Precore/basal core promoter mutants and hepatitis B viral DNA levels as predictors for liver deaths and hepatocellular carcinoma

AIM: To conduct a retrospective study in 400 chronic hepatitis B patients in order to identify hepatitis B viral factors associated with complications of liver disease or development of hepatocellular carcinoma.METHODS: The mean follow-up time was 83.6 ± 39.6 mo. Alpha-fetoprotein test and abdominal ultrasound were used for cancer surveillance. Hepatitis B basal core promoter mutants, precore mutants, genotypes, hepatitis B viral DNA (HBV DNA) level and hepatitis B e antigen (HBeAg) were measured. Univariate analysis and logistic regression were used to assess odds ratios for viral factors related to liver deaths and hepatocellular carcinoma development. RESULTS: During follow-up, 38 patients had liver deaths not related to hepatocellular carcinoma. On multivariate analysis, older age [odds ratio: 95.74 (12.13-891.31); P < 0.0001], male sex [odds ratio: 7.61 (2.20-47.95); P = 0.006], and higher log10 HBV DNA [odds ratio: 4.69 (1.16-20.43); P < 0.0001] were independently predictive for these liver related deaths. Also, 31 patients developed hepatocellular carcinoma. Multivariate analysis showed that older age [odds ratio: 26.51 (2.36-381.47); P = 0.007], presence of precore mutants [odds ratio: 4.23 (1.53-19.58); P = 0.02] and presence of basal core promoter mutants [odds ratio: 2.93 (1.24-7.57); P = 0.02] were independent predictors for progression to hepatocellular carcinoma.CONCLUSION: Our results show that high levels of baseline serum HBV DNA are associated with non- hepatocellular carcinoma-related deaths of liver failure, while genetic mutations in the basal core promoter and precore regions are predictive for development of hepatocellular carcinoma.

Early hepatitis B viral DNA clearance predicts treatment response at week 96

AIM To investigate whether hepatitis viral DNA load at 24 wk of treatment predicts response at 96 wk in patients with chronic hepatitis B.METHODS A total of 172 hepatitis B envelope antigen(HBe Ag)-positive chronic hepatitis B patients who received initial treatment at 16 tertiary hospitals in Hunan Province, China were enrolled in this study. All patients received conventional doses of lamivudine and adefovir dipivoxil, telbivudine, entecavir dispersible tablets, or entecavir tablets for 96 wk. Patients who used other antiviral drugs or antitumor and immune regulation therapy were excluded. Patients were stratified into three groups according to their viral DNA load at 24 wk: < 10 IU/m L(group 1), 10-103 IU/m L(group 2), and > 103 IU/m L(group 3). Correlations of 24-wk DNA load with HBe Ag negative status and HBe Ag seroconversion at 96 wk were analyzed. Receiver operating characteristic curve analysis was used to test the predictive value of the HBV DNA load at 24 wk for long-term response.RESULTS The rates of conversion to HBe Ag negative status and HBe Ag seroconversion rates were 53.7% and 51.9%, respectively, in group 1; 35.21% and 32.39% in group 2; and 6.38% and 6.38% in group 3. The receiver operating characteristic curves for the three subgroups revealed that the lowest DNA load(< 10 IU/m L) was better correlated with response at 96 wk than a higher DNA load(10-103 IU/m L). Nested PCR was used for amplifying and sequencing viral DNA in patients with a viral DNA load > 200 IU/m L at 96 wk; resistance mutations involving different loci were present in 26 patients, and three of these patients had a viral DNA load 10-103 IU/m L at 96 wk. CONCLUSION Hepatitis B viral DNA load at 24 wk of antiviral treatment in patients with chronic hepatitis B is a predictor of the viral load and response rate at 96 wk.

Distinctive Drug-resistant Mutation Profiles and Interpretations of HIV-1 Proviral DNA Revealed by Deep Sequencing in Reverse Transcriptase

Objective To investigate distinctive features in drug-resistant mutations(DRMs) and interpretations for reverse transcriptase inhibitors(RTIs) between proviral DNA and paired viral RNA in HIV-1-infected patients. Methods Forty-three HIV-1-infected individuals receiving first-line antiretroviral therapy were recruited to participate in a multicenter AIDS Cohort Study in Anhui and Henan Provinces in China in 2004. Drug resistance genotyping was performed by bulk sequencing and deep sequencing on the plasma and whole blood of 77 samples, respectively. Drug-resistance interpretation was compared between viral RNA and paired proviral DNA. Results Compared with bulk sequencing, deep sequencing could detect more DRMs and samples with DRMs in both viral RNA and proviral DNA. The mutations M184 I and M230 I were more prevalent in proviral DNA than in viral RNA(Fisher's exact test, P<0.05). Considering ‘majority resistant variants', 15 samples(19.48%) showed differences in drug resistance interpretation between viral RNA and proviral DNA, and 5 of these samples with different DRMs between proviral DNA and paired viral RNA showed a higher level of drug resistance to the first-line drugs. Considering ‘minority resistant variants', 22 samples(28.57%) were associated with a higher level of drug resistance to the tested RTIs for proviral DNA when compared with paired viral RNA. Conclusion Compared with viral RNA, the distinctive information of DRMs and drug resistance interpretations for proviral DNA could be obtained by deep sequencing, which could provide more detailed and precise information for drug resistance monitoring and the rational design of optimal antiretroviral therapy regimens.

HBV C基因型有关的HBsAg阴性HBV DNA阳性患者S区突变对HBsAg的影响

目的通过构建HBV C基因型突变质粒研究HBsAg阴性HBV DNA阳性患者HBV S区突变对HBsAg水平的影响。方法收集2022年8月至2023年4月首都医科大学附属北京佑安医院107例HBsAg-/HBV DNA+患者血液样本,对成功提取扩增的HBV DNA S区进行测序,通过构建HBV C基因型突变质粒对HBV S区突变位点进行细胞功能验证,探讨OBI可能发生的分子机制。结果对成功提取扩增的68例患者进行测序,发现HBV S区存在大量突变,包括免疫逃逸突变(如sG145R、sK122R、sS114T、sT131P等)和跨膜结构域(transmembrane domain,TMD)突变(如sT5A、sG10D、sF20S等)。通过构建HBV C基因型突变质粒,进行细胞转染和细胞免疫荧光实验发现sG145R突变会明显降低HBsAg的表达,但是sK122R、sI26N、sQ29N、sR169H、sS114T、sT131P这6个突变位点并未影响细胞内外HBsAg的表达。结论通过测序发现HBsAg-/HBV DNA+患者HBV S区存在大量突变位点,通过构建sG145R、sK122R、sI26N、sQ29N、sS114T和ST131P等突变质粒发现sG145R突变会明显降低细胞内外HBsAg的表达,但是sK122R、sI26N、sQ29N、sR169H、sS114T、sT131P并未明显降低细胞内外HBsAg的表达。

HBV-DNA病毒载量在不同HBV感染产妇产后血清、唾液、乳汁中的变化及与肝功能的相关性研究

目的 观察不同HBV感染产妇的HBV-DNA病毒载量及其与肝功能的相关性。方法 102例HBV产妇根据HBV血清标志物分为三组,比较各组的HBV-DNA载量以及ALT、 AST水平,分析HBV-DNA载量与肝功能的相关性。结果 产妇血清、唾液、乳汁中的HBV-DNA载量,以及血清中ALT、 AST水平由高到低依次为A组、 B组、 C组(P <0.05)。不同HBV感染产妇的血清、唾液、乳汁HBV-DNA载量与ALT、 AST水平均呈正相关(P <0.05)。结论 随着HBV感染程度的加深,产妇血清、唾液、乳汁中的HBV-DNA病毒载量呈上升趋势,产后血清、唾液及乳汁中HBV-DNA病毒载量均与肝功能密切相关。

Evolution of HBV Viral Load during Clinical and Biological Follow-Up of Chronic Hepatitis B Patients at the Saint Camille Hospital in Ouagadougou

Hepatitis B virus (HBV) infection is a major public health problem worldwide. The aim of this study was to document the dynamics of HBV viral load during the follow-up of chronic hepatitis B patients at the Saint Camille Hospital in Ouagadougou (HOSCO) from 2017 to 2021. This descriptive retrospective study was carried out in the Hepato-Gastro-Enterology Department of HOSCO and focused on patients who were undergoing treatment for chronic viral hepatitis B. A total of 260 cases of chronic hepatitis B were included in the study. The most affected age group was 21 to 30 years, accounting for 48.08% of the cases. Lifestyle factors included alcohol consumption (3.08%) and tobacco use (2.69%). Major risk factors for transmission included lack of vaccination (98.46%), family history of HBV infection (68.00%) and engagement in high-risk activities (28.00%). Patients requiring treatment were prescribed Tenofovir 300 mg tablets. FibroScan® showed the presence of stage F3-F4 fibrosis (2.14%) and S3 steatosis (13.33%). After one year of follow-up, 6.92% of patients achieved an undetectable viral load with normalized transaminase levels. The majority of other patients had a detectable viral load but below 20,000 IU/mL. The prevalence of viral hepatitis B remains significant worldwide. Although effective and well-monitored treatment can lead to undetectable viremia, prevention remains the most effective strategy for successful management of this disease.

Sequencing of PCR amplified HBV DNA pre-c and c regions in 2.2.15 cells and antiviral action by targeted antisense oligonucleotide directed against sequence

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DNA-guided hepatitis B treatment,viral load is essential,but not sufficient

Hepatitis B virus(HBV) infection is a global public health problem that concerns 350 million people worldwide.Individuals with chronic hepatitis B(CHB) are at increased risk of developing liver cirrhosis,hepaticde-compensation a nd hepatocellular carcinoma.To maintain undetectable viral load reduces chronic infection complications.There is no treatment that eradicates HBV infection.Current drugs are expensive,are associated with adverse events,and are of limited efficacy.Current guidelines try to standardize the clinical practice.Nevertheless,controversy remains about management of asymptomatic patients with CHB who are hepatitis B e antigen(HBeAg)-positive with normal alanine aminotransferase,and what is the cut-off value of viral load to distinguish HBeAg-negative CHB patients and inactive carriers.We discuss in detail why DNA level alone is not sufficient to begin treatment of CHB.

血清EBV抗体及其DNA联合检测对鼻咽癌诊断价值

目的探讨血清EB病毒(EBV)抗体以及EBV-DNA联合检测在鼻咽癌治疗前诊断中的临床价值。方法采用酶联免疫吸附试验(ELISA)法检测163例鼻咽癌病人和140例健康对照者血清EBV衣壳抗原IgA(VCA-IgA)、早期抗原IgA(EA-IgA)、Rta蛋白IgG(Rta-IgG)抗体水平,荧光定量聚合酶链式反应法检测EBV-DNA载量,评价各项指标在鼻咽癌诊断中的价值。结果鼻咽癌病人血清EBV VCA-IgA、EA-IgA、Rta-IgG抗体效价和EBV-DNA载量水平以及其阳性率均显著高于健康对照者(t=12.499~14.597,Z=12.893,χ^(2)=51.274~153.132,P<0.05)。VCA-IgA+EA-IgA+Rta-IgG+EBV-DNA联合检测诊断鼻咽癌的曲线下面积(AUC)为0.992。Ⅲ~Ⅳ期鼻咽癌病人VCA-IgA、Rta-IgG抗体效价及EBV-DNA载量均显著高于Ⅰ~Ⅱ期病人(t=3.332、4.324,Z=10.507,P<0.05)。结论VCA-IgA+EA-IgA+Rta-IgG+EBV-DNA联合检测对于鼻咽癌早期筛查及诊断具有较高的临床价值。

房水与角膜样本对疱疹病毒阳性角膜移植后不同层次病毒DNA检测效率比较

目的研究疱疹病毒DNA在疱疹病毒阳性角膜移植患者不同角膜层次中的分布,比较角膜和房水样本在该人群中的病毒DNA检测效率。方法采用诊断试验研究方法,通过临床病历系统收集2015年5月至2021年8月于北京大学第三医院眼科中心行角膜移植且术中角膜和/或房水疱疹病毒DNA阳性患者。分析疱疹病毒DNA阳性患者的一般资料和分布层次。计算疱疹病毒在角膜和房水中的检出率,通过受试者工作特征曲线分析角膜和房水病毒DNA检测灵敏度,记录曲线下面积(AUC)和95%置信区间(CI)。结果角膜移植术中疱疹病毒DNA阳性患者共166例166眼,其中巨细胞病毒(CMV)75眼(占45.2%),单纯疱疹病毒1型(HSV-1)34眼(占20.5%),水痘-带状疱疹病毒(VZV)30眼(占18.1%),EB病毒(EBV)27眼(占16.3%)。CMV和VZV DNA在角膜内皮层分布者分别为47眼(占62.7%)和26眼(占86.7%),明显多于基质层的28眼(占37.3%)和4眼(占13.3%),差异均有统计学意义(χ^(2)=4.813、16.133,均P<0.05)。HSV-1和EBV DNA在角膜内皮层分布者分别为8眼(占23.5%)和5眼(占18.5%),分别少于基质层的26眼(占76.5%)和22眼(占81.5%),差异均有统计学意义(χ^(2)=9.529、10.704,均P<0.001)。疱疹病毒DNA阳性样本的检测灵敏度结果显示,角膜样本的病毒PCR检测总体灵敏度为71.6%,高于房水的54.1%,其中,CMV和VZV DNA阳性的角膜样本检测灵敏度分别为64.3%(AUC=0.821,95%CI:0.705~0.938)和35.7%(AUC=0.679,95%CI:0.475~0.882),分别低于房水样本的71.4%(AUC=0.875,95%CI:0.750~0.964)和85.7%(AUC=0.929,95%CI:0.816~1.000)。HSV-1和EBV DNA阳性的角膜样本检测灵敏度分别为100%(AUC=1.000,95%CI:1.000~1.000)和92.3%(AUC=0.962,95%CI:0.875~1.000),明显高于房水样本的27.8%(AUC=0.639,95%CI:0.455~0.823)和23.1%(AUC=0.615,95%CI:0.395~0.835)。结论在疱疹病毒DNA阳性的角膜移植患者中,CMV DNA的检出率最高,CMV和VZV DNA多在角膜内皮层被检出,HSV-1和EBV DNA多在角膜基质层被检出。相较房水样本,角膜组织病毒DNA的检测灵敏度更高。

野生大雁新发单链环状DNA病毒基因组鉴定和分析

野鸟作为多种致病性病毒的天然宿主,可通过迁徙活动广泛传播病毒,给人类和其他动物的生命安全带来了严峻挑战。本研究中,我们从青海湿地公园的野生大雁泄殖腔拭子中鉴定出13个新型CRESS-DNA病毒全基因组。此外,基于Rep蛋白的系统发育分析表明,这13株新型CRESS-DNA病毒被划分为CRESS-DNA病毒家族的两个不同进化枝,其中1株隶属于未分类的CRESS-DNA病毒簇的分支,而其余12株则全部归类为类双生病毒科(Genomoviridae)。本研究在野生大雁体内发现13个新型CRESS-DNA病毒,将有助于我们对于CRESS-DNA病毒的多样性以及进化起源的研究。

HBV DNA定量与血清学标志物及CEA、HA联合检测HBV感染的临床价值

目的 探究乙型肝炎病毒(HBV DNA)定量与血清学标志物及血清癌胚抗原(CEA)、血清透明质酸酶(HA)联合检测HBV感染的临床价值。方法 选取2019年1月至2021年11月阜南县人民医院收治的慢性乙型病毒性肝炎患者92例作为研究对象,所有患者均行临床乙肝血清学标志物[包含乙肝表面抗原(HBsAg)、乙肝表面抗体(抗-HBs)、乙肝e抗原(HBeAg)、乙肝e抗体(抗-HBe)、乙肝病毒的核心抗体(抗-HBc)]、CEA、HA以及HBV DNA检测,观察并记录所有患者HBV DNA、CEA、HA的检测结果,比较血清标志物对HBV DNA的检测阳性率,分析HBV DNA定量与血清学标志物及CEA、HA联合检测HBV感染的临床价值。结果 92例患者中,HBV DNA阳性患者54例(58.70%),阴性38例(41.30%)。大三阳组患者HBV DNA阳性31/33例(93.94%),小三阳组患者HBV DNA阳性15/31例(48.39%),其他类型组患者HBV DNA阳性3/28例(10.71%)。92例患者CEA水平4.20(3.20,5.30)ng/mL;HA水平分别为112.00(98.00,126.00)ng/mL。HBV DNA阳性组患者CEA、HA水平显著高于HBV DNA阴性组,差异有统计学意义(P<0.05)。HBV DNA阳性组中,HBsAg阳性检出率显著高于HBeAg,差异有统计学意义(P<0.05)。Spearman相关结果显示,患者的HBV DNA定量与CEA、HBsAg、HA指标成正相关关系(P<0.05)。ROC分析显示:HBV DNA定量与血清学标志物及血清CEA、HA联合检测乙肝病毒感染的AUC=0.985(P<0.05),诊断敏感度为97.76%。结论 HBV DNA定量与血清学标志物CEA、HA联合检测在HBV感染诊断中具有较高的应用价值,可起到互补作用,为临床检测提供了新路径。

DNA-guided hepatitis B treatment:Viral load is insufficient with few exceptions

In DNA-guided hepatitis B treatment,viral load is insufficient,and requires other viral markers for treatment of hepatitis B patients as in patients with acute exacerbation of chronic hepatitis B,end-stage renal disease on dialysis,human immunodeficiency virus co-infected patients.There are exceptions to this rule:a residual level hepatitis B virus(HBV)DNA at 24 wk predicts beneficial outcome and reduced resistance at 1 year.The genotypic viral resistance to antiviral agents and occult HBV infection can be determined by HBV-DNA levels.

采用高敏检测技术检测血清HBV DNA载量筛选低病毒血症的无偿献血人群隐匿性乙型肝炎病毒感染研究

目的 探讨采用高敏检测技术检测血清乙型肝炎病毒(HBV)DNA筛选低病毒血症(LLV)的无偿献血人群隐匿性乙型肝炎病毒感染(OBI)的价值。方法 2017年2月~2021年12月我市收集的11352份血清HBsAg阴性的无偿献血人群血液标本,采用电化学发光法定性检测血清(HBeAg、HBeAb和HBcAb),定量检测血清HBsAb,使用AU5800型全自动生化分析仪检测血生化指标,使用ABI ViiA7型荧光定量PCR扩增仪,采用高敏PCR法检测血清HBV DNA载量,对所有经高敏PCR法检测为HBV DNA阳性的血清再使用Cobas AmpliPrep/Cobas TaqMan全自动核酸定量检测系统复核。结果 以全自动核酸定量检测系统检测结果为金标准,发现高敏PCR检测为HCV DNA阳性的67例(0.59%)为LLV人群,结果显示,该方法诊断OBI人群LLV的灵敏度和特异度均为100.0%和100.0%;金标准方法与高敏PCR检测血清HCV DNA载量差异无统计学意义【(110.7±20.2)IU/ml对(108.2±19.6)IU/ml,P>0.05】;经高敏PCR法检验发现,LLV人群血清HBV DNA载量为100~200 IU/ml者41例(61.2%),20~100 IU/ml者15例(22.4%),和<20 IU/ml者11例(16.4%);5例血清HBsAb/HBeAb/HBcAb阳性人群血清HBV DNA载量为(162.4±18.3) IU/ml,显著高于9例血清HBcAb阳性人群【(82.3±14.1)IU/ml,P<0.05】或16例HBeAb/HBcAb阳性人群【(136.9±15.7)IU/ml,P<0.05】或32例HBsAb/HBcAb阳性人群【(99.3±15.5)IU/ml,P<0.05】或3例HBsAb阳性人群【(71.5±12.9)IU/ml,P<0.05】或2例血清HBV标志物全阴性人【分别为55.0 IU/ml和56.1 IU/ml】。结论 采用高敏PCR法检测血清HBV DNA载量能够在献血员人群中筛选LLV的OBI感染者,为临床用血安全又加了一道保险。

昆明地区低病毒载量慢性乙肝患者血清高敏HBV DNA检测分析

目的 探讨昆明地区持续低水平病毒血症的慢乙肝患者,高敏HBV-DNA载量、HBV的基因型分布特点、HBV P区耐药位点的突变特征,和HBeAg、HBsAg、ALT之间的关系及临床应用价值。方法 采集2021年1月至2021年12月期间于昆明市第三人民医院就医的707例慢性乙肝患者的血清,分析高敏HBVDNA、HBV的基因型以及HBV P区的耐药位点突变情况,并分析不同HBV-DNA载量与HBeAg、 HBsAg、ALT之间的关系。结果 研究707例持续低载量慢性乙肝患者中,高敏HBV DNA(<500 IU/mL)446例,占(63.50%),高敏HBV DNA小于2 000 IU/mL的慢乙肝患者共有576例,占(81.90%);HBeAg阳性262例(37.05%);基因分型以C基因型占比最高60.53%(428/707)。在196例HBeAg阳性且HBV DNA <2 000 IU/mL患者组中,男性为主,占69.89%;ALT> 40 U/L占28.57%,有73.47%患者的HBV DNA> 20 IU/mL。在265例HBV DNA <20 IU/mL的患者中,80.38%(213例)患者HBeAg阴性,19.62%(52例)HBeAg呈阳性。临床指标比较,HBeAg阳性率、ALT异常率、耐药位点和其它位点突变率在HBV DNA载量水平不相同组之间差异有统计学意义(P <0.05)。结论 对持续低水平病毒血症的慢性乙型肝炎患者,选择高敏的PCR技术定期监测乙肝病毒HBV DNA,结合HBeAg、HBsAg、ALT等临床指标的定量监测,可为后续患者的临床治疗提供客观的参考依据。

Conserved balance of hepatocyte nuclear DNA content in mononuclear and binuclear hepatocyte populations during the course of chronic viral hepatitis

瞄准：到有增加的原子 DNA 的 hepatocytes 的百分比满足的分析，即，四倍的(4n ) 和 octoploid (8n ) 原子核，然后比较单音原子并且双性人原子 hepatocyte 人口。方法：百分比单音原子双( 2n )，双性人的 4n ，和 8n hepatocytes 和那些原子 2 x 2n ， 2 x 4n ，并且 2 x 8n hepatocytes 与一个方法被决定能同时与长期的肝炎 B 或 C 在 62 个病人测量原子 DNA 满足的 hepatocyte 和 binuclearity 。在单音的原子 hepatocyte 人口的 4n 和 8n hepatocytes 的百分比在双性人与 2 x 4n 和 2 x 8n hepatocytes 的百分比相比原子 hepatocyte 人口。结果：在双性人的在单音的原子 hepatocytes 的 4n 和 2 x 4n 和 2 x 8n hepatocytes 的百分比原子 hepatocytes 是类似的，不管这项活动或长期的肝炎并且不管感染的病毒的纤维变性等级。结论：在内的原子 DNA 内容的分发单音原子并且双性人原子 hepatocyte 人口在长期的病毒的肝炎的功课期间被保存。

HBsAg/HBV DNA值与乙型肝炎患者TGF-β1、Tim-3水平的关系

【目的】探讨乙型肝炎患者乙型肝炎表面抗原(HBsAg)/乙型肝炎病毒(HBV)DNA值与转化生长因子-β1(TGF-β1)、T淋巴细胞免疫球蛋白黏蛋白分子3(Tim-3)水平的关系。【方法】两院收治的70例乙型肝炎患者,依据病情严重程度将患者分为轻度HBV组(22例)、中度HBV组(30例)、重度HBV组(18例),另选同期体检的健康志愿者30例为对照组。收集所有研究对象的临床血生化资料,比较各组肝功能指标及HBsAg/HBV DNA、TGF-β1、Tim-3水平,采用Pearson相关分析HBsAg/HBV DNA值与乙型肝炎患者TGF-β1、Tim-3水平的关系。【结果】不同病情严重程度的HBV患者及对照组间血清谷丙转氨酸(ALT)、谷草转氨酸(AST)、总胆红素(TBIL)、血小板计数(PLT)水平比较,均为对照组<轻度HBV组<中度HBV组<重度HBV组,且各组比较差异均有统计学意义(均P<0.05)。各组HBsAg/HBV DNA值比较,轻度HBV组>中度HBV组>重度HBV组(均P<0.05);各组TGF-β1、Tim-3水平比较,对照组<轻度HBV组<中度HBV组<重度HBV组(均P<0.05)。HBsAg/HBV DNA比值与乙型肝炎患者TGF-β1、Tim-3水平呈显著负相关(P<0.05)。【结论】乙型肝炎患者HBsAg/HBV DNA值与TGF-β1、Tim-3水平呈显著负相关。

联合检测EB病毒不同抗体及EB病毒DNA在鼻咽癌血清学诊断中的价值

目的:评价EB病毒(EBV)抗衣壳抗原VCA-IgA抗体、抗早期抗原EA-IgA抗体、抗立即早期抗原Rta-IgG抗体和EBV-DNA检测在鼻咽癌诊断中的价值。方法:收集160例初治鼻咽癌,133例症状相似的非鼻咽癌患者和163名健康体检者的血清和血浆。采用酶联免疫法检测血清VCA-IgA、EA-IgA和RtaIgG抗体的水平,用实时荧光定量PCR检测血浆EBV-DNA的相对含量。按鼻咽癌2008临床TNM分期法进行分期,计算不同分组、各临床分期以及鼻咽癌治疗前后的各抗体阳性率、抗体水平以及EB-DNA的检测结果并进行数据分析。结果:鼻咽癌组VCA-IgA、EA-IgA、Rta-IgG和EBV-DNA阳性率均高于鼻咽相关疾病组及健康对照组(均P<0.05)。血清VCA-IgA和EA-IgA结果相对A值(即r A或S/CO值)在Ⅰ、Ⅱ期低于Ⅲ、Ⅳ期,差异有统计学意义(P<0.05),但阳性率在各期间比较差异无统计学意义(P>0.05);Ⅰ、Ⅱ期患者Rta-IgG的r A值和阳性率明显低于Ⅲ、Ⅳ期患者(P<0.05);血浆中EBV-DNA阳性率及EBVDNA中位数水平随着临床分期的升高而增高,Ⅰ、Ⅱ期与Ⅲ、Ⅳ期比较差异有统计学意义(P<0.05)。治疗有效(CR+PR)患者的EBV-DNA含量明显低于治疗前水平(P<0.05)。结论:VCA-IgA、EA-IgA、RtaIgG、EBV-DNA检测有助于鼻咽癌的辅助诊断、临床分期预测及疗效评估。

用分子对接方法研究HIV-1整合酶与病毒DNA的结合模式

用分子对接方法研究了HIV-1整合酶(Integrase,IN)二聚体与3′端加工(3′Processing,3′-P)前的8bp及27bp病毒DNA的相互作用,并获得IN与27bp病毒DNA的特异性结合模式.模拟结果表明,IN有特异性DNA结合区和非特异性DNA结合区;IN二聚体B链的K14,R20,K156,K159,K160,K186,K188,R199和A链的K219,W243,K244,R262,R263是IN结合病毒DNA的关键残基;并从结构上解释了能使IN发挥活性的病毒DNA的最小长度是15bp.通过分析结合能发现,IN与DNA稳定结合的主要因素是非极性相互作用,而关键残基与病毒DNA相互识别主要依赖于极性相互作用.模拟结果与实验数据较吻合.

氧化苦参碱对HepG2.2.15细胞中乙型肝炎病毒DNA表达量的影响

目的 :观察氧化苦参碱对 Hep G2 .2 .15细胞中乙型肝炎病毒 (HBV ) DNA表达量的影响 ,进一步探讨其抗病毒机制。方法 :用不同浓度的氧化苦参碱作用 Hep G2 .2 .15细胞 ,留取培养上清后 ,采用 PCR- EL ISA技术定量上清中 HBV DNA,并比较其抑制率。结果 :氧化苦参碱能直接抑制 Hep G2 .2 .15细胞内 HBV DNA的复制 ,且随着药物浓度升高抑制作用逐渐增强。保持药物在培养上清中的浓度是保证抑制率的关键。 结论 :氧化苦参碱可以在 DNA复制水平直接抑制乙型肝炎病毒的合成。