to its ability to catalyze Fenton chemistry. Alcohol and iron have been shown to interact synergistically to cause liver injury. Iron-mediated cell signaling has been reported to be involved in the pathogenesis of experimental alcoholic liver disease. Hepcidin is an iron-regulatory hormone synthesized by the liver, which plays a pivotal role in iron homeostasis. Both acute and chronic alcohol exposure suppress hepcidin expression in the liver. The sera of patients with alcoholic liver disease, particularly those exhibiting higher serum iron indices, have also been reported to display reduced prohepcidin levels. Alcohol-mediated oxidative stress is involved in the inhibition of hepcidin promoter activity and transcription in the liver. This in turn leads to an increase in intestinal iron transport and liver iron storage. Hepcidin is expressed primarily in hepatocytes. It is noteworthy that both hepatocytes and Kupffer cells are involved in the progression of alcoholic liver disease. However, the activation of Kupffer cells and TNF-α signaling has been reported not to be involved in the down-regulation of hepcidin expression by alcohol in the liver. Alcohol acts within the parenchymal cells of the liver to suppress the synthesis of hepcidin. Due to its crucial role in the regulation of body iron stores, hepcidin may act as a secondary risk factor in the progression of alcoholic liver disease. The clarification of the mechanisms by which alcohol disrupts iron homeostasis will allow for further understanding of the pathogenesis of alcoholic liver disease.