混合单克隆抗体ELISA直接法和夹心法检测包虫病人循环抗原

本文对混合单克隆抗体ＥＬＩＳＡ直接法和ＥＬＩＳＡ夹心法检测包虫病人循环抗原的效果进行了比较研究。结果表明,ＥＬＩＳＡ夹心法对细粒棘球蚴囊液纯化抗原的最低检出量（１．２ｎｇ／ｍｌ）较直接法（１０ｎｇ／ｍｌ）低,但检测包虫病人循环抗原时,ＥＬＩＳＡ直接法的阳性检出率为５６．３９％（２７／４８）,ＥＬＩＳＡ夹心法为６０．４％（２９／４８）,二者无显著性差异（Ｐ＞０．０５）。两法同时检测１４份猪囊尾蚴病人血清和４４份正常人血清,均未出现假阳性反应。     

清洁级实验动物四种病毒抗体玻片酶免疫检测试剂盒的研制

本文报道对清洁级实验动物应排除的四种病毒（淋巴细胞脉络丛脑膜炎病毒、小鼠脱脚病病毒、鼠肝炎病毒和仙台病毒）抗体玻片酶免疫（ＥＩＡ）检测试剂盒的研制。四种病毒感染的细胞和对照细胞经冷丙酮固定于载玻片上制成特异性抗原和对照抗原,此四种病毒的抗血清各１０份和ＳＰＦ小鼠血清２０份分别与四种病毒的特异性抗原和对照抗原进行ＥＩＡ交叉试验,结果显示,抗原只与其相应抗血清发生特异性显色反应,与非特异性小鼠血清和ＳＰＦ小鼠血清不显色。与ＨＩ或ＥＬＩＳＡ方法比较,通过对１１２份普通小鼠血清进行测试,结果表明,ＥＩＡ对仙台病毒抗体的检出率（１９．６％）显著高于（＜０．００５）ＨＩ（６．３％）,对小鼠脱脚病病毒抗体的检出率（２３．３％）与ＨＩ（２１．４％）无显著性差异（Ｐ＞０．０５）。ＥＩＡ对淋巴细胞脉络丛脑膜炎病毒和鼠肝炎病毒抗体的检出率分别为１．８％和７１．２％,ＥＬＩＳＡ对两种病毒抗体的检出率分别为１．８％和６７．６％,两种方法对两种病毒抗体的检出率无显著性差异（Ｐ＞０．０５）。重复性试验表明两批四种病毒抗体试剂盒对１０８份小鼠血清两次测定的符合率为９６～１００％。四种病毒的ＥＩＡ抗原在－１８℃保存１２个月或在２－８℃保存３     

应用ELISA法检测纯化狂犬病疫苗制备过程中的病毒回收率

应用ＥＬＩＳＡ和病毒毒力滴度测定两种方法对狂犬病疫苗纯化过程中各步样品进行检测,并应用ＮＩＨ效力测定法对ＥＬＩＳＡ法测定的结果进行验证。结果显示,ＥＬＩＳＡ法具有灵敏度高、特异性强、重复性好、简便易行等优点,是一种较理想的病毒回收率测定方法。     

丙型肝炎病毒核心蛋白基因在大肠杆菌内的表达及应用

将从中国丙肝病人血清中扩增克隆的丙型肝炎病毒核心蛋白基因（４０８ｂｐ）酶切处理后插入表达载体ｐＪＬＡ５０２内,获得高表达核心蛋白的重组工程菌。将重组菌经４２℃热诱导５ｈ,ＳＤＳ－ＰＡＧＥ分析表明,表达的核心蛋白占菌体蛋白总量的２０％。经分子筛和吸附层析纯化后获得的核心蛋白,ＥＬＩＳＡ检测证实有较好的抗原性和特异性。用表达的核心抗原加用表达的ＮＳ＿３抗原（Ｃ＿３３）装配的抗－ＨＣＶ试剂盒,经用标准血清验证及与国外第二代抗－ＨＣＶ试剂盒比较,证实符合丙肝诊断试剂要求。     

草鱼生长激素非竞争式酶联免疫吸附测定法的建立及鉴定

应用草鱼生长激素（ｇｃＧＨ）单克隆抗体及多价兔抗血清建立了草鱼ＧＨ非竞争式酶’联免疫吸附测定ＥＬＩＳＡ系统。用正辛酸法对腹水单抗进行了分离纯化,获得了高纯度的单抗制备物。聚丙烯酸胺凝胶电泳表明纯化的单抗由分子量分别为５５ｋＤ和２５ｋＤ的两条蛋白带组成。用纯化单抗铺底,用兔抗血清作后续抗体建立了一种测定草鱼ＧＨ的非竞争式双抗夹心ＥＬＩＳＡ方法。交叉试验表明该测定系统只与草鱼ＧＨ和基因重组鲤生长激素（ｒｃＧＨ）具有剂量依存的结合反应,而与大马哈鱼生长激素（ｓＧＨ）、牛生长激素（ｂＧＨ）、大马哈鱼促性腺激素（ｓＧｔＨ）、及黑鲢促性腺激素（ｂｓｃＧｔＨ）等均无交叉反应。该 ＥＬＩＳＡ方法的灵敏度可达０．８ｎｇ／ｍｌ,组内变异系数为 ５．９ ％,组间变异系数为７．６％,回收率达９０％以上。初步应用表明,鲤和团头鲂垂体抽提液、草鱼血清、鲤血清及鲫血清在该测定系统中有剂量依存的反应曲线,而大口鲶、黄颡鱼、中华鲟及黄鳝鱼垂体抽提液及大口鲶、胡子鲶和罗非鱼血清在该测定系统中没有交叉反应。     

免疫聚合酶链反应技术的建立及其对甲胎蛋白的检测

免疫ＰＣＲ是一种新的具高敏感性的抗原检测技术,它类似传统的ＥＬＩＳＡ法,若与抗体连接的酶用ＤＮＡ片段代替,则该ＤＮＡ片段可用于ＰＣＲ扩增。以链酶亲合素搭桥将生物素标记的抗体与ＤＮＡ相连建立了免疫ＰＣＲ技术,并将其用于检测甲胎蛋白（ＡＦＰ）,其敏感性比ＥＬＩＳＡ法高１０４。因此,免疫ＰＣＲ有可能作为一种具高敏感性的检测手段用于临床早期诊断     

免疫—PCR：一种新的抗原检测系统

免疫－ＰＣＲ是１９９２年建立的抗原检测系统，其基本过程和ＥＬＩＳＡ相似，免疫－ＰＣＲ用一段可扩增的ＤＮＡ分子代替ＥＬＩＳＡ中的酶来放大检出信号，因而大大提高了灵敏度，尽管此法尚处于探索阶段，但应用前景是诱人的。     

幽门螺杆菌热休克蛋白A基因的克隆、表达及免疫原性研究

幽门螺杆菌的感染可诱发人体产生胃炎和消化性溃疡,其组成成分热休克蛋白Ａ（ＨｓｐＡ）可刺激机体产生保护性的免疫反应。用ＰＣＲ方法从幽门螺杆菌的染色体ＤＮＡ上扩增出ＨｓｐＡ基因片段,将其插入原核表达载体ｐＥＴ２２ｂ（＋）中,并在ＢＬ２１（ＤＥ３）大肠杆菌表达。经测序ＨｓｐＡ基因片段有３５４ｂｐ组成,可编码１１８个氨基酸残基的多肽。ＳＤＳＰＡＧＥ和免疫印迹分析检测发现,ＨｓｐＡ基因表达的蛋白质分子量约为１５ｋＤ,并证实该重组蛋白质可以被幽门螺杆菌感染阳性患者的血清所识别,同时将其免疫小鼠可刺激机体产生抗该重组蛋白质的抗体。ＨｓｐＡ有可能作为一种有效的蛋白质疫苗用于幽门螺杆菌感染的预防和治疗。     

双抗体夹心ELISA法检狂犬病疫苗抗原活性组分

采用多克隆双抗体夹心ＥＬＩＳＡ法快速检测狂犬病毒抗原含量。结果表明,灵敏度达到１５μｇ／ｍｌ,同时特异性及变异系数均合呼要求,本方法用于精制狂苗制备过程中有效抗原活性组分的检测准确,快速,重复性好,且抗原的ＥＬＩＳＡ效价与ＮＩＨ动物法测定效价具有平行趋势。     

毕赤酵母表达的重组乙肝表面抗原SS1的纯化及性质鉴定

对毕赤酵母（Ｐｉｃｈｉａ ｐａｓｔｏｒｉｓ）表达的重组乙肝表面抗原ＳＳ１的纯化以及蛋白质的理化性质及免疫原性进行了进一步的研究。采用单抗亲和层析的方法,一步纯化即可得到纯度为９５％的纯化蛋白质。ＥＬＩＳＡ和Ｗｅｓｔｅｒｎ印迹鉴定表明,纯化的ＳＳ１融合蛋白同时具有良好的Ｓ和ＰｒｃＳ１抗原性。ＣｓＣ１密度梯度离心和电镜检测的结果则表明,这一重组抗原可以形成与ＨＢＶ亚病毒颗粒类似的颗粒结构。在ＢＡＬＢ／     

胃癌与幽门螺杆菌cagA、hrgA基因相关性的研究

目的:探讨幽门螺杆菌(Hpylori)菌株中cagA和hrgA基因对胃癌的致病作用及其检测的意义。方法:胃癌及消化性溃疡术后切除标本,组织学检查,快速尿素酶法和PCR检测。结果:40例标本经组织学检查24例为胃腺癌,2例为胃黏膜相关淋巴样组织(MALT)瘤,14例为消化性溃疡。经快速尿素酶法检测,胃腺癌中,12例H pylori( ),消化性溃疡中,12例H pylori( )。经PCR检测,胃腺癌中,18例hrgA( ),6例hrgA(-),20例cagA( ),4例cagA(-);消化性溃疡中,6例hrgA( ),8例hrgA(-),12例cagA( ),2例cagA(-)。结论:H pylori感染与胃癌的发生有密切关系。PCR检测较快速尿素酶法准确。检测cagA和hrgA基因对了解Hpylori菌株的致病性、估计疾病程度、了解病变预后及临床治疗都具有重要意义。     

结核分枝杆菌重组38kD蛋白用于新疆南疆维吾尔族和湖南湘中汉族血清学诊断的研究

目的：对结核分枝杆菌38kD蛋白编码基因进行克隆表达及纯化,建立基于重组38kD蛋白的酶联免疫吸附法（EusA）检测结核病人血清标本,评价重组38kD蛋白用于结核病血清学诊断抗原的价值。并比较分析其在汉族和维吾尔族人群中的血清学诊断的差异。方法：用PCR方法扩增38kD蛋白的编码基因,构建重组质粒,转化到大肠杆菌BL21中,经IPTG诱导表达,得到纯化的38kD蛋白,建立以38kD蛋白为包被抗原的ELISA,并检测临床确诊的结核病人血清标本。结果：ELISA检测结核病患者血清标本的维吾尔族阳性率为34％（52／153）,汉族为52．4％（65／124）,两者对比有统计学差异（x2=9．538,P〈O．005）。在阴性对照中的维吾尔族特异度为96．4％（159／165）,汉族为98．8％（130／133）,结果无统计学意义（x2=0．111,P〉0．5）。结论：重组38kD蛋白用于血清学诊断的敏感度在维吾尔族和汉族中有差异,而其诊断特异度无差别。     

结核分枝杆菌重组38kD蛋白用于新疆南疆维吾尔族和 湖南湘中汉族血清学诊断的研究

目的：对结核分枝杆菌38kD 蛋白编码基因进行克隆表达及纯化,建立基于重组38 kD 蛋白的酶联免疫吸附法(ELISA)检测 结核病人血清标本,评价重组38 kD蛋白用于结核病血清学诊断抗原的价值。并比较分析其在汉族和维吾尔族人群中的血清学 诊断的差异。方法：用PCR方法扩增38 kD 蛋白的编码基因, 构建重组质粒, 转化到大肠杆菌BL21 中,经IPTG诱导表达, 得到纯 化的38 kD 蛋白,建立以38 kD蛋白为包被抗原的ELISA,并检测临床确诊的结核病人血清标本。结果：ELISA 检测结核病患者 血清标本的维吾尔族阳性率为34%（52/153）,汉族为52.4%（65/124）,两者对比有统计学差异（X2＝9.538,P＜0.005）。在阴性对照 中的维吾尔族特异度为96.4%（159/165）,汉族为98. 8%（130/133）,结果无统计学意义（X2＝0.111,P＞0.5）。结论：重组38kD 蛋白 用于血清学诊断的敏感度在维吾尔族和汉族中有差异,而其诊断特异度无差别。     

幽门螺杆菌尿素酶的纯化及其特性

本文利用Ｓｅｐｈａｃｒｙ１ Ｓ－２００和Ｑ－Ｓｅｐｈａｒｏｓｅ两步层析,从ＨＰ蒸馏水浸液中提取纯化尿素酶,并对其特性进行了测定,证明ＨＰ尿素酶各含一个６６ｋＤ和２９．５ｋＤ的亚单位,并以６个分子聚合成６２５ｋＤ大分子蛋白,有很好的抗原性,并显示特异的血清学反应。用ＨＰ超声浸液抗原和尿素酶,加入２μｇ霍乱毒素粘膜佐剂,给ＳＰＦ ＢＡＬＢ／Ｃ小鼠口服免疫,可使８０％小鼠抵抗ＨＰ活菌的攻击,证明尿素酶是一种抗ＨＰ的保护性抗原。     

Clinical usefulness of urine-based enzyme-linked immunosorbent assay for detection of antibody to Helicobacter pylori: a collaborative study in nine medical institutions in Japan

Background. A urine-based enzyme-linked immunosorbent assay (ELISA) kit for detection of antibody to Helicobacter pylori has been developed in Japan. Urine samples can be obtained noninvasively and are easier and safer to handle than are serum samples. The aim of this study was to examine the clinical usefulness of this urine-based ELISA kit.
Materials and Methods. A pair of random, single-void urine and serum samples was collected from each of 1,061 subjects, including 238 patients with gastroduodenal disease. The sensitivity and specificity of the urine-based ELISA was compared with those of three commercially available serum-based ELISA kits. For those patients with gastroduodenal disease, the urine- and serum-based ELISA results were also compared with those for other diagnostic methods using endoscopic biopsy specimens, such as culture, histology, and rapid urease tests.
Results. Based on the three serum-based ELISA results, the sensitivity, specificity, and accuracy of the urine-based ELISA were 97.7%, 95.6%, and 96.8%, respectively. On the basis of the biopsy test results, the sensitivity (96.2%), specificity (78.9%), and accuracy (91.0%) of the urine-based ELISA were almost equivalent or superior to all three serum-based ELISAs tested. In addition, 10 of the 12 false-positive cases for urine-based ELISA were confirmed to be true positives for antibodies to H. pylori by Western blot analysis and inhibition ELISA.
Conclusions. The urine-based ELISA (URINELISA H. pylori Antibody) is very accurate and should be useful as an alternative to serum-based ELISAs for screening of H. pylori infection.     

口蹄疫病毒P1基因在大肠杆菌中的高效表达及其生物活性的初步分析

将口蹄疫病毒 (FMDV)结构蛋白基因P1的完整cDNA序列插入原核表达性载体pGEX KG中 ,使P1基因与GST融合 ,获得融合表达质粒pKG P1,转化E .coliBL₂₁ (DE3) ,经IPTG诱导 ,SDS PADE结果表明GST P1融合蛋白获得高效表达 ,Western blot检测证实表达的融合蛋白具有免疫学活性 ,表达产物主要存在于细菌裂解液上清中。进一步采用GST纯化试剂盒纯化P1蛋白并作为诊断抗原 ,建立了P1 ELISA诊断方法 ,与FMD间接血凝 (IHA)检测方法平行检测 86 4份血清样品 ,总的符合率达87%。     

Ureaplasma urealyticum urease genes; use of a UGA tryptophan codon

Nucleotide sequence analysis of a Ureaplasma urealyticum DNA fragment, homologous to cloned urease genes of other prokaryotes, revealed three consecutive open reading frames. The molecular weights of the three deduced polypeptides are 11.2 kD, 13.6 kD and 66.6 kD. These values are consistent with the size of the three subunits previously reported for purified native urease. A significant sequence homology was found between the three polypeptides of the ureaplasmal urease and the single polypeptide of jack bean (Canavalia ensiformis) urease. Codon usage indicates that UGA is a tryptophan codon in this mollicute. Use of polymerase chain reactions has disclosed the existence of genetic polymorphism among the urease genes of different serotypes of U. urealyticum.     

马西尼罗热病毒E蛋白部分基因在大肠杆菌中的表达

参考GenBank发表的西尼罗病毒(west nile virus,WNV)的E蛋白基因序列,自行设计合成一对引物,利用RT-PCR扩增出了WMV E基因318bp片段,将其克隆入pMD18-T-Vector载体中,阳性克隆命名pMD-E,并进行序列分析。进一步亚克隆入表达载体pET-32a( )。重组质粒pET32a-E转化BL21(DE3)感受态细胞中表达,表达产物经SDS-PAGE可检测到分子量约为32kD的目的蛋白带,经薄层扫描分析,目的蛋白占菌体总蛋白的33．1%。表达产物纯化后,Wester-blotting分析证明表达产物能被WNV的阳性血清所识别,为下一步建立以表达产物为包被抗原建立检测马的WNV的ELISA方法打下了基础。     

Sex differences in the subunits of glutathione-S-transferase isoenzyme from rat and human kidney

Glutathione-S-transferase (GST) isoenzymes were purified from cytosolic preparations from kidneys of male and female rats and kidney cortical specimens from 2 male and 1 female human subjects. GST isoenzyme expression was analyzed by SDS-PAGE, measurement of catalytic activities with specific substrates and determination of their subunits by ELISA and Western blotting using specific antibodies. GST from female rat kidneys showed a preponderance of subunits 3 and 4; levels of these isoenzymes were 3-4 times greater in females than in males. Levels of subunits 1 and 2 were 1.5-2 times greater in the male rat kidneys. Additional minor bands at 24 and 22 kD were observed in GST preparations from both male and female rat kidneys while a band at 25.3 kD was observed only in the male rat kidney. These bands did not react with antibodies to GST 1-1, GST 2-2 or GST 3-4. Both male and female human kidney samples contained GST isoenzymes comparable to the near-neutral (25-5 kD) and basic forms (25 kD) of GSTs found in human liver. In addition a 28-kD band was present in GST preparations from both male and female human kidneys. Additional bands at 29 and 25.2 kD were present only in male human kidneys. Both the kidney cytosol and the total GSTs prepared from female rats shared 2- to 4-fold greater activity with 1,2-dichloro-4-nitrobenzene, ethacrynic acid and trans-4-phenyl-3-buten-2-one than those from males. The measurement of specific subunit amounts by ELISA were in agreement with these results.(ABSTRACT TRUNCATED AT 250 WORDS)     

Detection of antibody to hepatitis delta virus in human serum by double antigen sandwich ELISA

A simple rapid detection of antibody to hepatitis delta virus (anti-HDV) in human serum was developed by using double antigen sandwich ELISA. HDV gene fragment encoding HDAg was isolated from a Chinese patient infected with HDV by RT-PCR, and a high-efficient expression HD-PQE31 strain was constructed with the fragment. We obtained high titer and good quality hepatitis delta virus protein purified by Ni-NTA metal-affinity chromatography, which was identified by Western blot and ELISA, then we set up the double antigen sandwich ELISA for detection of anti-HDV in human serum, and the performance of the sandwich ELISA was evaluated in terms of specificity and sensitivity. Results were: 1) The purified HDAg protein's purity was 90%, and its ELISA titer was 1/100 000. 2) 42 anti-HDV positive sera were detected and showed that the sensitivity of sandwich ELISA was higher than that of competitive ELISA (t=2.44, p<0.01). 3) The inhibitory rates for 2 anti-HDV positive sera by the specific HDAg were 74% and 93% respectively. 4) For the assay of specificity, all 60 samples infected by other hepatitis viruses and 30 normal samples were negative for anti-HDV. These results suggested that the double antigen sandwich ELISA with purified recombinant HDAg showed higher specificity and sensitivity, It can be used in routine laboratories to diagnose the HDV infection.