RAD51C表达下调对小鼠卵巢癌体内成瘤和VEGF、NRP-2表达的调控

目的探讨RAD51旁系同源基因C(RAD51C)表达下调对小鼠卵巢癌体内成瘤和血管内皮生长因子(VEGF)、神经纤毛蛋白-2(NRP-2)表达调控的影响。方法使用A2780卵巢癌细胞,通过培养检测细胞中RAD51C的表达,构建3种RAD51C干扰载体(SiRNA-47、SiRNA-183和SiRNA-285),并包装成慢病毒,转染细胞,逆转录实时定量聚合酶链式反应(RT-qPCR)验证转染效果,进行稳筛,构建稳转细胞株。使用Balb/c雌性裸鼠建立细胞系来源的异体移植肿瘤模型(CDX)模型,将18只建模成功的裸鼠分为3组:A2780细胞组(Control组)、A2780细胞+空载体对照组(NC组)、A2780细胞+RAD51C干扰组(Si-RAD51C组),每组各6只。Control组注射生理盐水,NC组注射空载慢病毒50μL,Si-RAD51C组注射RAD51C干扰慢病毒50μL。观察各组成瘤情况,取肿瘤组织,采用蛋白质印迹法(WB)、免疫组织化学检测RAD51C、VEGF、NRP-2蛋白表达情况。结果RT-qPCR验证RAD51C干扰慢病毒转染效果以SiRAN-285最明显(P<0.05)。Si-RAD51C组与Control组、NC组比较瘤体的体积最小、重量也最轻,且RAD51C、NRP-2及VEGF蛋白的表达显著降低(P<0.05)。结论RAD51C干扰慢病毒可抑制小鼠A2780卵巢癌细胞肿瘤的形成,且对RAD51C、NRP-2及VEGF蛋白的表达均有抑制作用。

CRP水平及其基因多态性与2型糖尿病的相关性

目的探讨C反应蛋白(CRP)水平及其基因多态性、外周血炎症标志物与2型糖尿病(T2DM)的相关性。方法2021年10月1日至2022年9月30日南方医科大学第十附属医院内分泌科100例T2DM患者为T2DM组,100例同期健康人群为对照组,收集两组抗凝血标本,采用PCR反应和测序技术确定CRP基因rs2794521(CRP-717A/G)位点基因型分布,通过收集患者临床资料,分析CRP及其基因多态性与中性粒细胞/淋巴细胞比值(NLR)、血小板淋巴细胞比值(PLR)、单核细胞/淋巴细胞比值(MLR)、衍生中性粒细胞/淋巴细胞比值(dNLR)、系统免疫炎症指数(SII)与T2DM的相关性。结果T2DM组AA基因频率显著高于对照组(P<0.05)。与A/G+G/G基因型比较,A/A基因型携带者CRP值增高(P<0.05)。不同基因型间其他临床指标比较,差异无统计学意义(P>0.05)。Pearson相关性分析发现,CRP水平与体质指数(BMI)、PLR、MLR和SII呈正相关(P<0.05)。两组受试对象性别、总胆固醇(TCH)、MLR等基本资料比较,差异无统计学意义(P>0.05),两组年龄、BMI、TG、NLR、PLR、dNLR、SII和CRP比较,差异有统计学意义(P<0.05)。多因素logistic回归分析结果显示TG(OR=1.945)、NLR(OR=2.022)、SII(OR=7.312)、PLR(OR=1.512)、dNLR(OR=2.121)、CRP(OR=10.126)、CRP-A/A(OR=2.132)是T2DM的危险因素(P<0.05)。结论CRP基因A/A多态性可能是T2DM的遗传危险因素;此基因型携带者具有较高的CRP水平;TG、NLR、SII、PLR、dNLR、CRP升高是T2DM的危险因素;CRP水平与BMI、NLR、SII、PLR、dNLR呈正相关。

基于快速CYP2C19基因检测的颈内动脉重度狭窄患者双联抗血小板治疗1例报道

本文报道了一例老年女性院内卒中患者的临床诊疗过程。该患者于肛肠外科手术后2 d突发急性缺血性卒中,经影像学检查确诊为右侧颈内动脉起始部重度狭窄。在接受了1个月的卒中二级预防药物治疗后,择期行血管内治疗。术前该患者进行了快速细胞色素P450酶家族2亚家族C成员19(cytochrome P450 family 2 subfamily C member 19,CYP2C19)基因检测,结果为中间代谢型,提示应用氯吡格雷的效果可能不佳。基于这一检测结果调整抗血小板治疗方案,选择替格瑞洛联合阿司匹林作为替代治疗。治疗后,患者病情稳定,预后较好。本病例报道提示,在非轻型卒中患者中,快速CYP2C19基因检测可帮助选择抗血小板治疗策略,改善患者预后。

血清sST2、CRP及S1P在冠状动脉临界病变患者中的水平及其临床意义

目的:探究血清可溶性生长刺激表达基因2蛋白(sST2)、C反应蛋白(CRP)以及1–磷酸鞘氨醇(S1P)在冠状动脉临界病变患者中的水平及其临床意义。方法:选择2021年7月至2023年7月在河南大学第一附属医院确诊为冠状动脉临界病变的90例患者为观察组,另取同期心电图存在明确缺血性病变,但经冠状动脉造影示无狭窄的90例患者为对照组,比较两组患者血清sST2、CRP及S1P水平差异,采用相关性分析探究观察组患者血清sST2、CRP、S1P水平与其Gensini评分关联。并将观察组患者按照是否出现功能性心肌缺血区分亚组,并分析其危险因素。结果:观察组患者血清sST2、CRP及S1P水平均显著高于对照组,差异具有统计学意义(P<0.05)。观察组患者的血清sST2、CRP及S1P水平与其Gensini评分均呈正相关(r=0.3811,r=0.3788,r=0.6162,P均<0.001);观察组中缺血亚组患者血清sST2、CRP、S1P水平显著高于无缺血亚组,差异具有统计学意义(P<0.05);多因素Logistic回归分析显示,血清sST2、CRP、S1P水平是冠状动脉病变患者心肌缺血独立危险因素(P<0.05)。结论:冠状动脉临界病变患者血清sST2、CRP、S1P水平有异常升高,与患者的冠状动脉血管病变狭窄程度相关,且血清sST2、CRP、S1P水平异常升高是冠状动脉临界病变患者功能性心肌缺血的独立危险因素。

超声波辅助法合成离子液体[C2OHmim]BF4及其双水相体系的研究

采用超声波辅助法合成了N-(2-羟乙基)-3-甲基咪唑四氟硼酸盐([C2OHmim]BF4),产率达57.69%,并建立了[C2OHmim]BF4和无机盐形成的离子液体双水相体系。结果表明,盐的种类和浓度对体系的形成影响很大,(NH4)2SO4能与[C2OHmim]BF4水溶液形成双水相体系。在2 mL[C2OHmim]BF4与3 mL水的混合溶液中加入0.750 0 g(NH4)2SO4后,能形成稳定的双水相且相比达0.923,接近于1;在pH=6～9时,溶液酸度对体系相比的影响较小;在不同温度下体系的热稳定性较好,受温度影响不大;离子液体可再利用。

广东汉族人群补体C_2,Bf、C_4的遗传多态现象

对110例广东汉族人血清作了补体 C2、Bf、C4的测定,它们的基因频率分别为:C2*C:0.9500,C2*Q0:0.009,C2*B:0.0227,C2*A:0.0182;Bf*S:0.8364,Bf*F:0.1409,Bf*S07:0.0091,Bf*S025:0.0091,Bf*S055:0.0045;C4A*5:0.0255,4:0.1327,3:0.6327,2:0.0918,1:0.0053,Q5:0.1020;C4B*5:0.0152,3:0.0102,2:0.4416,1:0.4569,92:0.0051,96:0.0152,Q0:0.0558。本调查在我国首次发现一例 C2Q0纯合子。本结果与湖北汉族人群的结果分别进行了比较。

团头鲂补体因子Bf/C2的克隆和表达分析

为探索团头鲂(Megalobrama amblycephala)补体因子Bf和C2(complement factor B/C2,Bf/C2)的可能功能,在转录组数据基础上,采用RT-PCR克隆得到Bf/C2A和Bf/C2B基因的cDNA序列;采用荧光实时定量PCR技术检测了两基因在团头鲂早期发育过程、健康成鱼及感染嗜水气单胞菌后各组织中的表达变化。结果显示,Bf/C2AcDNA全长2 520bp,包含5′UTR 42bp、ORF 2 298bp、3′UTR 180bp,编码765个氨基酸。Bf/C2B基因ORF全长2 130bp,编码710个氨基酸。两基因的氨基酸序列分别与鲤B/C2-A2及草鱼Bf/C2B相似性最高。在早期发育阶段Bf/C2A和Bf/C2B均在在出膜后1d表达量最高,肠管形成期次之,其他时期的表达量相对较低;两基因在健康成鱼10个组织中均有表达,肝脏中表达量最高,肾脏、头肾、脾脏次之,其他组织表达量相对较低;在嗜水气单胞菌感染后,两基因在免疫相关组织如肝脏和脾脏中的表达均显著上升。上述结果表明Bf/C2在应对细菌感染的免疫过程中发挥着重要的作用。

Cu(BF_4)_2,Cu(C_3H_7COO)_2与双(二苯膦基)烷烃配体形成配位化合物的红外光谱

用红外光谱法对二苯基膦系列配体及其分别与Cu(BF_4)_2和Cu(C_3H_7COO)_2。形成的系列配位化合物进行了研究,讨论了谱带的归属和Cu(Ⅰ)配合物形成前后相关谱带的变化规律,并参照元素分析、X-射线粉末衍射分析和热重分析的结果,讨论了所形成配位化合物的可能的结构模式。

Study of differential polymerase chain reaction of C-erbB-2 oncogene amplification in gastric cancer

AIM To study the significance of C-erbB-2 oncogene amplification in gastric cancer.METHODS C-erbB-2 oncogene amplification was examined by using differential polymerase chain reaction (dPCR) in surgical and endoscopic specimens of 83 cases of gastric cancer and 101 metastatic lymph nodes.RESULTS C-erbB-2 amplification was found in 28.9% (24/ 83) surgical specimens and 20.5% (17/ 83) endoscopic ones of gastric cancer patients. The amplification was significant in both types of specimens of advanced cancer cases (P＜0.05) and surgical specimens with lymph node metastasis (P＜0.01). The incidence of C-erbB-2 amplification in lymph nodes with metastasis was higher than in primary sites (surgical specimens, P＜0.05). The patients with amplification tumors had poorer 5-year survival rates than those with unamplification ones in the early cancers and well to moderately differentiated adenocarcinomas (P＜0.05). The same surgical samples were tested again by Southern blot hybridization to ascertain C-erbB-2 amplification, and the positive rate of C-erbB-2 amplification (15.7%) was lower than that of dPCR (28.9%, P＜0.05).CONCLUSION Examining C-erbB-2 amplification by dPCR is a quick, simple, reliable and independent method, and is helpful in predicting prognosis and metastatic potential of gastric cancer.

血清脑钠肽、高敏C反应蛋白、可溶性生长刺激表达基因2在阵发性心房颤动患者射频消融术后复发中的预测价值

目的分析研究血清脑钠肽(BNP)、高敏C反应蛋白(hs-CRP)、可溶性生长刺激表达基因2(sST2)在阵发性心房颤动(PaAF)患者射频消融术后复发中的预测价值。方法选取2020年1月—2022年1月张家口市第一医院心内四科收治的96例PaAF患者作为研究对象,均进行射频消融术治疗,术后对患者进行1年随访,根据有无房颤复发将患者分为复发组(n=24)与未复发组(n=72)。比较2组的血清BNP、hs-CRP与sST2水平;收集2组患者的临床资料,采用多因素Logistic回归分析PaAF患者射频消融术后房颤复发的影响因素,并绘制受试者工作特征(ROC)曲线,分析血清BNP、hs-CRP与sST2水平对PaAF患者射频消融术后房颤复发的预测价值。结果复发组PaAF患者的血清BNP、hs-CRP与sST2水平均显著高于未复发组,差异均具有统计学意义(t/P=14.916/<0.001、11.974/<0.001、7.229/<0.001);多因素Logistic回归分析显示,有冠心病史、BNP水平升高、hs-CRP水平升高及sST2水平升高均是PaAF患者射频消融术后房颤复发的独立危险因素[OR(95%CI)=1.718(1.200~2.459)、1.891(1.214~2.945)、2.104(1.237~3.579)、1.902(1.243~2.910)];ROC曲线分析显示,血清BNP、hs-CRP与sST2水平及联合检测评估PaAF患者射频消融术后房颤复发的曲线下面积(AUC)分别为0.975、0.965、0.870、0.989,联合检测优于单一检测(Z=2.027、2.309、3.001,均P<0.05)。结论血清BNP、hs-CRP、sST2在PaAF患者射频消融术后复发中呈高表达,对PaAF患者射频消融术后房颤复发具有一定的预测价值。

Time serial transcriptome reveals Cyp2c29 as a key gene in hepatocellular carcinoma development

Objective:Hepatocellular carcinoma(HCC)is a severely lethal cancer that usually originates from chronic liver injury and inflammation.Although progress on diagnosis and treatment is obvious,the cause of HCC remains unclear.In this study,we sought to determine key genes in HCC development.Methods:To identify key regulators during HCC progression,we performed transcriptome sequencing to obtain time series gene expression data from a mouse model with diethylnitrosamine-induced liver tumors and further verified gene expression and function in vitro and in vivo.Results:Among the differentially expressed genes,Cyp2c29 was continuously downregulated during HCC progression.Overexpression of Cyp2c29 suppressed N F-kB activation and proinflammatory cytokine production by increasing the production o f 14,15-epoxyeicosatrienoic acid in vitro.Furthermore,overexpression of Cyp2c29 in vivo protected against liver inflammation in mouse models of liver injury induced by both acetaminophen and CC14.Two human homologs of mouse Cyp2c29,CYP2C8 and CYP2C9,were found to be downregulated in human HCC progression,and their expression was positively correlated with overall survival in patients with HCC(significance:P=0.046 and 0.0097,respectively).Conclusions:Collectively,through systematic analysis and verification,we determined that C yp2c29 is a novel gene involved in liver injury and inflammation,which may be a potential biomarker for HCC prevention and prognosis determination.

HepG2 cells support viral replication and gene expression of hepatitis C virus genotype 4 in vitro

AIM： TO establish a cell culture system with longterm replication of hepatitis C virus （HCV） genome and expression of viral antigens in vitro. METHODS： HepG2 cell line was tested for its susceptibility to HCV by incubation with a serum from a patient with chronic hepatitis C. Cells and supernatant were harvested at various time points during the culture. Culture supernatant was tested for its ability to infect na＇ive cells. The presence of minus （antisense） RNA strand, and the detection of core and E1 antigens in cells were examined by RT-PCR and immunological techniques （flow cytometry and Western blot） respectively. RESULTS： The intracellular HCV RNA was first detected on d 3 after infection and then could be consistently detected in both cells and supernatant over a period of at least three months. The fresh cells could be infected with supernatant from cultured infected cells. Flow cytometric analysis showed surface and intracellular HCV antigen expression using in house made polyclonal antibodies （anti-core, and anti-E1）. Western blot analysis showed the expression of a cluster of immunogenic peptides at molecular weights extended between 31 and 45 kDa in an one month old culture of infected cells whereas this cluster was undetectable in uninfected HepG2 cells. CONCLUSION： HepG2 cell line is not only susceptible to HCV infection but also supports its replication in vitro. Expression of HCV structural proteins can be detected in infected HepG2 cells. These cells are also capable of shedding viral particles into culture media which in turn become infectious to uninfected cells.

The 5-HT2c receptor gene Cys23Ser polymorphism influences the intravaginal ejaculation latency time in Dutch Caucasian men with lifelong premature ejaculation

It has been postulated that the persistent short intravaginal ejaculation latency time （IELT） of men with lifelong premature ejaculation （LPE） is related to 5-hydroxytryptamine （HT）2c receptor functioning. The aim of this study was to investigate the relationship of Cys23Ser 5-HT2c receptor gene polymorphism and the duration of IELT in men with LPE. Therefore, a prospective study was conducted in 64 Dutch Caucasian men with LPE. Baseline IELT during coitus was assessed by stopwatch over a 1-month period. All men were genotyped for Cys23Ser 5-HT2c receptor gene polymorphism. Allele frequencies and genotypes of Cys and Ser variants of 5-HT2c receptor gene polymorphism were determined. Association between Cys/Cys and Ser/Ser genotypes and the natural logarithm of the IELT in men with LPE were.investigated. As a result, the geometric mean, median and natural mean IELT were 25.2, 27.0, 33.9s, respectively. Of all men, 20.0%, 10.8%, 23.1% and 41.5% ejaculated within 10, 10-20, 20-30 and 30-60s after vaginal penetration. Of the 64 men, the Cys/Cys and Ser/Ser genotype frequency for the Cys23Ser polymorphism of the 5-HT2c receptor gene was 81% and 19%, respectively. The geometric mean IELT of the wildtypes （Cys/Cys） is significantly lower （22.6s; 95% CI 18.3-27.8s） than in male homozygous mutants （Ser/Ser） （40.4s; 95% CI 20.3-80.4s） （P = 0.03）. It is concluded that Cys23Ser 5-HT2c receptor gene polymorphism is associated with the IELT in men with LPE. Men with Cys/Cys genotype have shorter IELTs than men with Ser/Ser genotypes.

Development of "Multi-Resistance Rice" by Pyramiding of Insect (Cry1C) and Blast Resistance (Pi1 and Pi2) Genes

[Objective] The paper was to improve the blast resistance of insect-resistant transgenic rice. [Method] The Japonica rice variety Jikang10, a new transgenic variety with exogenous insect-resistant gene Cry1C, was used as the receptor, and Kongyu 131, a traditional breeding variety with broad-spectrum high blast resistance genes Pi1 and Pi2, was used as the donor to breeding new rice varieties. The genes were polymerized by hybridization and multi-generation backcrossing, and the offspring of each generation was screened by molecular marker assisted selection, field identification of multi-resistance against insect pests and diseases and agronomic trait selection. [Result] Four lines SK01, SK02, SK03 and SK04 with better resistances to insect pests and blast and outstanding agronomic traits in field were selected. [Conclusion] The results will lay foundations for breeding new multi-resistance rice varieties in Huanghuai rice region.

The heterodimeric structure of heterogeneous nuclear ribonucleoprotein C1/C2 dictates 1,25-dihydroxyvitamin D-directed transcriptional events in osteoblasts

Heterogeneous nuclear ribonucleoprotein （hnRNP） C plays a key role in RNA processing but also exerts a dominant negative effect on responses to 1,25-dihydroxyvitamin D （1,25（OH）2D） by functioning as a vitamin D response element-binding protein （VDRE-BP）. hnRNPC acts a tetramer of hnRNPC1 （huC1） and hnRNPC2 （huC2）, and organization of these subunits is critical to in vivo nucleic acid-binding. Overexpression of either huC1 or huC2 in human osteoblasts is sufficient to confer VDRE-BP suppression of 1,25（OH）2D-mediated transcription. However, huC1 or huC2 alone did not suppress 1,25（OH）2D-induced transcription in mouse osteoblastic cells. By contrast, overexpression of huC1 and huC2 in combination or transfection with a bone-specific polycistronic vector using a ＂self-cleaving＂ 2A peptide to co-express huC1/C2 suppressed 1,25D-mediated induction of osteoblast target gene expression. Structural diversity of hnRNPC between human/NWPs and mouse/rat/rabbit/dog was investigated by analysis of sequence variations within the hnRNP CLZ domain. The predicted loss of distal helical function in hnRNPC from lower species provides an explanation for the altered interaction between huC1/C2 and their mouse counterparts. These data provide new evidence of a role for hnRNPC1/C2 in 1,25（OH）2D-driven gene expression, and further suggest that species-specific tetramerization is a crucial determinant of its actions as a regulator of VDR-directed transactivation.

血清可溶性生长刺激表达基因2蛋白联合中性粒细胞、C反应蛋白检测对预测慢性阻塞性肺疾病急性加重期患者不良预后的临床价值

目的 探讨血清可溶性生长刺激表达基因2蛋白(sST2)联合中性粒细胞数(NEU)、C反应蛋白(CRP)检测对预测慢性阻塞性肺疾病急性加重期(AECOPD)患者不良预后的临床价值。方法 选择2022年5—8月本院收治的100例慢性阻塞性肺疾病(COPD)患者为研究对象,其中70例为COPD急性加重期,30例为COPD稳定期,选择同期体检且年龄和性别相匹配的健康体检者30例为对照组。采用方差分析比较不同组间sST2、NEU、CRP的水平;Spearman分析sST2、NEU、CRP与AECOPD临床分级的相关性;记录AECOPD患者出院后6个月内不良事件的发生情况,通过受试者工作特征(ROC)曲线评估sST2、NEU、CRP检测对AECOPD患者不良预后的预测效能,Cox回归分析AECOPD患者不良预后的相关风险因素。结果 AECOPD组sST2、NEU、CRP水平高于COPD稳定组和对照组,COPD稳定组sST2、NEU、CRP水平高于对照组(P<0.05);sST2、NEU、CRP水平随AECOPD患者临床分级的增加而升高,与AECOPD临床分级呈正相关,差异均有统计学意义(P<0.01);sST2、NEU、CRP对AECOPD患者6个月发生不良预后有较高的预测价值(AUCROC=0.861、0.674、0.729,P<0.05),最佳截断点分别为108.30 ng/mL、8.94×10^(9)/L、72.90 mg/L,且三项联合检测的预测价值最高(AUCROC=0.907,敏感性为95.5%,P<0.05);sST2>108.30ng/mL是AECOPD患者出院后6个月内发生不良预后的独立风险因素。结论 血清sST2、NEU、CRP可反映AECOPD病情严重程度,联合检测对预测AECOPD不良预后具有一定的临床价值。

Detection of ATP2C1 Gene Mutation in Familial Benign Chronic Pemphigus

Summary： The ATP2C1 gene mutation in one ease of familial benign chronic pemphigus was investigated.One patient was diagnosed as familial benign chronic pemphigus by pathology, ultrastructral examination and clinical features. Genomic DNA was extracted from blood samples. Mutation of ATP2CI gene was detected by polymerase chain reaction （PCR） and DNA sequencing. The results showed that deletion mutation was detected in ATP2C1 gene in this patient, which was 2374delTTTG. No mutation was found in the family members and normal individuals. It was coneluded that the 2374delTTTG mutation in ATP2C1 gene was the specific mutation for the clinical phenotype for this patient and was a de novo mutation.

二代基因测序技术检测急性髓系白血病患者CRLF2、FLT3及C-KIT突变的价值

目的探讨二代基因测序技术检测急性髓系白血病患者细胞因子受体样因子2(CRLF2)、FMS样酪氨酸激酶3(FLT3)及C-KIT突变的价值。方法选择2017年1月至2020年1月在我院接受治疗的78例急性髓系白血病患者为研究对象,采用二代基因测序技术检测CRLF2、FLT3及C-KIT突变情况。比较CRLF2、FLT3及C-KIT不同突变类型患者的临床参数;比较CRLF2、FLT3及C-KIT不同突变类型患者治疗≤2个疗程的完全缓解率和复发率。结果78例患者中CRLF2突变11例,突变率为14.10%,正常核型突变率高于异常核型,差异具有统计学意义(P<0.05);FLT3突变9例,突变率为11.54%,正常核型突变率高于异常核型,差异具有统计学意义(P<0.05);C-KIT突变6例,突变率为7.69%,正常核型突变率低于异常核型,差异具有统计学意义(P<0.05)。CRLF2不同突变类型患者的年龄、白细胞计数、血小板计数比较,差异具有统计学意义(P<0.05);FLT3不同突变类型患者的白细胞计数比较,差异具有统计学意义(P<0.05);C-KIT不同突变类型患者的血红蛋白水平比较,差异具有统计学意义(P<0.05)。开展随访跟踪共计76例患者可评价干预效果,CRLF2不同突变类型患者治疗≤2个疗程的完全缓解率和复发率比较,差异无统计学意义(P>0.05);FLT3突变阳性患者治疗≤2个疗程的完全缓解率低于突变阴性患者,复发率高于突变阴性患者,差异具有统计学意义(P<0.05);C-KIT不同突变类型患者治疗≤2个疗程的完全缓解率比较,差异无统计学意义(P>0.05);C-KIT突变阳性患者复发率高于突变阴性患者,差异具有统计学意义(P<0.05)。结论急性髓系白血病患者CRLF2、FLT3及C-KIT突变较为常见,利用二代基因测序技术开展上述基因突变检测有助于指导临床治疗及预后评估。

Specific activation of 2'-5'oligoadenylate synthetase gene promoter by hepatitis C virus-core protein:A potential for developing hepatitis C virus targeting gene therapy

AIM： TO examine whether 2＇-5＇oligoadenylate synthetase （OAS） gene promoter can be specifically activated by hepatitis C virus （HCV）-core protein. METHODS： Human embryo hepatic cell line L02 was transfected with pcDNA3.1-core plasmid and selected by G418. Expression of HCV-core was detected by reverse transcription polymerase chain reaction and Western blotting. The OAS promoter sequence was amplified from the genomic DNA and inserted into pGL3-basic vector. The resultant pGL3-OAS-Luci plasmid was transiently transfected into L02/core cells and luciferase activity was assayed. I^ESULTS： L02/core cell line stably expressing HCV- core protein was established. The pGL3-OAS-Luci construct exhibited significant transcriptional activity in the L02/core cells but not in the L02 cells. CONCLUSION： HCV-core protein activates the OAS gene promoter specifically and effectively. Utilization of OAS gene promoter would be an ideal strategy for developing HCV-specific gene therapy.