Melatonin and schistosomal antigens ameliorate the anti-oxidative and biochemical response to Schistosoma mansoni infection in hamster

The present study was designed to investigate the potential protective effect of melatonin as an antioxidant separately or in combination with antigens (cercarial; CAP or soluble worm; SWAP) against Schistosoma mansoni infection in hamsters. Each hamster was sensitized with an initial immunization of 0.6 ml of the extracted antigen (30 μg protein/mL). After four days,a second injection of 0.4 mL was given (20 μg protein/mL). Then,each hamster was exposed to 260±20 S.mansoni cercariae followed with melatonin treatment (3.5 mg/kg) for thirty days from the 1st day of post infection. Levels of lipid peroxidation (LPO) products,catalase (CAT) activity,hepatic glutathione (GSH) and biochemical changes in the liver and kidneys functions were investigated. The results revealed a high significant increasing of LPO and decreasing of CAT and GSH in liver of infected hamsters. Biochemical observations showed severe damage in the liver enzyme activities and increasing cholesterol level in infected animals. Melatonin co-treatment with antigen to the infected-hamster attenuated the increase of LPO and restored the activity of CAT and levels of hepatic GSH. Also,the biochemical damages in the liver and kidneys functions were reduced. The present study suggests that melatonin may be useful in combating free radical-induced damage due to infection toxicity. The immunization with previous antigens resulted in a remarkable improvement on the liver enzyme activities,which were increased after infection. Thus,vaccination of hamsters with antigens (both CAP and SWAP) and melatonin treatment has more potent effect on the enhancement of antioxidant and biochemical of S.mansoni infected-hamster than each treatment separately. Immunization of the hamster with SWAP followed by melatonin was the best way among the other regime treatments to improve the biochemical and antioxidant parameters of the

Mapping the Antigenic Peptides of Sm26/2 in Glutathione S-Transferases of Schistosoma Mansoni

Six antigenic peptides of Sm26/2 glutathione S-transferase of schistosoma mansoni have been predicted according to their hydrophilicity, flexibility, accessibility, charge distribution and beta-turn in the secondary structure by the determination of its primary structure, and synthesized by solid phase method. Two of them showed good antigenicity by Dot-ELISA. They would be candidate peptides of synthetic anti-schistosomal vaccine.

Screening and Primary Characterization of NewAntigen Genes of Schistosoma Japonicum

To find Schistosoma japonicum(S.j)new antigen gene thus provide more useful vaccine candidates, the cDNA library of S.j adult worm was screened with sera of rabbits immunized with the membrane antigens of Schistosoma japonicum hepato-portal schistosomula (SjHmAg). The positive clones were amplified by PCR and sequenced, then the sequences of clones were compared with all sequences in GenBank database using Blast process. The new clones were submitted to GenBank for accession numbers. Fifteen positive clones were obtained after three rounds of immunoscreening. The size of S.j cDNA fragments in positive clones ranged from 0.7?kb-3.0?kb after automatically excised with the helper phage. Sequence analysis revealed that partial sequence of clone M5 had significant homology with S.j mitochondria mRNA, the other positive clones were new S.j genes. M2 clone sequence (GenBank accession number AF502579) was 730?bp long it had a 117?bp open reading frame (ORF). The sequence of M15 (GenBank accession number AF502582) has no transmembrane region and encodes 92 amino acids, and its protein contains a ferredoxins iron-sulfur binding region signature and two VWFC signal regions. The size of M1、M8、M9、M12(GenBank accession numbers: AF502578, AF502580, AF500622, AF502581) ranges from 402?bp to 766?bp. It concluded that the sera from rabbit immunized with SjHmAg could recognize S.j specific antigens molecules, and these antigens may induce the protective immunity against S.j infection.

The Construction of Schistosoma Japonicum Vaccine BCG-Sj26GST and Its Identification

Summary: The expression of foreign gene, Schistosoma Japonicum 26 ku antigen (Sj26GST), in Bacillus Calmette Guerin (BCG), Mycobacterium ( M. smegmatis ) and Escherichia coli ( E. coli ) were studied. The cDNA fragment encoding Sj26GST was amplified by PCR using plasmid pGEX, which could express Sj26GST in E. coli as template. The Sj26GST cDNA was cloned into the downstream of human M. tuberculosis heat shock protein (hsp) 70 promoter with correct reading frame, and then the DNA fragment containing hsp70 promoter and Sj26GST gene were subcloned together into E. coli Mycobacteria shuttle plasmid pBCG 2000 to construct the expression shuttle plasmid pBCG Sj26. The recombinant BCG and M. smegmatis mc 2 155, which were electroplated with pBCG Sj26, could express Sj26GST and the recombinant Schistosoma Japonicum vaccine BCG Sj26GST was made. The recombinant Sj26GST (rSj26GST) were soluble and could be observed on SDS PAGE at molecular weight of 26 ku. The content of rSj26GST accounted for 15 % and 10 % of total bacterial protein in BCG and M. smegmatis respectively. The results of Western blot showed the combination of rSj26GST with antibody of GST.

Isolation and Characterization of 44.6 kDa Protein from Schistosoma japonicum Male Worm

Soluble male worm antigen of Schistosoma japonicum ( Sj ) was investigated for development of new vaccine candidate. SDS-PAGE and Western blotting were performed to compare the difference between soluble antigens from worms of different sex. Mice vaccination with the testing purified protein was followed by Sj cercariae challenge to detect the protective effect against Sj . Sixteen bands were seen for the soluble male worm antigen and 12 for the female worm. In addition, a distinct band of 44.6 kDa from the male worm antigen was observed, and its antigenicity was demonstrated by Western blotting. This 44.6 kDa protein could induce significant worm and egg reduction rate in mice (39.31%, 41.98%, P <0.001). In this study a 44.6 kDa protein was isolated and partially characterized. Its antigenicity, immunogenicity and the partial immune protection suggest its potential vaccine candidte against Sj .

用噬菌体随机肽库鉴定日本血吸虫22.6kDa抗原分子的表位

目的 筛选和鉴定日本血吸虫 (中国大陆株 ) 2 2 .6kDa抗原 (Sj2 2 .6)的表位。 方法 用纯化的抗Sj2 2 .6的多克隆抗体IgG对噬菌体十二肽库进行 5轮免疫学筛选 ,挑取克隆 ;采用Westernblotting免疫识别 ,将获得的阳性克隆免疫小鼠 ,并采用dot ELISA筛选能刺激小鼠产生较高滴度抗Sj2 2 .6抗体的阳性克隆 ;测定核苷酸序列 ,分析其表位与Sj2 2 .6抗原的同源性。 结果 经 5轮免疫学筛选后挑取的 1 4个克隆 ,用Westernblotting方法均能被抗Sj2 2 .6抗体识别。经动物免疫初步实验筛选 ,共获得 6个免疫原性较强的阳性克隆 ,测序结果获得 4种不同表位 ,其中 1种表位与Sj2 2 .6抗原具有较高的同源性 ,其余 3种表位与其无一级结构的同源性。 结论 获得的 4种日本血吸虫中国大陆株抗原表位 ,1种可能为结构表位 。

日本血吸虫成虫和虫卵主要血清学抗原的鉴定和理化学分析

应用SDS—聚丙烯酰胺凝胶电泳、化学染色和免疫印斑对日本血吸虫成虫和虫卵的主要血清学抗原进行了鉴定和理化学分析。成虫有8个主要的血清学抗原分子,其分子量和化学性质分别为152kDa、脂蛋白;145kDa、脂蛋白;32kDa、脂蛋白;30kDa、脂蛋白;28kDa、糖脂蛋白;15kDa、糖脂蛋白;12kDa、糖脂蛋白;11kDa、糖脂蛋白。虫卵有7个主要血清学抗原分子,其分子量和化学性质性质分别为32kDa、脂蛋白;28kDa、脂蛋白;15kDa、糖蛋白;12.5kDa、脂蛋白;12kDa、糖蛋白;11kDa、糖蛋白;10.5kDa、糖蛋白。

日本血吸虫31/32kDa分子抗原快速诊断试剂盒的研制与现场应用

目的基于纯化的日本血吸虫31／32kDa分子抗原，建立一种敏感、特异、简便、快速诊断血吸虫病的试剂盒。方法采用Chappell方法分离纯化Sj31／32kDa抗原并建立快速ELISA，检测急、慢性血吸虫病人，并以肺吸虫病人、肝吸虫病人及正常人血清作为平行对照。结果血吸虫病人457例，阳性检出率为94．3％，67例肺吸虫病人及76例肝吸虫病人血清均未出现明显交叉反应，正常人群假阳性率为1％。结论提示采用纯化的优势诊断抗原分子建立的快速诊断试剂盒有较好的现场应用潜能，且具有简便、快速、无需特殊设备等优点，值得推广应用。

抗rSjCTPI单克隆抗体检测血吸虫循环抗原的研究

为探讨抗重组血吸虫磷酸丙糖异构酶 (r Sj CTPI)的单克隆抗体检测血吸虫循环酶抗原在血吸虫病免疫诊断和疗效考核中的价值。制备日本血吸虫 r Sj CTPI表达蛋白 ,以此重组蛋白免疫小鼠 ,筛选出高效价的抗 r Sj CTPI单抗 ,建立以纯化的抗血吸虫可溶性虫卵抗原 (SEA)的多克隆抗体 (Ig G)为捕捉系统 ,以酶标的抗 r Sj CTPI单抗为检测系统的酶联免疫吸附试验 (P- M- EL ISA)法检测血吸虫病人等血清。并对该法的敏感性、特异性、交叉反应以及疗效考核与常规的 SEA- EL ISA比较。结果获得了一株抗 r Sj CTPI的单克隆抗体 ,其抗体同型为 Ig G1。P- M- EL ISA检测急性、慢性血吸虫病人、健康人以及华枝睾吸虫病人、肺吸虫病人血清的阳性率分别为 10 0 %、91.7%、 0、0和0。而 SEA- EL TSA为 10 0 %、98.3%、6 .6 9%、10 %和 2 0 %。P- M- EL ISA法对 30例同批血吸虫病人治疗前的阳性率和治愈后 4个月的阴转率分别为 10 0 %和 30 % ;而 SEA- EL TSA分别为 10 0 %和 10 %。结果表明 ,应用抗 r Sj CT-PI单抗检测血吸虫病人循环抗原的 P- M- EL ISA法具有较高的敏感性和特异性 ,并有一定的疗效考核价值。

日本血吸虫未成熟虫卵67kDa分子抗原诊断血吸虫病的研究

本文通过SDS－PAGE和电渗方法，从日本血吸虫未成熟虫卵可溶性抗原（SIEA）中分离纯化出67kDa蛋白分子，以该分子包被微板进行ELISA，检测了急、慢性日本血吸虫病人血清，其阳性检出率达100％和94．6％，与60例正常人血清、30例肝吸虫和31例肺吸虫病人血清均未出现明显交叉反应，慢性血吸虫病人治疗后3个月、半年和1年的阴转率分别为58．1％，75．4％和84．6％。提示SIEA67kDa分子抗原具有较好的疗效考核价值和现场应用前景。

日本血吸虫循环抗原动态消长的实验研究

目的：了解日本血吸虫三类循环抗原（ＣＡｇ）在感染家兔的动态变化及治疗后的消长情况。方法：制备日本血吸虫的三株单抗，以辣根过氧化物酶标记，分别建立检测日本血吸虫肠相关抗原（ＧＡＡ）、膜相关抗原（ＭＡＡ）和可溶性虫卵抗原（ＳＥＡ）的斑点酶联免疫吸附试验（ｄｏｔ－ＥＬＩＳＡ），观察感染日本血吸虫家兔血中三类抗原的动态变化情况。结果：家兔感染后第４ｗｋ，有３９％家兔血中ＧＡＡ呈阳性反应，而仅８．６％家兔ＭＡＡ、ＳＥＡ呈阳性反应，第８ｗｋ三类ＣＡｇ均呈阳性反应，并于第１０ｗｋ左右达高峰。未治疗组家兔直至感染后第２７ｗｋ，血中三类ＣＡｇ一直维持较高水平。感染后第９ｗｋ家兔接受吡喹酮治疗，治疗后第４ｗｋ，ＣＡｇ水平开始下降，治疗后第６ｗｋ有１０％家兔ＳＥＡ阴转，治疗后第８ｗｋ，ＧＡＡ阴转率为２０％，ＳＥＡ为７０％，ＭＡＡ为８０％，治疗后第１４ｗｋ除１例外，三类ＣＡｇ全部阴转。结论：ＧＡＡ早期诊断效果较好，而ＭＡＡ和ＳＥＡ在治疗后较ＧＡＡ消失快。

抗日本血吸虫SEA鸡卵黄抗体的制备与鉴定

目的制备特异性抗日本血吸虫可溶性虫卵抗原(SEA)的鸡卵黄免疫球蛋白(IgY)并检测其特异性、敏感性。方法用日本血吸虫SEA经翅膀下静脉和皮下免疫25周龄海兰母鸡4次(首次剂量为60μg/只,加强剂量为30μg/只),每次间隔10d。取免疫前和首次免疫后35d的鸡蛋卵黄,分别用水稀释法提取IgY,BCA法测定蛋白含量,并进行十二烷基磺酸钠-聚丙烯酰胺凝胶电泳(SDS-PAGE)和蛋白质印迹(Westernblotting)分析,ELISA检测纯化后IgY特异性和敏感性。分别提取免疫后不同时间的卵黄抗体,观察抗体效价的变化。结果海兰母鸡经SEA首次免疫后35d,每枚蛋经提纯后可得到约61mg抗体,经SDS-PAGE和Westernblotting分析,纯化的IgY有1条主要蛋白带,相对分子质量(Mr)为130000,并可被SEA识别。母鸡初次免疫后第10天,经SDS-PAGE和ELISA分析,鸡蛋卵黄内即有抗体产生,初次免疫后31d效价可达1∶1600。双抗体夹心ELISA结果显示纯化后的IgY有较高的敏感性,可检测到的SEA达2.4ng/ml。结论制备的抗SEA鸡卵黄抗体的特异性和敏感性均较高。

日本血吸虫Mr23000抗原与白细胞介素-12多价DNA疫苗诱导小鼠保护性免疫的研究

目的研究能共同表达日本血吸虫Mr23000膜抗原(Sj23)与白细胞介素-12(IL-12)的多价DNA疫苗PV-IL12-Sj23诱导BALB/c小鼠免疫保护作用。方法在多价DNA疫苗PV-IL12-Sj23和PV-IL12的基础上,构建空白质粒PV和仅表达Sj23的质粒PV-Sj23。50只BALB/c小鼠分为5组,每组10只,分别注射多价DNA疫苗PV-IL12-Sj23、表达Sj23的质粒PV-Sj23、表达IL-12质粒PV-IL12、空白质粒PV和生理盐水,100μg/只,免疫1次。4周后每只鼠攻击感染40±2条尾蚴,42d后剖杀,计数成虫及肝内虫卵数。结果成功地构建了空白质粒PV和只表达Sj23的质粒PV-Sj23及多价DNA疫苗PV-IL12-Sj23。PV-IL12-Sj23组和PV-Sj23组分别获得了45.5%和27.2%的减虫率,两组比较差异有显著性(P<0.05),减卵率分别为58.4%和33.9%。结论多价DNA疫苗PV-IL12-Sj23可诱导BALB/c小鼠产生较显著的抗血吸虫免疫保护作用,且保护性效果比单价DNA疫苗PV-Sj23好。

日本血吸虫虫卵中毛蚴抗原的融合表达及抗原性分析

目的重组表达制备日本血吸虫虫卵中毛蚴抗原(SjMP10)。方法根据日本血吸虫虫卵中毛蚴抗原SjMP10分子的读框序列设计合成1对引物,扩增SjMP10DNA片段并克隆到表达载体pGEX-4T-3中。转化BL21(DE3)后,诱导表达谷胱甘肽转移酶-虫卵中毛蚴抗原10(GST-SjMP10)融合蛋白。采用洗脱法制备GST-SjMP10融合蛋白,应用免疫印迹法(Westernblotting)和淋巴细胞增殖试验进行重组蛋白的抗原性分析。结果SjMP10基因克隆到表达质粒pGEX-4T-3后,经异丙基-β-D-硫代半乳糖苷(IPTG)诱导能表达出Mr39000的GST-SjMP10融合蛋白,经电洗脱法纯化的上述重组融合蛋白可被血吸虫感染兔血清所识别,并能刺激血吸虫感染鼠脾淋巴细胞增殖。结论日本血吸虫虫卵中毛蚴抗原SjMP10融合表达获得成功。

日本血吸虫未成熟卵可溶性抗原的初步分析

采用ＳＤＳ－ＰＡＧＥ和ＥＬＩＢ技术分析了日本血吸虫未成熟卵可溶性抗原（ＳＩＥＡ），并与可溶性成熟卵抗原（ＳＥＡ）进行比较，二者主要蛋白区带存在明显差异。同时，ＥＬＩＢ结果表明，ＳＩＥＡ中感染血清和免疫血清所识别的６７ｋＤａ、６２ｋＤａ、５４ｋＤａ、５０ｋＤａ、２８ｋＤａ和２６ｋＤａ等抗原组分不出现于ＳＥＡ，推测其在ＳＩＥＡ诱导宿主产生抗雌虫生殖及抗卵胚发育免疫应答方面起作用。

日本血吸虫中国大陆株基因重组抗原Sj 22.6kDa的核苷酸序列分析

目的：对ｐＧＳｊ２４克隆化基因进行核苷酸序列分析，了解其编码蛋白的属性。方法：常规制备ｐＧＳｊ２４克隆化基因并重组入测序载体Ｍ１３ｍｐ１９，以ＤＹＥＰＲＩＭＥＲ荧光测序试剂盒进行核苷酸序列测定。分别以ＤＮＡＳＩＳ和ＧＯＬＤＫＥＹ软件对序列资料进行分析。结果：ｐＧＳｊ２４克隆化基因长８４０ｂｐ，含一开放阅读框，可编码一分子量为２２．６ｋＤａ的蛋白质。开读框上游和下游均有终止密码子。该基因与已发表的日本血吸虫２２．６ｋＤａ蛋白的编码基因同源性达９５％，编码区同源性达９９．７％。在该基因内有一段典型的ＥＦ－Ｈａｎｄ钙结合区序列，并有内质网导肽、微体导向信号等功能位点。预测该蛋白质内可能的抗原决定簇位置为第２９－３２、６３－６８和８７－１０１等氨基酸片段。结论：ｐＧＳｊ２４克隆化基因为日本血吸虫２２．６ｋＤａ抗原编码基因。

日本血吸虫SIEA26-28kDa的抗雌虫生殖免疫作用——HGPRT是否是主要的靶抗原(英文)

目的 观察日本血吸虫SIEA2 6 2 8kDa抗原的抗雌虫生殖作用。方法用AcA柱层析纯化日本血吸虫早期胚卵中的SIEA和SIEA2 6 2 8kDa成分 ,并以此纯化产物免疫BALB/c小鼠。将小鼠分为三组 ,分别用SIEA、SIEA2 6 2 8kDa和免疫佐剂免疫动物 ,然后进行尾蚴攻击感染。 4 6天后剖杀动物 ,冲虫 ,然后作虫荷测定及虫卵分类计数。结果 SIEA2 6 2 8kDa免疫组雌虫子宫内减卵率为 5 4 .8% ,与对照组比较有极显著性差异 ;该实验组动物肝脏和小肠组织内的虫卵数比对照组分别降低了 4 8.0 7%和 77.4 1% ,且以成熟虫卵数的下降较为显著 ,分别降低了 83.6 %和 93.3% ;粪卵数的下降幅度最为显著 ,达87.2 6 %。结论 SIEA2 6 2 8kDa可作为一种抗卵胚发育及抗雌虫生殖的候选抗原分子。

日本血吸虫24-26kDa抗原和重组Sj26抗原的抗原性和免疫原性比较研究

本文报告从日本血吸虫大陆株成虫抽提的24—26kDa抗原与源于日本血吸虫菲律宾株的重组Sj26抗原之间在抗原性和免疫原性上所进行的一系列比较研究。ELISA、IFA和Westernblotting等方法观察结果均表明,24—26kDa和rSj26抗原免疫后所诱导的特异性抗体与其对应的抗原之间具有明显的抗原交叉反应,而与其它血吸虫抗原如可溶性虫卵抗原也有交叉反应。若以两种抗原加福氏佐剂分别免疫小鼠,以日本血吸虫大陆株尾蚴攻击感染,减虫率相似(26～32％),表明两种抗原存在一定程度的交叉免疫保护性。这些研究结果为开发rSj26抗原,或是根据已知Sj26 cDNA核苷酸序列制备DNA探针,从已构建的日本血吸虫(大陆株)cDNA库筛选相关目的基因,加速血吸虫疫苗的研制起着重要作用。

日本血吸虫未成熟卵抗原和成虫抗原分别与联合免疫小鼠的研究

目的探讨日本血吸虫未成熟卵可溶性抗原（SIEA）和成虫抗原（SA）分别与联系免疫小鼠的抗卵胚胎发育效果和抗感染效果。方法采用SIEA与SA分别与联合免疫小鼠，于攻击感染后48天剖杀，统计雌雄虫数及肝脏各期虫卵数。结果与对照组比较，SIEA单独免疫产生显著抗卵胚胎发育的免疫力，肝组织成熟卵数下降37，3％，成熟卵比例下降24．0％；SA单独免疫产生显著抗感染免疫力，减虫率为34．5％；SIEA与SA联合免疫，产生显著抗感染免疫力和最佳抗卵胚胎发育免疫力，减虫率33．5％，成熟卵数和成熟卵比例分别下降73．8％和45．0％，抗卵胚胎发育免疫力显著高于SIEA单独免疫组。结论提示来源于成虫的抗感染抗原与来源于未成熟虫卵的抗卵胚胎发育抗原联合应用是血吸虫疫苗研制中有希望的发展方向。