人可溶性DSG2胞外域蛋白的真核表达、纯化及活性鉴定

目的:构建DSG2与人IgG Fc片段融合的分泌型真核表达载体,在293T细胞中验证其表达,纯化具有生物活性的分泌型蛋白。方法:通过PCR扩增DSG2胞外域片段基因(DSG2 extracellular domain,DSG2ex),并将其整合到真核表达质粒pCMV3-IgG1中,构建重组真核表达质粒pCMV3-DSG2ex-IgG1。将构建成功的真核表达质粒转染入293T细胞中,使细胞外分泌表达DSG2胞外域蛋白,收集细胞上清液,经亲和层析Protein A纯化后,进行Western Blotting和ELISA活性鉴定。结果:成功构建了pCMV3-DSG2ex-IgG1真核表达质粒。转染后96 h蛋白表达量最高,表达产物纯化后经SDS-PAGE电泳分析其相对分子质量在100~130 kDa之间,与预期一致,纯化的融合蛋白纯度达90%以上,含量为0.8 mg/mL。通过Western Blot检测纯化后带有IgG1标签的DSG2胞外域蛋白能被IgG单克隆抗体识别。ELISA结果显示制备的DSG2胞外域蛋白具有明显结合人55型腺病毒(HAdV-55)Fiber Knob蛋白的活性,结论:成功建立了一种简单高效的人可溶性DSG2胞外域蛋白真核表达及纯化的方法,且纯化出来了具有生物活性的DSG2胞外域蛋白,为后期其蛋白功能研究及抗腺病毒药物的研究奠定了基础。

Eukaryotic expression, purification and activity characterization of human soluble DSG2 extracellular domain protein

Objective:To construct a secretory eukaryotic expression vector of DSG2 fused with the Fc region of the human IgG,to validate its expression in 293T cells,and to purify the secretory protein with biological activity.Methods:The DSG2 extracellular domain fragment gene(DSG2ex),was amplified by PCR,and was inserted into the eukaryotic expression plasmid pCMV3-IgG1 to construct the recombinant eukaryotic expression plasmid-pCMV3-DSG2ex-IgG1.The successfully constructed eukaryotic expression plasmid was transfected into 293T cells to express and secrete DSG2 extracellular domain protein.The targeted protein was purified from the cell culture supernatant by Protein A affinity chromatography and confirmed by Western Blotting and ELISA.Results:The pCMV3-DSG2ex-IgG1 eukaryotic expression plasmid was successfully constructed.The highest protein expression level was obtained with 293T cells after 96 h of transfection.The relative molecular mass of the purified product was between 100 and 130 kDa was estimated by SDS-PAGE,which was consistent with the expectation.The yield of the purified protein reached 0.8 mg/ml with a purity over 90%.The purified DSG2 extracellular domain protein with IgG1 tag was recognized by IgG monoclonal antibodies by Western blotting.Moreover,the ELISA results showed that the prepared DSG2 extracellular domain protein had significant binding activity to human type 55 adenovirus Fiber Knob protein(HAdV-55).Conclusion:A simple and efficient method for eukaryotic expression and purification of human soluble DSG2 extracellular domain protein was successfully established,and biologically active DSG2 extracellular domain protein was purified,which laid the foundation for the later study of its protein function and anti-adenovirus drugs.

Dpagt1和Dsg2相关信号通路与肿瘤干细胞

肿瘤干细胞(cancer stem cells,CSCs)是肿瘤发生、发展、侵袭、转移、复发及耐药的决定性因素。基于微环境对干细胞的重要影响作用,本课题组在前期研究中成功的将鼠诱导的多能干细胞(mouse induced plur ipotent stem cel l s,mi PS)在肿瘤微环境的作用下诱导成CSCs,并发现Dsg2基因和Dpagt1基因的表达分别上调了4倍和6倍。有研究表明Dsg2和Dpagt1在多种肿瘤中过表达,在细胞黏附、增殖及恶性转化中起着至关重要的作用,并且与肿瘤干细胞关系密切。本文主要就Dpagt1和Dsg2在Wnt/β-catenin、EGFR等信号通路中对肿瘤干细胞的作用及其信号通路间的相互联系进行综述。

钙黏蛋白E、桥粒芯糖蛋白2、磷酸化Akt和转录因子Snail在侵袭性前列腺癌中的作用

目的探讨钙黏蛋白E(E-cadherin)、桥粒芯糖蛋白(2DSG2)、磷酸化Akt(pAkt)和转录因子Snail在前列腺癌发病进程中的作用;阐明E-cadherin、DSG2、pAkt和Snail对前列腺癌发病进程的影响及在临床预后中的作用。方法组织芯片法检测E-cadherin、DSG2、pAkt和Snail在前列腺癌组织中的表达情况。结果前列腺癌组织中E-cadherin表达明显低于正常前列腺组织,细胞质和细胞核中均可观察到pAkt表达,且在肿瘤高分化区和低分化区内均有较高表达。E-cadherin和DSG2表达呈显著正相关。E-cadherin和DSG2表达下降提示前列腺癌患者血清前列腺特异性抗原(PSA)浓度含量增加,Gleason评分较高及病理分期更高。结论前列腺癌低分化细胞中钙黏蛋白表达降低,钙黏蛋白低表达提示肿瘤细胞侵袭性更强,转移发生率高。钙黏蛋白在前列腺癌发展中发挥关键作用,E-cadherin和DSG2有望成为侵袭性前列腺癌的预后因子。

桥粒黏蛋白2在消化系统肿瘤中的功能研究进展

桥粒黏蛋白2(desmoglein-2,DSG2)是钙黏着蛋白家族成员之一,作为桥粒的重要组成部分,主要起维持细胞间黏附的作用。研究发现,DSG2还可以通过信号转导调控细胞的增殖、分化和凋亡,在调节肠上皮屏障中也发挥着关键作用。随着研究的深入,越来越多的证据表明DSG2在多种消化系统肿瘤中表达异常,表达水平各有不同,而表达水平与肿瘤的预后密切相关,推测DSG2在不同的消化系统肿瘤的发生和发展中发挥不同的作用。该文就DSG2的生物学功能及其在消化系统肿瘤中的作用进行综述。

Desmoglein 2(DSG2) Is A Receptor of Human Adenovirus Type 55 Causing Adult Severe Community-Acquired Pneumonia

Human adenovirus type 55(HAdV-B55) is a re-emergent acute respiratory disease pathogen that causes adult communityacquired pneumonia(CAP). Previous studies have shown that the receptor of HAdV-B14, which genome is highly similar with HAdV-B55, is human Desmoglein 2(DSG2). However, whether the receptor of HAdV-B55 is DSG2 is undetermined because there are three amino acid mutations in the fiber gene between HAdV-B14 and HAdV-B55. Here, firstly we found the 3T3 cells, a mouse embryo fibroblast rodent cell line which does not express human DSG2, were able to be infected by HAdV-B55 after transfected with pcDNA3.1-DSG2, while normal 3T3 cells were still unsusceptible to HAdV-B55 infection. Next, A549 cells with h DSG2 knock-down by siRNA were hard to be infected by HAdV-B3/-B14/-B55, while the control siRNA group was still able to be infected by all these types of HAdVs. Finally, immunofluorescence confocal microscopy indicated visually that Cy3-conjugated HAdV-B55 viruses entered A549 cells by binding to DSG2 protein.Therefore, DSG2 is a major receptor of HAdV-B55 causing adult CAP. Our finding is important for better understanding of interactions between adenoviruses and host cells and may shed light on the development of new drugs that can interfere with these processes as well as for the development of potent prophylactic vaccines.

电励磁双凸极发电机分裂电容全桥整流拓扑分析

以12/8极电励磁双凸极发电机(DSEG)为研究对象,针对DSG2发电方式,提出分裂电容全桥整流方式,即发电机三相绕组中点接分裂电容式整流。借助有限元计算分析电容的不同接法对发电机输出特性的影响。研究结果表明,合理的选择容值,分裂电容全桥整流方式能提高换相后相绕组电流的上升率和有效值,使得一周期内的磁场储能得到提高,从而提高发电机的输出功率;傅里叶分析结果表明,分裂电容全桥整流方式对相电压和相电流的相位关系有一定的改善作用。原理样机的实验结果验证了此方式的有效性。

双凸极电机并联补偿电容全桥整流特性的研究

双凸极电机相绕组自感较大,限制了相电流的变化率和幅值。相绕组呈感性使得相电流滞后相电势,在电机工作过程中,存在无功功率,从而降低发电机的功率因数和发电功率。针对相绕组自感对电机特性的影响,提出一种在全桥整流方式基础上并联补偿电容的发电拓扑(Parallel Capacitances Full-Bridge Rectifier,PCFBR),并借助有限元仿真软件,针对一台8/6极电励磁双凸极发电机,得到在新的拓扑下的发电特性曲线。对原理样机进行实验,验证了仿真分析的正确性。分析结果表明:通过并联电容补偿,可以明显提高电励磁双凸极发电机的发电功率。