Pre-S1Ag、Pre-S2Ag及HBV-LP在乙肝病毒检测中的性能

目的对三种HBV表面蛋白(Pre-S1 Ag、Pre-S2 Ag和HBV-LP)在HBV检测中的性能进行比较。方法通过对乙肝患者(包括HBsAg携带者和HBV DNA阳性患者)及健康人群Pre-S1 Ag、Pre-S2 Ag和HBV-LP的检测,对比分析其灵敏度、特异性和检出限。结果在进行HBV筛查时,三种表面蛋白特异性保持在99%~100%,反观Pre-S2 Ag和HBV-LP在检测HBsAg携带者、HBV-DNA阳性患者时,其敏感性表现要比Pre-S1 Ag更高(P<0.001)。三种表面蛋白吸光度与HBV-DNA水平呈正相关(P<0.001),Pre-S2 Ag和HBV-LP在HBV对应的检出限是2~3 Log10IU/mL,反观Pre-S1 Ag对HBV的检出限高于5 Log10IU/mL。结论通过Pre-S2 Ag、HBV-LP、Pre-S1 Ag对比来看,前面两者的敏感性较高,检出限较低,故可以用于HBV筛查、识别病毒的血清标志物。

PCR检测HBV DNA与HBV血清标志物常见模式和Pre-S2相互关系研究

目的 探讨乙型肝炎病毒 (HBV)DNA与六种常见HBV血清免疫学标志物模式、前S2 蛋白抗原 (Pre -S2 )之间的相互关系及其临床检测意义。方法 采用PCR法对HBVDNA、ELISA法对HBV血清免疫学标志物、Pre -S2 同时进行检测。结果 1484例六种常见模式HBVDNA阳性率依次为 89 8% >5 5 6 % >2 1 8% >7 5 % >7 1% >6 8% ,即模式 (1) >(3) >(2 ) >(5 ) >(6 )>(4) ;而HBV血清免疫学标志阳性例数依次为 (2 ) >(1) >(3) >(5 ) >(4) >(6 )。 (2 )、(3)种模式HBVDNA与Pre S2阳性率比较P <0 0 1,其余 (1)、(4)～ (6 )种模式HBVDNA与Pre-S2 阳性检出率无显著性差异 (P >0 0 5 )。结论 HBV血清免疫学标志物、Pre -S2、HBVDNA的检测 ,三者缺一不可 ,ELISA法检测HBV血清免疫学标志物、Pre -S2 ,只是HBV的表型指标 ,提供HBV感染的间接证据。而PCR -HBVDNA的检测是HBV感染与否的直接证据。因此它们各自有其独特的临床检测意义。

Pre-S2蛋白抗体结合部位的确定

本文研究了Pre-S2蛋白体液免疫反应的精细特异性。结果表明小鼠对Pre-S2蛋白的抗体反应部位主要局限于14—24共11个连续的氨基酸残基内,与我们理论预测的B细胞表位相吻合;人的抗Pre-S2阳性血清除识别与小鼠抗血清及其Pre-S2特异性单抗同一肽段外,还识别1—13肽段。这些结果对于设计新一代合成疫苗及诊断试剂有意义。

乙型肝炎患者Pre-S1、Pre-S2抗原与HBV-DNA的相关性分析

目的探讨乙型肝炎病毒(HBV)Pre-S1、Pre-S2抗原与HBV-DNA的相关性。方法对180例标本采用ELISA方法检测前S1抗原、前S2抗原,采用荧光定量PCR方法检测HBVDNA。结果在150例HBVDNA阳性的乙肝患者中,Pre-S1、Pre-S2的阳性率分别为89.33%和86.00%;30例HBVDNA阴性的乙肝患者中,Pre-S1、Pre-S2的阳性率分别为36.67%和26.67%。HBVDNA阳性和阴性患者的Pre-S1、Pre-S2的阳性率差异有统计学意义(P<0.05)。结论随着HBVDNA载量的增加,HBV乙肝患者的Pre-S1、Pre-S2的阳性率逐渐升高。Pre-S1、Pre-S2抗原与HBVDNA载量具有高度相关性,可作为HBVDNA检测的有效补充。

Pre-S2蛋白抗原表位及二级结构的预测与比较

本文采用Chou和Fasman方法预测adw,adr,ayw三种亚型的乙肝病毒Pre-S2蛋白的二级结构,并用双亲性方案和亲水性方案分析了抗原表位。结果显示三者均可能含有较多的β-片层和β-转折;N-末端30个残基所形成的二级结构较保守,而C-末端顺序的构象在亚型间差别较大;Th细胞识别的表位可能在39—49肽段,B细胞识别的表位可能主要在13—18残基或其附近,为分子免疫学的深入研究提供了线索。

Pre-S1Ag、Pre-S2Ag和HBeAg联合测定用于判断乙肝病毒传染性的研究

我国乙肝病毒感染率较高,目前判断乙肝病毒感染的最主要血清标志物为乙型肝炎“两对半”,其中乙肝表面抗原（HBsAg）是乙肝病毒感染检测中最为重要的一种标志物,但HBsAg阳性只能说明感染乙肝病毒,不能反映病毒是否复 制及传染性强弱。判断乙肝病毒是否复制就要进行HBV—DNA的检测。HBV—DNA检测步骤繁琐．条件要求较高。且成本高昂，一般基层医院无法开展。我们采用EUSA方法检测乙肝病毒前S1抗原（Pre-S1Ag）和前S2抗原（Pre-S2Ag），结合乙肝病毒e抗原（HBeAg）检测结果来判断乙肝病毒传染性强弱．取得了较好的效果。

Study of transactivating effect of pre-S2 protein of hepatitis B virus and cloning of genes transactivated by pre-S2 protein with suppression subtractive hybridization

AIM: To investigate the transactivating effect of pre-S2 protein of hepatitis B virus (HBV) and construct a subtractive cDNA library of genes transactivated by pre-S2 protein with suppression subtractive hybridization (SSH) technique, and to pave the way for elucidating the pathogenesis of HBV infection. METHODS: pcDNA3.1(-)-pre-S2 containing pre-S2 region of HBV genome was constructed by routine molecular methods. HepG2 cells were cotransfected with pcDNA3.1 (-)-pre-S2/pSV-lacZ and empty pcDNA3.1(-)/pSV-lacZ. After 48 h, cells were collected and detected for the expression of β-galactosidase (β-gal). SSH and bioinformatics techniques were used, the mRNA of HepG2 cells transfected with pcDNA3.1(-)-pre-S2 and pcDNA3.1(-) empty vector was isolated, respectively, cDNA was synthesized. After digestion with restriction enzyme RsaI, cDNA fragments were obtained. Tester cDNA was then divided into two groups and ligated to the specific adaptor 1 and adaptor 2, respectively. After tester cDNA was hybridized with driver cDNA twice and underwent two times of nested PCR, amplified cDNA fragments were subcloned into pGEM-Teasy vectors to set up the subtractive library. Amplification of the library was carried out with E.coli strain DH5oα. The cDNA was sequenced and analyzed in GenBank with Blast search after PCR. RESULTS: The pre-S2 mRNA could be detected in HepG2 cells transfected with pcDNA3.1(-)-pre-S2 plasmid. The activity of β-gal in HepG2 cells transfected with pcDNA3.1 (-)-pre-S2/pSV-lacZ was 7.0 times higher than that of control plasmid (P<0.01). The subtractive library of genes transactivated by HBV pre-S2 protein was constructed successfully. The amplified library contains 96 positive clones. Colony PCR showed that 86 clones contained 200-1 000 bp inserts. Sequence analysis was performed in 50 clones randomly, and the full length sequences were obtained with bioinformatics method and searched for homologous DNA sequence from GenBank, altogether 25 coding sequences were obtained, these cDNA sequences might be the target genes transactivated by pre-S2 protein. CONCLUSION: The pre-S2 protein of HBV has transactivating effect on SV40 early promoter. The obtained sequences may be target genes transactivated by pre-S2 protein among which some genes coding proteins involved in cell cycle regulation, metabolism, immunity, signal transduction and cell apoptosis.This finding brings some new clues for studying the biological functions of pre-S2 protein and further understanding of HBV hepatocarcinogesis.

Pre-S1Ag和Pre-S2Ag及HBV-LP在乙肝病毒筛查中的价值

目的:探讨乙肝病毒(HBV)前S1抗原(Pre-S1 Ag)、前S2抗原(Pre-S2 Ag)及乙肝大蛋白(HBV-LP)在乙肝病毒(HBV)筛查中的价值。方法:258例乙肝患者分为乙肝表面抗原(HBs Ag)携带组(n=182)及HBV DNA阳性组(n=76),另选100例健康体检者作为对照组;采用双抗体夹心(ELISA)法检测受检者血清Pre-S1Ag、Pre-S2 Ag及HBV-LP水平,比较Pre-S1 Ag、Pre-S2 Ag及HBV-LP筛查HBV的灵敏度和特异度,分析Pre-S1Ag、Pre-S2 Ag及HBV-LP对HBs Ag携带组3种血清学模式患者的HBV检出能力;采用线性回归法分析Pre-S1Ag、Pre-S2 Ag、HBV-LP与HBV DNA的相关性,推算3个指标的ABV病毒检出限。结果:Pre-S1 Ag、Pre-S2 Ag及HBV-LP应用于HBV筛查的特异度为99%～100%,但Pre-S2 Ag和HBV-LP筛查HBV的灵敏度显著高于Pre-S1 Ag(P <0. 01); HBe Ag阴性人群中(HBs Ag-HBeAb-HBcAb阳性和HBs Ag-HBcAb阳性模式)的Pre-S2 Ag、HBV-LP检出率均显著高于Pre-S1 Ag (P <0. 01); Pre-S1 Ag、Pre-S2 Ag及HBV-LP与HBV DNA正相关(r=0. 82、0. 76、0. 70,P <0. 01),Pre-S2 Ag、HBV-LP对HBV的检出限接近106IU/L,Pre-S1 Ag对HBV的检出限≥108IU/L。结论:Pre-S2 Ag、HBV-LP相较于Pre-S1 Ag具有更高的灵敏度和更低的检出限,更适合作为HBV筛查的血清标志物。

Construction of exogenous multiple epitopes of helper T lymphocytes and DNA immunization of its chimeric plasmid with HBV pre-S2/S gene

AIM: To design and construct an exogenous multiple epitope of helper T lymphocytes (HTL), and to evaluate its effect on anti-HBs response through DNA immunization. METHODS: Artificial HTL epitope, PADRE and four other HTL epitopes from different proteins were linked together using splicing by overlap extension to generate exogenous multiple epitopes of HTL, MTE5. pcMTE5 and pcHB were generated by cloning MTE5 and fragments of HBV pre-S2/S gene into mammalian expression plasmid pcDNA3. Four chimeric plasmids were constructed by cloning MTE5 into the region of pre-S2 gene (Barn HI), 5' terminal of S gene (HincII, Xba I) and 3' terminal of S gene (Acc I) of pcHB respectively. BALB/c mice were used in DNA immunization of the recombinant plasmids. Anti-HBs was detected using Abbott IMx AUSAB test kits.RESULTS: The sequences of MTE5 and the 6 constructs ofrecombinant plasmids were confirmed to be correct by DNA sequencing. The anti-HBs response of the coinoculation of pcHB and pcMTE5 was much higher than that of the inoculation of pcHB only (136.7+69.1 mIU/mL vs 27.6+17.3 mIU/mL, P<0.01, t =-6.56). Among the 4 chimeric plasmids, only the plasmid in which MTE5 was inserted into the pre-S2 region had good anti-HBs response (57.54±7.68 mIU/mL), and had no significant difference compared with those of pcHB and the co-inoculation of pcHB and pcMTE5. CONCLUSION: Exogenous multiple epitopes of HTL had immune enhancement when they were co-inoculated with pre-S2/S gene or inoculated in the chimeric form at a proper site of pre-S2/S gene of HBV. It might suggest that it was possible to improve hepatitis B vaccine using exogenous multiple epitopes of HTL. The antibody responses were very low using DNA immunization in the study. Thus, the immune enhancement effect of exogenous multiple epitopes of HTL has to be confirmed and the effect on overcoming the drawback of the polymorphism of HLA II antigens should also be evaluated after these chimeric plasmids are expressed in mammalian cell lines.

LC和HCC患者Pre-S2受体、HBV DNA检测分析

目的：探讨HCC患者不同血清HBV标志模式的Pre-S2受体和HBV DNA相互关系及临床诊治意义。方法：用ELISA和PCR同时检测血清HBV标志，Pre-S2受体和HBVDNA。结果：LC组(450例)，HCC组(468例)及对照组(696例)的HBV标志物阳性分别为66．7％，56．4％和12．9％。LC，HCC及对照组的HBV DNA阳性率分别为46．7％，35.2％和6.2％。LC组与对照组比较，HCC组与对照组比较，差异均显著。LC，HCC和对照组Pre-S2受体阳性率分别为48．0％，39．9％和5．8％。他们比较，均有显著性差异。结论：HBV血清标志模式、Pre-S2受体、HBVDNA对HBV患者的预后，LC，HCC发生的筛选有指导意义。

Pre-S1 Ag、Pre-S2 Ag及HBV-LP在乙肝病毒检测中的性能比较

目的通过对乙肝前S1抗原(Pre-S1 Ag)、乙肝前S2抗原(Pre-S2 Ag)及乙肝病毒大蛋白(HBV-LP)三种乙肝表面蛋白表达情况的检测,分析比较其灵敏度和特异性,以期获得适合常规乙肝筛查的血清标志物组合。方法应用ELISA法,分别检测健康人群和乙肝患者血清中三种表面蛋白的表达情况,利用实时荧光定量PCR法检测HBV-DNA载量。结果应用于HBV筛查时,三种表面蛋白特异性分别为97%、100%和100%,但Pre-S2 Ag和HBV-LP对HBsAg携带者、HBV-DNA阳性患者的灵敏度显著高于Pre-S1 Ag(P<0.0001),并且三种乙肝病毒表面蛋白阳性检出率随HBV DNA水平增高而递增,Pre-S2 Ag、HBV-LP对HBV的检测限接近于10^3IU/ml而Pre-S1 Ag约为10^5IU/ml。结论作为乙肝筛查的标志物,Pre-S2 Ag及HBV-LP更优于Pre-S1 Ag。

Hepatitis B virus pre-S2 start codon mutations in Indonesian liver disease patients

AIM: To identify the prevalence of pre-S2 start codon mutations and to assess their association with liver disease progression. METHODS: The mutations were identified by direct sequencing from 73 asymptomatic carriers, 66 chronic hepatitis (CH), 66 liver cirrhosis (LC) and 63 hepatocellular carcinoma (HCC) patients. Statistical significances were determined using Fisher's exact test, χ 2 test, and t -test analyses whenever appropriate. Pre-S mutation as a risk factor for advanced liver disease was estimated by unconditional logistic regression model adjusted with age, sex, and hepatitis B e antigen (HBeAg). P < 0.05 was considered significant. RESULTS: Mutation of the hepatitis B virus (HBV) pre-S2 start codon was found in 59 samples from 268 subjects (22.0%), with higher prevalence in patients with cirrhosis 27/66 (40.9%) followed by HCC 18/63 (28.6%), chronic hepatitis 12/66 (18.2%) and asymptomatic carriers 2/73 (2.7%) (P < 0.001). Logistic regression analysis showed that pre-S2 start codon mutation was an independent factor for progressive liver disease. Other mutations, at T130, Q132, and A138, were also associated with LC and HCC, although this was not statistically significant when adjusted for age, sex, and HBeAg. The prevalence of pre-S2 start codon mutation was higher in HBV/B than in HBV/C (23.0% vs 19.1%), whilst the prevalence of T130, Q132, and A138 mutation was higher in HBV/C than in HBV/B. The prevalence of pre-S2 start codon mutation was higher in LC (38.9%) and HCC (40.0%) than CH (5.6%) in HBeAg(+) group, but it was similar between CH, LC and HCC in HBeAg(-) group. CONCLUSION: Pre-S2 start codon mutation was higher in Indonesian patients compared to other Asian countries, and its prevalence was associated with advanced liver disease, particularly in HBeAg(+) patients.

乙型肝炎患者HBV-DNA与Pre-S1、Pre-S2抗原的相关性研究

目的探讨乙型肝炎患者乙型肝炎病毒DNA(HBV-DNA)与前-S1(pre-S1)抗原和前-S2(pre-S2)抗原的相关性。方法采用酶联免疫测定法检测800例HBeAg阳性慢性乙肝患者的前pre-S1抗原和pre-S2抗原,采用荧光定量聚合酶联反应法测定患者HBV-DNA。结果 213例HBV-DNA阴性患者的Pre-S1抗原阳性率为15.02%,PreS2抗原阳性率为9.86%;587例HBV-DN阳性患者的Pre-S1阳性率抗原为87.39%,Pre-S2抗原阳性率为80.75%;HBV-DNA阴性患者的Pre-S1和Pre-S2抗原阳性率显著地小于HBV-DNA阳性患者(P<0.05);HBV-DNA载量与pre-S1抗原和Pre-S2抗原具有高度的相关性(均P<0.001)。结论在HBeAg阳性慢性乙肝患者中,HBVDNA载量与Pre-S1抗原和Pre-S2抗原高度相关,pre-S1和pre-S2抗原检测是HBV-DNA检测的有效补充。

肾炎患者肾组织中乙型肝炎病毒Pre-S2蛋白的检测及意义

对30例经肾活检确诊为肾炎的患者,应用单克隆抗体和间接免疫酶标技术检测肾组织中的Pre-S_2蛋白,同时对肾脏中的HBsAg,HBeAg及血清HBsAg,HBeAg,抗HBs,抗HBe,抗HBc进行了观察。结果显示:7/22例原发性肾炎和6/8例狼疮性肾炎患者的肾小球中有Pre-S_2蛋白沉积,分布于毛细血管袢及(或)系膜区,其分布与肾炎类型、肾组织中免疫球蛋白和补体沉积的多少有关。肾脏中Pre-S_2蛋白的沉积与相同部位HBsAg的沉积有联系,与HBeAg的沉积无关。膜性肾病者Pre-S_2蛋白的沉积与病毒血症有良好的柑关性;狼疮性肾炎者Pre-S_2蛋白的沉积很可能是非特异性的。

Pre-S_2、抗Pre-S_2和HBV DNA在乙型肝炎患者中的相关性分析

目的 :探讨Pre_S2 、抗Pre_S2 二对半和HBVDNA对乙型肝炎患者血清学的诊断意义。方法 :用ELISA法和PCR法分别检测 93例乙型肝炎患者和 2 8例健康人血清中的Pre_S2 ,抗Pre_S2 ,二对半和HBVDNA水平。结果 :93例乙肝患者HBsAg、HBeAg、HBcAb阳性 32例 ,HBsAg、HBeAb、HBcAb阳性 39例 ,HBsAg、HBcAb阳性 18例 ,HBcAb阳性 4例。Pre_S2 结果阳性率 6 6 .7% (6 2 / 93) ,Pre_S2 抗体结果阳性率 1.1% (1/ 93) ,HBVDNA结果阳性率40 .9% (38/ 93)。 2 8例健康人二对半 ,五项全阴 16例 ,HBsAb阳性 12例 ,Pre_S2 阳性 1例 ,HBVDNA阳性 1例 ,Pre_S2 抗体阳性 5例占HBsAb阳性 41.7% (5 / 12 ) ,Pre_S2 和HBVDNA相比有明显差异 (P <0 .0 1) ,非HBeAg阳性组中HBVDNA阳性率约低于Pre_S2 。结论 :Pre_S2 ,抗Pre_S2 ,HBVDNA和二对半在乙型肝炎血清学诊断中显示 ,Pre_S2 优于HBVDNA和二对半。Pre_S2 抗体出现早于抗HBs和抗HBe ,抗Pre_S2 阳性检出率较低 ,可能同乙型肝炎疫苗中抗Pre_S2 含量低有关。

HBsAg阴性的HBV感染者血中pre-S_2和抗—pre—S_2的表达

本文分三个组(抗-HBc阳性组,抗-HBc、抗-HBe同时阳性组和抗-HBc、抗-HBe、抗-HBs同时阳性组),观察了97例HBsAg阴性的HBV感染者血清中的pre-S_2,抗-pre-S_2的情况,其中pre-S_2阳性5例,均分布在抗-HBc、抗-HBe同时阳性组,抗-pre-Sa_2阳性47例,以抗-HBc、抗-HBe、抗-HBs同时阳性组阳性率最高,占78.57％,且抑制率数值与抗-HBc和抗-HBe同时阳性组比较有显著差别。结果提示,抗-HBc、抗-HBe同时阳性组的部分人不能排除仍存在慢性HBV感染,而抗-pre-S_2在抗-HBc、抗-HBe、抗-HBs同时阳性组的存在应视为一种感染后的免疫标记。

乙肝病毒Pre-S_1、S_2抗原检测在乙型肝炎临床诊断中的价值

目的探讨乙肝病毒Pre-S1、S2抗原检测在乙型肝炎临床诊断中的作用及临床价值。方法对115例乙型肝炎患者采用ELISA法对乙肝五项、Pre-S1、Pre-S2抗原进行了检测,并对其结果进行回顾性分析。结果①115例HBV患者血清中的HBsAg、HBeAg、HBcAb患者,Pre-S1抗原阳性率为40.9%,其它均为零;Pre-S2抗原阳性率为78.0%。HBsAg、HBeAg、HBcAb组和HBsAg、HBeAb、HBcAb组Pre-S2与Pre-S1比较,经χ2检验,P<0.01。而63例HBsAg、HBeAb、HBcAb患者Pre-S2抗原阳性率为19.1%;11例HBsAg、HBcAb患者Pre-S2抗原阳性率为27.3%。②乙肝各项指标与Pre-S1、Pre-S2结果显示HBeAg最高,Pre-S1和Pre-S2分别是41.5%和78.0%;HBeAb检测Pre-S1无1例阳性,而Pre-S2结果12例阳性,阳性率为19.0%,Pre-S1与Pre-S2比较,经χ2检验,P<0.01,结果有显著性意义。结论PreSl、PreS2抗原与HBV呈不同程度相关性,是病毒感染、复制的指标较HBeAg敏感,是HBV存在和复制较为直接的标志,对HBV检测起重要的补充作用,对临床上判断HBV复制和疾病预后有重要的参考价值。其Pre-S2诊断乙肝患者对HBV的病毒感染、病毒复制、传染性及对不同临床类型肝炎等均优于其他检测指标。

乙型肝炎患者血清Pre-S2抗原的意义

目的研究ＰｒｅＳ２抗原与乙型肝炎患者ＨＢＶ标记的关系．方法血清ＨＢｓＡｇ（＋），ＨＢｅＡｇ（＋），ＨＢｃＡｂ（＋）的乙型肝炎患者２６例，血清ＨＢｓＡｇ（＋），ＨＢｅＡｂ（＋），ＨＢｃＡｂ（＋）的乙型肝炎患者４７例及健康献血者２０例，血清用ＲＩＡ法检测ＰｒｅＳ２抗原及用ＰＣＲ法检测ＨＢＶＤＮＡ．结果血清ＨＢｓＡｇ（＋），ＨＢｅＡｇ（＋），ＨＢｃＡｂ（＋）的乙型肝炎患者２６例，ＰｒｅＳ２抗原与ＨＢＶＤＮＡ均阳性（１００％）；血清ＨＢｓＡｇ（＋），ＨＢｅＡｂ（＋），ＨＢｃＡｂ（＋）的乙型肝炎患者４７例，ＰｒｅＳ２抗原３０例阳性（６３８％），１７例阴性（３６２％），ＨＢＶＤＮＡ３２例阳性（６８１％），１５例阴性（３１９％），ＰｒｅＳ２抗原与ＨＢＶＤＮＡ均阳性２８例（５９６％），均阴性１４例（３００％）．健康献血者２０例，ＰｒｅＳ２抗原阳性１例（５０％），阴性１９例（９５０％），ＨＢＶＤＮＡ阳性２例（１００％），阴性１８例（８００％），ＰｒｅＳ２抗原及ＨＢＶＤＮＡ均阳性０例（０％），均阴性１８例（８００％）．结论ＰｒｅＳ２抗原可作为预测慢性乙型肝炎患者病情活动与传染的标志．

乙肝病毒Pre-S2基因的研究新进展

Pre-S2作为HBV表面外膜蛋白重要的蛋白之一,在其基因表达、HBV感染复制、免疫逃逸等方面起重要作用,且与慢性肝炎、重型肝炎及HCC的发病机制密切相关。其免疫学研究尤其是Pre-S2核酸疫苗、单克隆抗体的制备为HBV预防感染提供了有力依据。本文对上述几个方面Pre-S2的研究进展进行了概述。