B19病毒非结构蛋白11 kD对p6启动子和细胞因子启动子的调控作用

【背景】人细小病毒B19是可以感染并引起人类疾病的两种细小病毒科成员之一。B19病毒的唯一启动子p6负责病毒RNA的转录。研究表明p6启动子活性与其转录因子结合位点以及B19病毒NS1蛋白的调节有关。但是,关于其他重要位点和B19病毒蛋白是否也具有影响p6启动子活性的作用还未有报道。【目的】探究影响p6启动子活性的重要因素,并明确B19病毒11 kD蛋白与p6启动子及细胞因子启动子的调控关系。【方法】通过生物信息方法预测分析p6启动子转录结合位点及其CpG位点,利用体外甲基化分析CpG位点对p6启动子活性的影响。同时,利用增强绿色荧光蛋白(enhanced green fluorescent protein,EGFP)和荧光素酶报告系统分析影响p6启动子活性的转录因子结合区域以及11 kD蛋白对p6启动子和细胞因子启动子的影响。【结果】p6启动子在不同非敏感细胞系中均有较高活性,并且其302-479区段的转录结合位点CCCTC结合因子(CCCTC-binding factor,CTCF)、阴阳因子(Yin Yang 1,YY1)、信号传导与转录激活因子(signal transducer and activator of transcription 3,STAT3)、Sp1/3和E2F转录调节因子7(E2F transcription factor 7,E2F7)对维持启动子活性很重要。同时,p6启动子活性可被其CpG位点的甲基化修饰所抑制,但不被11kD蛋白所调控。然而11 kD蛋白却能显著上调肿瘤坏死因子(tumor necrosis factor alpha,TNF-α)、白介素6(interleukin 6,IL6)、STAT3启动子的活性。【结论】本研究明晰了B19病毒p6启动子的潜在转录因子结合位点和CpG位点对维持其启动子活性的重要性,并进一步揭示了非结构蛋白11kD与p6启动子以及细胞内因子启动子的关系,推测11 kD蛋白可能通过影响细胞内相关因子的表达,进而在B19病毒与细胞相互作用过程中扮演重要角色。

肌细胞增强因子2c启动子的克隆与活性鉴定

【目的】克隆小鼠肌细胞增强因子2c(Myocyte enhancer factor 2c,Mef2c)的近端启动子,并检测启动子的活性。【方法】提取小鼠畸胎瘤P19细胞基因组DNA,用RT-PCR方法扩增Mef2c近端启动子片段(-1 130/+200),分别构建3个长度不同的Mef2c荧光素酶报告基因载体(约1.3 kb/0.8 kb/0.4 kb),双酶切鉴定所扩增的DNA序列,阳性质粒转染P19细胞,运用DualLuciferase®Reporter Assay System来检测启动子的活性,初步比较分析启动子片段间的活性差异。【结果】小鼠肌细胞增强因子Mef2c近端的启动子克隆成功,并构建了3段不同长度的启动子荧光素酶报告基因载体,双荧光素酶报告基因实验提示Mef2c近端启动子中的3段不同长度的启动子活性不一致。【结论】成功克隆肌细胞增强因子Mef2c的近端启动子并鉴定了相关活性,为进一步研究各种反式因子对Mef2c近端启动子的转录活性调节奠定了基础。

Farnesoid X receptor expression is reduced in human hepatocellular carcinoma

Farnesoid X receptor (FXR, NR1H4) is a member of nuclear hormone receptor superfamily. Previously studies showed that FXR-/- mice spontaneously developed liver tumors when they aged, however, the relevance of which to human hepatocellular carcinoma (HCC) is unclear. The aim of this study is to observe whether FXR expression is also downregulated in HCC and discuss the mechanism of the reduced FXR expression in HCC. Expression of FXR and small heterodimer partner (SHP) was measured by real-time PCR and immunohistochemical technique. Effect of pro-inflammatory cytokines on expression of FXR and its promoter activity were determined in primary hepatocytes or HepG2 and Huh7 cell lines. Our results showed that expression of FXR and its target gene SHP in human HCC was strongly downregulated compared to the normal liver tissues. In addition, pro-inflammatory cytokines were able to decrease FXR expression by inhibiting the FXR promoter activity. In conclusion this work demonstrates FXR expression is strongly downregulated in human HCC, which may be caused by decreased FXR promoter activity, suggesting a potential role of FXR in human HCC development.