基因Ⅲ型新城疫病毒感染鸡外周血单个核细胞后的靶细胞分析

新城疫(ND)是鸡新城疫强毒株引起的一种鸡的烈性传染病,目前疫苗接种是防治该病的主要手段。临床上曾分离到与中等毒力疫苗株Mukteswar高度同源的强毒株JS/7/05/Ch,其通过静脉注射后毒力显著增强。为了探究JS/7/05/Ch经血液途径毒力增强的机制,本研究选用鸡外周血单个核细胞(PBMC)作为研究模型,分析基因Ⅲ型NDV在PBMC中的靶细胞。细胞分选结果表明病毒感染可诱导PBMC中单核细胞的增殖。实验组病毒感染后单核细胞相对占比上升,感染后1d Mukteswar组(Muk组)单核细胞占比16.3%,JS/7/05/Ch组(JS组)为13.21%,而对照组单核细胞仅占比3.18%。荧光定量PCR测定分选后各细胞中的病毒载量,感染后3d JS组单核细胞中的病毒含量与感染后1d相比极显著性增加(P<0.01)。感染后1d病毒以感染淋巴细胞为主,而在感染后3d单核细胞的相对病毒含量均超过淋巴细胞占据主导地位,Muk组和JS组分别为54.2%和60.2%。综上所述,基因Ⅲ型NDV在PBMC中的靶细胞是单核巨噬细胞。这为进一步研究这对基因Ⅲ型模式病毒毒力差异的机制奠定了一定基础。     

番茄果实成熟过程中番茄红素含量及合成相关基因表达的分析

以2个高代自交系粉果番茄MLK1和红果番茄FL1为材料,利用实时荧光定量PCR技术及色差仪法,对果实成熟过程中4个时期的番茄红素含量分析及八氢番茄红素合成酶(Psy1和Psy2)和番茄红素环化酶(Lcy)基因的表达进行研究。结果表明,在番茄果实成熟的过程中,番茄红素的含量也逐渐增高,在完熟期达到最高,且红果中的含量高于粉果中的。在2个番茄品种果实不同部位中,Psy1、Psy2和Lcy基因在果实逐渐成熟的过程中转录水平均逐渐增加,在完熟期表达量最高,且红果FL1中的表达量高于粉果MLK1表达量,果实中Psy基因的表达量高于Lcy基因的表达量。     

红色原鸡外周血单个核细胞IFN-γ的诱导表达及其荧光定量PCR检测

为建立检测红色原鸡外周血单个核细胞(PBMC)中干扰素γ(IFN-γ)mRNA表达水平的方法,通过优化刀豆蛋白A(Con A)诱导PBMC表达IFN-γ的条件,采用RT-PCR方法以3-磷酸甘油脱氢酶(GAPDH)基因为内参扩增IFN-γ基因,插入克隆载体pMD18-T分别构建重组质粒pMD-IFN-γ和pMD-GAPDH,以其作为标准品采用SYBR Green I染料法建立荧光定量PCR检测方法,并将该方法应用于34只红色原鸡PBMC IFN-γ表达量的检测。结果发现,PBMC在20μg/mL Con A刺激培养12-25 h时IFN-γ处于高表达水平;标准品质粒pMD-IFN-γ和pMD-GAPDH分别在拷贝数6.72×102-6.72×109、3.94×102-3.94×109范围内与其对应的Ct值呈现良好的线性关系(R20.99),扩增产物的熔解曲线均只有特异的单峰,表明所用引物特异性强。在优化Con A诱导红色原鸡PBMC表达IFN-γ条件的基础上,建立了可用于定量检测红色原鸡PBMC IFN-γmRNA表达水平的荧光定量PCR方法。     

绵羊ghrelin基因表达的组织分布和发育性变化

选取2、30、60、90和120日龄的雄性哈萨克羊和新疆细毛羊各6只（无120日龄的哈萨克羊）,测体重后屠宰,采下丘脑、垂体、心脏、肝脏、瘤胃、网胃、瓣胃、皱胃、十二指肠、背最长肌,用RT-PCR和荧光实时定量PCR法检测ghrelin基因表达的组织分布,及其在皱胃中的发育性变化。研究结果表明：（1）品种内各生长时期的体重差异显著（P〈0．05）。雄性哈萨克羊和新疆细毛羊的体重在2日龄时无显著差异（P〉0．05）,30～90日龄间,前者的体重极显著高于后者（P〈0．01）;（2）所检测的各组织中都有ghrelin mRNA分布,但主要在皱胃中表达,其表达量远高于其他组织（P＜0．05）;（3）两品种绵羊皱胃ghrelin基因表达的发育性变化模式基本相似,都随着日龄的增加而呈上升趋势,其中雄性哈萨克羊的表达量在2～60日龄间持续上升,60日龄后趋于水平;雄性新疆细毛羊的表达量在2～90日龄间持续上升,90日龄后趋于水平。研究还发现雄性哈萨克羊皱胃胂relin基因的表达量在2～90日龄间极显著高于新疆细毛羊（P＜0．01）。     

温肾咳喘片主要成分对HepG2细胞中CYP相关基因表达的影响

观察温肾咳喘片组方中5种主要单体成分甘草酸、厚朴酚、和厚朴酚、蛇床子素和 欧前胡素对细胞色素P450(cytochrome P450, CYP) 1A2,2D6,2E1和3A4基因表达的影 响. 采用实时荧光定量PCR技术检测HepG2细胞中药物处理后各CYP mRNA的表达.厚朴酚 、和厚朴酚、蛇床子素和欧前胡素在不同浓度均能明显的诱导CYP2E1和CYP3A4,同时欧 前胡素也能诱导CYP1A2的表达,而甘草酸、厚朴酚、和厚朴酚、蛇床子素和欧前胡素在 不同浓度对CYP2D6的表达均具有较弱的抑制作用.甘草酸、厚朴酚、和厚朴酚、蛇床子 素和欧前胡素能明显影响CYP1A2、2D6、2E1或3A4的表达.此研究为中西药物代谢性相互 作用及毒理学的研究提供实验依据.     

基因表达常规研究方法概述

基因的表达和功能研究作为当前分子生物学领域的热点,其研究方法也在不断发展,本文对发展过程中出现的应用较为广泛和近年来新发展起来的几种技术作一简要的概述。     

应用基因表达芯片分析水稻高温胁迫相关基因

非生物逆境,如低温、高温、干旱通常会严重影响到农作物的生长及产量,其中高温胁迫则是造成植物伤害的主要原因之一.为深入了解水稻高温胁迫反应的分子机理,发现新的耐高温相关功能基因,为水稻生物工程育种提供候选材料,采用Affymetrix水稻表达芯片分析了超级稻两优培九母本培矮64S(Oryza sativa L.)在高温逆境胁迫下,孕穗期、抽穗开花期的叶片全基因组表达谱,得到大量高温诱导表达基因.应用实时定量PCR方法对其中一部分基因的表达水平进一步分析,所得结果与基因芯片结果基本吻合,证明芯片分析数据是可靠的,为下一步耐高温相关基因的克隆、功能分析等研究提供了基础.     

HBV感染者外周血PBMC中TLR4 mRNA与病毒载量的相关性研究

目的探讨乙型肝炎病毒感染者外周血PBMC中TLR mRNA与乙肝病毒复制的相关性。方法采用逆转录PCR检测外周血单个核细胞（PBMC）中TLR4 mRNA的含量,实时荧光定量Real Time PCR的方法检测HBV DNA,进行相关性分析。结果不同病毒载量组（〈1×103copies/μg DNA,1×103copies/μg DNA〈且〈1×105copies/μg DNA,〉1×105copies/μg DNA）TLR4 mRNA水平差异具有显著性（P〈0.01）,HBV病毒载量的对数值与TLR4 mRNA的含量存在负相关（r=-0.537,P〈0.01）。TLR4 mRNA的相对表达量与患者的ALT、AST呈正相关（r=0.608、r=0.659,P〈0.01）。结论HBV在患者体内复制活跃、病毒载量增高与外周血单个核细胞TLR4mRNA的表达下调有关。     

支气管哮喘患者血清IL-4、TNF-α 及IgE 水平变化及临床意义

目的:研究支气管哮喘患者白细胞介素-4(IL-4)、肿瘤坏死因子-α(TNF-α)及免疫球蛋白E(IgE)水平变化及临床意义.方法:对78例支气管哮喘患者(急性发作期组39例、缓解期组39例)血清IL-4、TNF-α、IgE水平进行检测,并与正常对照组的40例健康受试者进行比较分析.结果:支气管哮喘患者组血清IL-4、TNF-α、IgE水平显著高于正常对照组,差异均有统计学意义(P＜0.05);急性发作期组血清IL-4、TNF-α、IgE水平均显著高于缓解期组,差异亦均有统计学意义(P＜0.05);支气管哮喘患者血清IL-4、TNF-α、IgE水平两两之间呈正性显著相关(P＜0.05).结论:检测支气管哮喘患者血清IL-4、TNF-α、IgE水平对患者疾病预测及治疗具有重要的临床意义.     

应用基因芯片检测酸味抗病甜瓜果实基因表达

利用Melon cDNA array ver1.0检测新疆厚皮甜瓜(Cucumis melo var.ameri)果实基因表达的可行性,并检测了经60Coγ射线辐射诱变后的新疆厚皮甜瓜酸味抗病变异株成熟果实基因的表达.结果显示:该芯片平均能够检测新疆厚皮甜瓜基因2 008个,检测出的基因占该芯片基因探针总数的65.4%;检测酸味抗病变异株上调表达的基因251个,占检出基因总数的12.5%;下调表达的基因224个,占检出基因总数的11.16%.利用RT-PCR验证芯片结果的可靠性,结果表明,用Melon cDNA array ver 1.0检测新疆厚皮甜瓜成熟果实基因表达水平是可行的.     

轮状病毒感染患者外周血单个核细胞的转录组学分析

轮状病毒(Rotavirus,RV)是引起急性肠胃炎的主要病原体,分析RV感染患者的人外周血单个核细胞(Peripheral blood mononuclear cell,PBMC)中差异表达基因(Differentially expressed genes,DEGs)有利于探讨人PBMC在清除RV中的作用。为此,本研究采集2019年2月-2019年6月长春儿童医院中RV感染患者和健康儿童血液,分离PBMC,通过转录组测序(RNA sequencing,RNA-seq)技术比较RV感染患者与健康儿童之间的RNA表达图谱,借助基因本体论(Gene Ontology,GO)数据库功能富集分析、京都基因与基因组百科全书(Kyoto Encyclopedia of Genes and Genomes,KEGG)、Reactome通路富集分析DEGs,使用实时荧光定量PCR(Real-time quantitative PCR,qPCR)技术进行验证。结果显示,与健康对照组相比,RV感染轻症患者PBMC中有1619个DEGs;重症患者PBMC中有2816个DEGs,主要与干扰素(Interferon,IFN)反应、中性粒细胞、溶酶体、核小体、染色质等相关。qPCR验证轻症患者干扰素刺激基因(IFN-stimulated genes,ISGs)15表达上调,白介素(Interleukin,IL)1β表达下调;重症患者IL15、ISG15表达上调,IL1β表达下调,与转录组结果相一致。本研究提示,RV感染可能激活人I型和II型IFNs反应抵御病毒感染,但也会抑制溶酶体相关基因,对细胞自噬过程产生影响。     

A Comparative Analysis of Gene Expression Patterns and Cell Phenotypes between Cervical and Peripheral Blood Mononuclear Cells

Studies of the immunological environment in the female genital tract (FGT) are critical for the development of vaccines or microbicides to halt the spread of sexually transmitted infections. Challenges arise due to the difficulties of sampling from this site, and the majority of studies have been conducted utilising peripheral blood mononuclear cells. Identifying functional differences between immune cells of the FGT and peripheral blood would aid in our understanding of mucosal immunology. We compared the gene expression profile of mononuclear cells at these two sites. Messenger RNA expression analysis was performed using gene expression arrays on matched cervical mononuclear cells and peripheral blood mononuclear cells. Further cellular phenotyping was done by 10 colour flow cytometry. Of the 22,185 genes expressed by these samples, 5345 genes were significantly differentially expressed between the cell populations. Most differences can be explained by significantly lower levels of T and B cells and higher levels of macrophages and dendritic cells in the FGT compared with peripheral blood. Several immunologically relevant pathways such as apoptosis and innate immune signalling, and a variety of cytokines and cytokine receptors were differentially expressed. This study highlights the importance of the unique immunological environment of the FGT and identifies important differences between systemic and mucosal immune compartments.     

全基因组SHIV-KB9克隆的构建及其在人、猴外周血单核细胞中的复制

将分别携带SHIV-KB9 (SIV/HIV-1 KB9) 基因组的3′端和5′端的两个半长克隆,体外连接成SHIV-KB9全基因组克隆.含有全长基因的质粒培养时易发生同源重组和缺失,采用JM109作为宿主菌以及30℃、低转速的培养条件,可保持质粒的稳定性.通过PCR , RT-PCR 和猴免疫缺陷病毒(SIV) gag p27 核心抗原滴度检测表明感染性克隆SHIV-KB9可有效在人、恒河猴及食蟹猴的外周血单核细胞中复制.     

全基因组SHIV—KB9克隆的构建及其在人、猴外周血单核细胞中的复制

将分别携带SHIV—KB9(SIV/HIV—1KB9)基因组的3′端和5′端的两个半长克隆,体外连接成SHIV—KB9全基因组克隆。含有全长基因的质粒培养时易发生同源重组和缺失,采用JM109作为宿主菌以及30℃、低转速的培养条件,可保持质粒的稳定性。通过PCR,RT—PCR和猴免疫缺陷病毒(SIV)gagp27核心抗原滴度检测表明：感染性克隆SHIV—KB9可有效在人、恒河猴及食蟹猴的外周血单核细胞中复制。     

Herpesvirus DNA in Peripheral Blood Mononuclear Cells of Some Patients with Meniere's Disease

Herpes simplex virus‐1 (HSV) or varicella zoster virus (VZV) DNA was detected by nested polymerase chain reaction in peripheral blood mononuclear cells of patients with Meniere's disease (one of 28 patients for HSV‐1,2 of 28 patients for VZV) during acute illness (within 5 days after onset). On the other hand, neither HSV‐1 DNA or VZV DNA was detected in PBMCs of 50 age‐ and sex‐matched healthy individuals and 50 pregnant women. These findings may imply that reactivation of HSV‐1 or VZV may be associated with the development of some cases of Meniere's disease.     

The Effect of Lung Cancer on Cytokine Expression in Peripheral Blood Mononuclear Cells

The purpose of this study is to evaluate cytokine expression by peripheral blood mononuclear cells (PBMC) from stage I lung cancer patients and to confirm these expression patterns by exposing PBMCs to lung cancer cells in vitro. Five altered cytokines in stage I lung cancer patients (CCL3, IL8, IL1β, CXCL10, sIL2Rα) were identified in plasma from subjects (n = 15) before and after resection using a 30-plex panel protein assay. Gene expression studies using quantitative RT-qPCR were performed on PBMCs from stage I lung cancer patients (n = 62) before and after resection, and compared to non-cancer patients (n = 32) before and after surgery for benign disease. Co-culture experiments that exposed healthy donor PBMCs to lung cancer cells in vitro were performed to evaluate the effect on PBMC cytokine expression. PBMC gene expression of CCL3, IL8 and IL1β was higher in lung cancer patients compared to the same patients at each of four sequential timepoints after removal of their tumors, while CXCL10 and IL2Rα were essentially unchanged. This pattern was also detected when lung cancer patients were compared to non-cancer patients. When non-cancer patients underwent surgery for benign diseases, these cytokine expression changes were not demonstrable. Lung cancer cell lines, but not benign bronchial epithelial cells, induced similar changes in cytokine gene and protein expression by healthy donor PBMCs in an in vitro co-culture system. We conclude that PBMCs from stage I lung cancer patients possess distinct cytokine expression patterns compared to both non-cancer patients, and lung cancer patients following tumor removal. These expression patterns are replicated by healthy donor PBMCs exposed to lung cancer cell lines, but not benign bronchial epithelial cells in vitro. These findings have implications for understanding the immune response to lung cancer.     

Inhibition of Varicella-Zoster Virus Glycoprotein Expression by Peripheral Blood Mononuclear Cells

The effect of peripheral blood mononuclear cells (PBMC) on expression of varicella-zoster virus (VZV) glycoproteins (Gps) was analyzed by flow cytometry. PBMC from VZV seropositive and seronegative donors and supernatant of PBMC co-cultured with VZV-infected human embryonic fibroblasts reduced VZV Gp expression. Neutralization of supernatant fluid with mixture of anti-interferons (IFN)-α, -β, -γ, and tumor necrosis factor (TNF)-α partially reduced inhibitory activity of supernatant on VZV Gp expression. Deletion of natural killer (NK) cells and adherent cells from PBMC reduced inhibitory activity of PBMC on VZV Gp expression. These results suggest that IFN-α, -β, -γ, TNF-α and other soluble factors released from NK cells and monocytes by co-cultivation with VZV-infected fibroblasts inhibit VZV Gp expression.     

脱氧雪腐镰刀菌烯醇对人外周血单个核细胞 HLA-I分子表达的影响

研究探讨了脱氧雪腐镰刀菌烯醇(DON)对人外周血单个核细胞HLA-I(human leucocyte cyte antigen I)分子表达影响.采用流式细胞术(FCM)和免疫印迹方法研究了不同剂量DON对体外培养人外周血单个核细胞表面HLA-I分子表达的影响及其量效关系.FCM定量检测结果表明,不同浓度DON处理均可一定程度降低人外周血单个核细胞表面HLA-I分子的表达,DON 50ng/mL、100ng/mL、1000 ng/mL和2000 ng/mL组HLA-I类分子的平均表达量分别为6.92±0.68、6.64±0.69、5.95±0.48和5.48±0.77,在50～2000ng/mL范围内随着DON浓度增加,外周血单个核细胞HLA-I分子表达降低,两者呈显著负相关(r=0.737,P＜0.01).Western印迹结果显示,大剂量DON(1000ng/mL和2000ng/mL)组人外周血单个核细胞HLA-I分子表达明显减弱.研究结果表明脱氧雪腐镰刀菌烯醇可剂量依赖地抑制体外培养的人外周血单个核细胞HLA-I分子的表达.     

黑线仓鼠及其白化突变系TYR、TYRP1的基因表达水平比较分析

目的本研究旨在研究TYR、TYRP1基因在黑线仓鼠与白化突变系皮肤组织中的表达情况,探索其与白化毛色性状的产生是否具有相关性。方法以黑线仓鼠和白化突变系皮肤组织为研究对象,采用实时荧光定量PCR技术,分别得到黑线仓鼠与白化突变系TYR和TYRP1基因的相对表达量。结果黑线仓鼠皮肤中的TYR和TYRP1基因的mRNA相对表达量分别是白化突变系皮肤组织中的2.5倍和5.3倍。结论表明黑线仓鼠皮肤中TYR、TYRP1的基因表达水平存在表达差异,白化突变系TYR、TYRP1基因发生表达下调,揭示出了TYR、TYRP1基因的表达量与白化突变系白化性状的产生有关。