AAV-mediated expression of p65shRNA and bone morphogenetic protein 4 synergistically enhances chondrocyte regeneration

BACKGROUND:Adeno-associated virus(AAV)gene therapy has been proven to be reliable and safe for the treatment of osteoarthritis in recent years.However,given the complexity of osteoarthritis pathogenesis,single gene manipulation for the treatment of osteoarthritis may not produce satisfactory results.Previous studies have shown that nuclear factorκB could promote the inflammatory pathway in osteoarthritic chondrocytes,and bone morphogenetic protein 4(BMP4)could promote cartilage regeneration.OBJECTIVE:To test whether combined application of AAV-p65shRNA and AAV-BMP4 will yield the synergistic effect on chondrocytes regeneration and osteoarthritis treatment.METHODS:Viral particles containing AAV-p65-shRNA and AAV-BMP4 were prepared.Their efficacy in inhibiting inflammation in chondrocytes and promoting chondrogenesis was assessed in vitro and in vivo by transfecting AAV-p65-shRNA or AAV-BMP4 into cells.The experiments were divided into five groups:PBS group;osteoarthritis group;AAV-BMP4 group;AAV-p65shRNA group;and BMP4-p65shRNA 1:1 group.Samples were collected at 4,12,and 24 weeks postoperatively.Tissue staining,including safranin O and Alcian blue,was applied after collecting articular tissue.Then,the optimal ratio between the two types of transfected viral particles was further investigated to improve the chondrogenic potential of mixed cells in vivo.RESULTS AND CONCLUSION:The combined application of AAV-p65shRNA and AAV-BMP4 together showed a synergistic effect on cartilage regeneration and osteoarthritis treatment.Mixed cells transfected with AAV-p65shRNA and AAV-BMP4 at a 1:1 ratio produced the most extracellular matrix synthesis(P<0.05).In vivo results also revealed that the combination of the two viruses had the highest regenerative potential for osteoarthritic cartilage(P<0.05).In the present study,we also discovered that the combined therapy had the maximum effect when the two viruses were administered in equal proportions.Decreasing either p65shRNA or BMP4 transfected cells resulted in less collagen II synthesis.This implies that inhibiting inflammation by p65shRNA and promoting regeneration by BMP4 are equally important for osteoarthritis treatment.These findings provide a new strategy for the treatment of early osteoarthritis by simultaneously inhibiting cartilage inflammation and promoting cartilage repair.

血管生成素样蛋白4通过调节成纤维细胞和内皮细胞功能影响糖尿病足进程

背景:研究表明,血管因素对糖尿病足的发生具有重要影响。目的:探讨血管生成素样蛋白4在糖尿病足形成中的重要作用。方法:①对糖尿病足患者的基因表达谱数据进行生物信息学分析,找到关键基因。收集糖尿病足患者以及无糖尿病健康人的皮肤标本进行苏木精-伊红染色、免疫组化染色以及qRT-PCR实验,检测血管生成素样蛋白4表达情况。②培养人永生化皮肤成纤维细胞系和原代人脐静脉内皮细胞,将2种细胞分别分为对照组和外源性补充血管生成素样蛋白4组,通过划痕实验以及CCK-8实验分别检测成纤维细胞的迁移能力和增殖能力,通过Ki67实验检测内皮细胞的增殖能力。结果与结论:①生信分析发现,血管生成素样蛋白4基因的下调可能是导致糖尿病足形成的关键基因。②苏木精-伊红染色结果显示,与正常皮肤相比,血管生成素样蛋白在糖尿病足皮肤内弱表达,且其mRNA水平相对表达量降低(P<0.01)。③划痕实验结果显示,与对照组相比,血管生成素样蛋白4组成纤维细胞迁移能力明显增强;CCK-8细胞增殖实验显示,血管生成素样蛋白4组成纤维细胞的吸光度值在24,48 h均高于对照组(P<0.01,P<0.001);提示血管生成素样蛋白4可增强高糖处理的成纤维细胞迁移及增殖能力。④Ki67实验结果显示,与对照组相比,血管生成素样蛋白4组内皮细胞Ki67阳性细胞数目明显多于对照组;CCK-8细胞增殖实验显示,血管生成素样蛋白4组内皮细胞的吸光度值在24,48 h均高于对照组(P<0.05,P<0.001)。(5)以上结果均提示血管生成素样蛋白4可增强高糖处理内皮细胞的增殖能力。

Neuroprotective effects of acteoside in a glaucoma mouse model by targeting Serta domain-containing protein 4

AIM:To explore the therapeutic effect and main molecular mechanisms of acteoside in a glaucoma model in DBA/2J mice.METHODS:Proteomics was used to compare the differentially expressed proteins of C57 and DBA/2J mice.After acteoside administration in DBA/2J mice,anterior segment observation,intraocular pressure(IOP)monitoring,electrophysiology examination,and hematoxylin and eosin staining were used to analyze any potential effects.Immunohistochemistry(IHC)assays were used to verify the proteomics results.Furthermore,retinal ganglion cell 5(RGC5)cell proliferation was assessed with cell counting kit-8(CCK-8)assays.Serta domain-containing protein 4(Sertad4)mRNA and protein expression levels were measured by qRT-PCR and Western blot analysis,respectively.RESULTS:Proteomics analysis suggested that Sertad4 was the most significantly differentially expressed protein.Compared with the saline group,the acteoside treatment group showed decreased IOP,improved N1-P1 wave amplitudes,thicker retina,and larger numbers of cells in the ganglion cell layer(GCL).The IHC results showed that Sertad4 expression levels in DBA/2J mice treated with acteoside were significantly lower than in the saline group.Acteoside treatment could improve RGC5 cell survival and reduce the Sertad4 mRNA and protein expression levels after glutamate injury.CONCLUSION:Sertad4 is differentially expressed in DBA/2J mice.Acteoside can protect RGCs from damage,possibly through the downregulation of Sertad4,and has a potential use in glaucoma treatment.

Quantitative trait loci identification reveals zinc finger protein CONSTANS-LIKE 4 as the key candidate gene of stigma color in watermelon(Citrullus lanatus)

Stigma color is a critical agronomic trait in watermelon that plays an important role in pollination.However,there are few reports on the regulation of stigma color in watermelon.In this study,a genetic analysis of the F2 population derived from ZXG1553(P1,with orange stigma)and W1-17(P2,with yellow stigma)indicated that stigma color is a quantitative trait and the orange stigma is recessive compared with the yellow stigma.Bulk segregant analysis sequencing(BSA-seq)revealed a 3.75 Mb segment on chromosome 6 that is related to stigma color.Also,a major stable effective QTL Clqsc6.1(QTL stigma color)was detected in two years between cleaved amplified polymorphic sequencing(CAPS)markers Chr06_8338913 and Chr06_9344593 spanning a~1.01 Mb interval that harbors 51 annotated genes.Cla97C06G117020(annotated as zinc finger protein CONSTANS-LIKE 4)was identified as the best candidate gene for the stigma color trait through RNA-seq,quantitative real-time PCR(qRT-PCR),and gene structure alignment analysis among the natural watermelon panel.The expression level of Cla97C06G117020 in the orange stigma accession was lower than in the yellow stigma accessions with a significant difference.A nonsynonymous SNP site of the Cla97C06G117020 coding region that causes amino acid variation was related to the stigma color variation among nine watermelon accessions according to their re-sequencing data.Stigma color formation is often related to carotenoids,and we also found that the expression trend of ClCHYB(annotated asβ-carotene hydroxylase)in the carotenoid metabolic pathway was consistent with Cla97C06G117020,and it was expressed in low amounts in the orange stigma accession.These data indicated that Cla97C06G117020 and ClCHYB may interact to form the stigma color.This study provides a theoretical basis for gene fine mapping and mechanisms for the regulation of stigma color in watermelon.

Prognostic and immunological roles of heat shock protein A4 in lung adenocarcinoma

BACKGROUND Heat shock protein A4(HSPA4)belongs to molecular chaperone protein family which plays important roles within variable cellular activities,including cancer initiation and progression.However,the prognostic and immunological significance of HSPA4 in lung adenocarcinoma(LUAD)has not been revealed yet.AIM To explore the prognostic and immunological roles of HSPA4 to identify a novel prognostic biomarker and therapeutic target for LUAD.METHODS We assessed the prognostic and immunological significance of HSPA4 in LUAD using data from The Cancer Genome Atlas database.The association between HSPA4 expression and clinical-pathological features was assessed through Kruskal-Wallis and Wilcoxon signed-rank test.Univariate/multivariate Cox regression analyses and Kaplan-Meier curves were employed to evaluate prognostic factors,including HSPA4,in LUAD.Gene set enrichment analysis(GSEA)was conducted to identify the key signaling pathways associated with HSPA4.The correlation between HSPA4 expression and cancer immune infiltration was evaluated using single-sample gene set enrichment analysis(ssGSEA).RESULTS Overexpressing HSPA4 was significantly related to advanced pathologic TNM stage,advanced pathologic stage,progression disease status of primary therapy outcome and female subgroups with LUAD.In addition,increased HSPA4 expression was found to be related to worse disease-specific survival and overall survival.GSEA analysis indicated a significant correlation between HSPA4 and cell cycle regulation and immune response,particularly through diminishing the function of cytotoxicity cells and CD8 T cells.The ssGSEA algorithm showed a positive correlation between HSPA4 expression and infiltrating levels of Th2 cells,while a negative correlation was observed with cytotoxic cell infiltration levels.CONCLUSION Our findings indicate HSPA4 is related to prognosis and immune cell infiltrates and may act as a novel prognostic biomarker and therapeutic target for LUAD.

GATA-4在妊娠期糖尿病胎鼠心脏中的表达

目的:了解妊娠期糖尿病(gestational diabetes mellitus,GDM)胎鼠心脏发育过程中锌指转录因子GATA结合蛋白4(GATA binding protein 4,GATA-4)的变化规律,为深入探讨其在GDM胎鼠心脏发育异常中的作用机制奠定基础。方法:80只SPF级成年SD雌鼠随机分为对照组(n=40)和GDM组(n=40),通过阴道涂片确定受孕后,GDM组予腹腔注射2%链脲佐菌素(streptozotocin,STZ;每只40 mg/kg),对照组予腹腔注射等量的柠檬酸-柠檬酸钠缓冲液。给药72 h后每天监测血糖,各组分别于孕12、15、19 d剖取胎鼠心脏组织,HE染色观察心脏组织病理变化,免疫组化检测GATA-4的表达,实时荧光定量RT-PCR检测GATA-4 mRNA的表达,Western blot-ting检测GATA-4蛋白的变化。结果:对照组及GDM组GATA-4蛋白的表达呈动态变化:孕12 d可见表达,孕15 d表达最高,孕19 d表达下降;与对照组相比,GDM组GATA-4 mRNA及蛋白的表达呈现下降趋势,差异有统计学意义(P<0.05)。结论:妊娠期糖尿病胎鼠心脏发育异常率显著增高,GATA-4与GDM胎鼠心脏发育异常可能有相关性。

miRNA-330-3p/Ap2m1轴在过表达GATA-4骨髓间充质干细胞外泌体抗心肌细胞凋亡中的作用

目的探讨过表达GATA-4小鼠骨髓间充质干细胞(BMSC)分泌外泌体(BMSC^(GATA-4)exosome)通过miRNA-330-3p/Ap2m1轴减少心肌细胞凋亡,提高心肌梗死心功能。方法建立小鼠心梗模型,共分7组,分别经尾静脉注射BMSC^(miRNA-330-3p-mimic)-exosome、BMSC^(miRNA-330-3p-inhibitor)-exosome、BMSC^(空载体)-exosome、BMSCexosome 48 h,同时将心梗未处理组及正常小鼠作为对照组。采用心脏彩超检测各组心功能,RT-PCR检测心梗心肌细胞内miRNA-330-3p的表达,Tunel法检测各组心梗心肌细胞凋亡数量。miRNA-330-3p对应靶基因Ap2.m1、Cnot4蛋白采用Western blot法进行检测。结果BMSC^(miRNA-330-3p-mimic)-exosome组心梗心功能改善最为明显(P<0.05),其心肌细胞内miRNA-330-3p表达量最高(P<0.05)。BMSC^(miRNA-330-3p-mimic)-exosome组心肌细胞的凋亡率最低(P<0.05),BMSC^(miRNA-330-3p-mimic)-exosome组心梗心肌细胞内的Ap2.m1的表达最低(P<0.05)。结论过表达GATA-4小鼠骨髓间充质干细胞外泌体通过miRNA-330-3p/Ap2m1轴抗心肌细胞凋亡。

GATA-4在小鼠睾丸中的表达定位研究

目的:观察小鼠睾丸内GATA-4免疫反应产物的特征与分布。方法:选取刚出生、2、4、6周雄性B6SJLF1/J小鼠各6只,取睾丸进行石蜡切片,应用免疫组化ABC法,DAB显色,观察GATA-4在不同时期睾丸中的表达情况。结果:GATA-4免疫反应产物在以上4个阶段小鼠睾丸Sertoli细胞、Leydig细胞均有分布,且4、6周组小鼠睾丸Leydig细胞阳性率比刚出生和2周组小鼠更高(P<0.01);但4、6周组小鼠,除以上两种细胞外,生精细胞中也有分布,6周组小鼠比4周组小鼠阳性细胞率高(P<0.01)。结论:小鼠睾丸内存在GATA-4,为研究GATA-4在睾丸性别决定和分化以及激素调控方面提供了形态学依据。

叶酸缺乏对孕鼠子代心脏中GATA-4表达的影响

目的:探讨叶酸缺乏孕鼠的子代心脏发育过程中GATA-4基因和蛋白的表达改变。方法:成熟雌性SD大鼠36只随机分为实验组和对照组各18只,分别喂以缺乏叶酸和添加叶酸的纯合饲料。两周后与成熟SD雄性大鼠交配,分别取孕13.5天(E13.5d)、孕17.5天(E17.5d)胚胎的心脏及新生鼠的心脏。用RT-PCR检测GATA-4基因mRNA的表达。Western-blotting测GATA-4蛋白水平的表达。结果:GATA-4基因mRNA在E13.5d、E17.5d的胚胎心脏及新生鼠心脏中的表达量,实验组均显著低于对照组(P<0.05)。GATA-4蛋白在E13.5d、E17.5d的胚胎心脏及新生鼠心脏中的表达量,实验组均显著低于对照组(P<0.05)。结论:叶酸的缺乏影响GATA-4基因和蛋白水平的表达,可能导致心脏发生发育中形态的改变,从而造成心脏的功能缺陷。

GATA-4基因在大鼠胚胎心脏中的表达

目的:检测GATA-4基因在大鼠胚胎心脏中的蛋白表达变化。方法:取大鼠胚胎12、15、19天心脏,应用Westernblot、免疫组化的方法进行半定量、定位分析。结果:免疫组化显示,GATA-4基因在房室肌、心内膜、心内膜垫、房室瓣及大动脉根部均有表达。Western blot显示,在胚胎12天心脏中,GATA-4基因已有较高表达;在胚胎15天表达明显上调,胚胎19天时表达又有所下降。结论:GATA-4随大鼠胚胎心脏的生长发育呈动态表达,GATA-4与心脏发育密切相关。

骨髓间充质干细胞向心肌诱导过程中GATA-4和Nkx2-5基因的表达

目的观察骨髓间充质干细胞(MSCs)向心肌诱导分化过程中,心肌转录因子GATA-4和Nkx2.5基因表达的变化规律,探讨其分子生物学机理。方法体外培养大鼠骨髓间充质干细胞,取第3代以10μmol/L 5-氮杂胞苷(5-aza)诱导,分别于第1、2、3、4周收集细胞,免疫细胞化学法和Western blot法检测肌钙蛋白I(troponinI,TnI)表达,RT-PCR法分析GATA-4和Nkx2.5基因的表达。结果诱导后细胞停止生长,并倾向集落化,诱导第2周开始出现TnI阳性细胞,第1周开始即有GATA-4和Nkx2.5基因表达,逐渐增强,第3周达到高峰,持续到第4周。结论GATA-4和Nkx2.5基因表达在骨髓间充质干细胞向心肌样细胞诱导过程中逐渐增强,可能参与调控心肌细胞的分化过程。

转录因子T-bet、GATA-3、FoxP3及CD4~＋CD25~＋调节性T细胞在儿童过敏性紫癜发病机制中的作用

本研究旨在探讨转录因子T-bet、GATA-3和CD4+CD25+调节性T细胞及其转录因子FoxP3在儿童过敏性紫癜(HSP)发病机制中的作用。2009年2月-2010年2月在本院收治的46例急性期HSP患儿(HSP组)及30例健康对照儿童(对照组)纳入研究。采用SYBR GreenⅠ实时荧光定量PCR方法检测外周血单个核细胞T-bet、GATA-3及FoxP3 mRNA的表达。运用流式细胞术检测外周血中T淋巴细胞亚群CD4+CD25+的表达。结果表明,HSP组患儿GATA-3 mRNA相对表达水平(964.30±655.18)显著高于对照组儿童GATA-3 mRNA相对表达水平(78.09±57.20,P<0.01)。HSP组患儿T-bet mRNA(53.98±35.79)、FoxP3 mRNA(32.17±23.04)和CD4+CD25+(5.34±2.51)相对表达水平低于对照组儿童T-bet mRNA(181.56±96.90)、FoxP3 mRNA(147.91±99.15)和CD4+CD25+(7.85±1.97)相对表达水平(P<0.01)。结论:HSP患儿急性期存在Th1特异性转录因子T-betmRNA表达下调,Th2特异性转录因子GATA-3 mRNA表达上调。HSP患儿急性期存在CD4+CD25+调节性T细胞及其特异性转录因子FoxP3 mRNA表达下调,调节性T细胞的减少及由此引发的免疫抑制效应不足可能是HSP急性期免疫失衡的重要原因之一。本研究为从调节性T细胞及其调控的分子机制角度进一步阐明儿童HSP的发病机制提供了实验依据。

转录因子GATA-3在变应性鼻炎患者白细胞介素4和白细胞介素5表达中的作用

目的 探讨变应性鼻炎患者转录因子GATA-3和白细胞介素4(IL-4)、IL-5的表达及关系。方法 通过免疫组化、逆转录多聚酶链反应(RT-PCR)和酶联免疫吸附试验,检测23例变应性鼻炎患者和11例对照鼻黏膜组织中GATA-3和IL4、IL-5的表达。结果 23例变应性鼻炎患者鼻黏膜组织中20例GATA-3免疫组化染色呈阳性,占86.9％;PCR反应后变应性鼻炎患者和对照鼻黏膜组织中GATA-3相对密度分别为0.602±0.117和0.134±0.025;IL-4和IL-5的含量分别为(135.5±66.4)pg/mg和(77.5±29.4)pg/mg。GATA-3与IL-4、IL-5的表达呈正相关关系(r=0.45和0.62,P均<0.05)。结论 变应性鼻炎患者鼻黏膜GATA-3表达增高与IL-4、IL-5的上调有关。

GATA-4 M310V单基因突变参与家族性房间隔缺损的机制研究

目的:在以往发现家族性先天性房间隔缺损GATA-4 M310V单基因突变的基础上,本研究进一步探讨该突变导致家族性房间隔缺损的可能机制。方法:选取一个先天性房间隔缺损家族(三级亲属成员共31人中有8例单纯性房间隔缺损患者),采集外周血样,采集少量心肌组织标本。体外成功构建GATA-4基因野生型及突变型真核表达载体并转染细胞系,按照不同载体组合(16种组合)转染Hela细胞,应用双荧光素酶报告系统检测GATA-4基因突变对心脏肌球蛋白重链-α(α-Myhc)、心房利钠肽因子(ANF)启动子活性的影响。应用绿色荧光蛋白定位法检测GATA-4 M310V突变对GATA4蛋白核定位的影响。结果:双荧光素酶检测结果:对于α-Myhc启动子,引入GATA-4基因表达载体后,随着GATA-4表达载体浓度的上升,其启动子活性呈现上升趋势,差异有统计学意义(P<0.005);引入GATA-4(A928G)突变基因表达载体后,相同GATA-4表达载体转染剂量(100 ng、200 ng)调控的启动子活性增强,差异有统计学意义(P<0.005);但随GATA-4突变型表达载体引入量的增加(300 ng),启动子活性似乎有下降趋势,差异无统计学意义(P=0.195)。对于ANF启动子,引入GATA-4基因表达载体、GATA-4突变基因表达载体后,启动子活性变化组间差异及趋势变化并不明显(P>0.05)。结论:GATA-4 M310V突变影响了α-Myhc启动子活性及GATA4蛋白的核定位,该突变对GATA4蛋白核定位的影响可能是该突变导致家族性房间隔缺损新的重要分子生物学机制。

过表达GATA-4骨髓间充质干细胞分泌的外泌体促进骨髓间充质干细胞向心肌样细胞分化

背景:前期证明,过表达心脏基因转录因子GATA-4小鼠骨髓间充质干细胞分泌的外泌体(BMSCs GATA-4-exosome)可以促进BMSCs向心肌样细胞分化,提示其可以修复心肌梗死,另外还发现BMSCs GATA-4-exosome中及心肌梗死局部心肌组织中有miRNA-673-5p明显高表达且功能涉及细胞分化,可能是BMSCs GATA-4-exosome修复心肌梗死的关键分子。目的:探讨BMSCs GATA-4-exosome促进BMSCs向心肌样细胞分化的分子调控网络。方法:在小鼠BMSCs培养体系内加入miRNA-673-5p模拟物(miR-673-5p-mimic)作为实验组(BMSCs miR-673-5p-mimic),将BMSCs GATA-4组、BMSCs GATA-4-空载体组、BMSCs组、BMSCs miR-673-5p-inhibitor组作为混杂因素对照组,提取各组分泌的外泌体与BMSCs直接共培养24 h,采用免疫荧光定性检测和RT-PCR定量检测各组BMSCs中心肌特异性分子α-actin、Desmin、cTnT、Cx43的表达。根据microRNA靶基因预测结果,采用Western blot检测miRNA-673-5p对应靶基因TSC-1、ERK1/2及Mef2c转录蛋白表达。结果与结论:BMSCs miR-673-5p-mimic-exosome+BMSCs组荧光强度最强,心肌细胞特异性分子α-actin、Desmin、cTnT、Cx43的表达最高(P<0.05),TSC-1的表达最低(P<0.05)。结果表明BMSCs GATA-4-exosome通过miRNA-673-5p抑制TSC-1蛋白表达促进BMSCs向心肌样细胞分化。

GATA-4过表达增加大鼠骨髓间充质干细胞分化为心肌细胞

目的研究GATA-4转染骨髓间充质干细胞(MSCs)分化为心肌细胞及表达心肌细胞特异性标志物的能力。方法分离培养MSCs及心肌细胞(CM)。第3代MSCs转染GATA-4基因(MSCGATA-4)并通过实时定量聚合酶链反应(PCR)、Western blot和免疫组化鉴定GATA-4的表达。MSCGATA-4与CM嵌套式共培养1周,通过real-time PCR和Western blot检测其心肌基因BNP、α-actinin和Islet-1的表达,用免疫组化观察α-actinin的表达。与CM混合共培养后1周后,观察MSCs的搏动情况,并用流式细胞仪检测心肌分化率。结果 MSCGATA-4组GATA-4的表达明显高于对照组(只表达GFP)。MSC与CM嵌套式共培养后,MSCGATA-4组的BNP、α-actinin和Islet-1的mRNA和蛋白表达明显高于对照组(P<0.05)。混合共培养后,可见部分MSCGATA-4的搏动,同时部分MSC的α-actinin染色阳性。用流式细胞仪检测心肌分化率,MSCGATA-4组的心肌分化率明显高于对照组(P<0.05)。结论 GATA-4过表达可以增加MSCs分化成心肌样细胞,高表达BNP、α-actinin和Islet-1。

转录因子GATA-4在心肌分化、肥厚及凋亡中的作用

锌指结构家族成员GATA-4作为一种特定的细胞核转录因子,涉及基因调节的不同环节,控制着基因的表达和功能的调节,正日益受到高度重视。该文系统阐述了GATA-4因子的结构、表达及其在心脏发育、心肌肥厚和抗心肌细胞凋亡方面的作用。

T-bet、GATA-3、FoxP3及CD_4^+CD_(25)^+调节性T细胞在AA发病机制中的作用

目的探讨转录因子T-bet、GATA-3和CD+4CD+25调节性T细胞及其转录因子FoxP3在再生障碍性贫血(AA)发病机制中的作用。方法选择AA患者27例(AA组)、体检健康者25例(对照组),采用RT-PCR技术检测两组外周血单个核细胞(PBMCs)中Th1、Th2细胞及CD4+CD2+5调节性T细胞特异性转录因子T-bet、GATA-3、FoxP3 mR-NA的表达,运用流式细胞术检测外周血中T淋巴细胞亚群,ELISA法检测血浆中Th1和Th2类细胞因子IFN-γ、IL-4水平。结果与对照组相比,AA组的血浆T-bet mRNA相对表达量升高(P<0.01),GATA-3与FoxP3 mRNA相对表达量降低(P<0.05,P<0.01);AA组外周血中CD+3、CD+3CD+8T细胞占淋巴细胞的百分比较对照组升高(P均<0.05),CD+3CD+4、CD+4CD+25T细胞占淋巴细胞的百分比和CD+4/CD+8值较对照组降低(P<0.05或P<0.01);AA组血浆中IFN-γ水平及IFN-γ/IL-4高于对照组(P均<0.01)。结论 AA患者存在CD+4CD+25调节性T细胞及其特异性转录因子FoxP3 mRNA表达下调,调节性T细胞的减少及由此引起免疫抑制效应不足可能是AA发生的重要原因之一。

NKx2.5、GATA-4基因表达对骨髓间充质干细胞分化为心肌细胞的影响

观察NKx2.5、GATA-4基因在骨髓间充质干细胞 (mesenchymalstemcells,MSCs)分化为心肌细胞过程中表达时序性及表达强度的变化 ,初步阐明两基因对MSCs分化为心肌细胞的影响。以MSCs植入后的Wistar大鼠为研究对象 ,在移植后不同的时间点取心肌标本 ,采用逆转录聚合酶链反应技术 ,提取心肌组织的总RNA ,逆转录 ,加入特异性引物扩增目的基因 ,观察基因表达的时序性 ,并应用凝胶图像分析系统检测这两个基因表达强度的动态变化。显示在MSCs移植后 1d两个基因即出现弱的表达 ,1d～ 1周表达较低 ,2周～ 3周表达强度最高 ,达到高峰期 ,以后表达强度则逐渐降低。NKx2.5、GATA

转录因子Nkx2.5和GATA-4在心脏发育中的作用

转录因子是能直接或间接辨认和结合转录上游区段DNA的蛋白质。Nkx2.5和GATA-4是两个与心脏发育密切相关的转录因子。Nkx2.5参与了心脏形成,包括右侧环化、心腔分化、心脏间隔功能成熟以及工作心肌和传导系统的维持等过程。GATA-4在心肌分化增殖和存活及心脏肥大过程中起重要作用。Nkx2.5和GATA-4在蛋白质水平相互作用,调节心房利钠肽、骨形态发生蛋白和心脏限制性锚蛋白复制蛋白等启动子的表达。