基于黏附素HpaA B细胞表位的多抗原肽疫苗的免疫原性鉴定

目的制备以幽门螺杆菌(Hp)黏附素HpaA B细胞表位为基础的多抗原肽(MAP)疫苗,并分析其免疫原性。方法在GenBank数据库检索Hp黏附素HpaA的氨基酸及核苷酸序列。采用表位分析软件预测HpaA的B细胞表位,以此合成8分支MAP并免疫白毛黑眼兔,体外试验测定MAP与兔抗Hp多克隆抗体的亲和力,体内试验检测免疫血清抗体效价和抗体的特异性。结果HpaA的优势B细胞表位可能位于其氨基酸序列的第130~142和第212~219区段,并分别以上述B细胞表位合成8分支MAP1和MAP2。MAP1和MAP2均能在体外与兔抗Hp多克隆抗体结合,且MAP1具有较高的亲和力。仅MAP1能在体内诱导免疫应答,产生高滴度特异性抗体。结论HpaA氨基酸序列的第130~142区段为其优势B细胞表位,基于此合成的MAP具有较强的免疫原性。

Restriction fragment length polymorphism of adhesin gene hpaA from different Helicobacter pylori strains of Chongqing, China

AIM:To assess the variability of adhesin gene hpaA between different Helicobacter pylori (H pylori) strains with PCR-restriction fragment length polymorphism (RFLP). METHODS: Twelve different H pylori strains were chosen to amplify the 710-bp segments of gene hpaA. These strains were NCTC11637, SS1; Chongqing clinical isolates CCS9801, CCS9802, CCS9803, CCS9806, CCS9809, CCS9810, CCS9813, which were gained from patients of gastritis; Mongolia gerbil adapted H pylori strains (abbreviation MG), which were gained from the following steps: gastric mucosal specimens of Mongolia gerbils infected by clinical isolate CCS9803 were cultured and detected, the positive H pylori strains were named as the first generation of Mongolia gerbil adapted H pylori strains (abbreviation MG1) and then were subcultured with healthy Mongolia gerbil to generate MG2, in turn to gain the ninth generation (abbreviation MG9). All hpaA segments, obtained from 12 different H pylori strains, were digested by Hhal and HaeIll individually and analyzed by agarose gel electrophoresis. RESULTS: In all 12 strains, the 710-bp PCR products were successfully amplified and products were cloned to pMD18-T vector respectively, then the recombinant plasmids were digested simultaneously with Ncol and Xhol to recover the small fragments. The objective fragments from 12 different H pylori strains digested with Haelll could be seen as 4 types of bands and 5 types with Hha I. According to the hpaA RFLP patterns, the 12 H pylori strains could be divided into 5 groups: group I, NCTC11637 and SS1; group II, CCS9809, which RFLP type digested with HaeIll was the same as strains of group I, but Hhal RFLP showed difference compared with the other groups; group III, CCS9810; group IV, CCS9803; group V: CCS9801, CCS9802, CCS9806, CCS9813, MGl, MG3 and MG9. The sequence data of 12 hpaA segments were analyzed by DNAsis software and it was observed that: (1) The homologies of base pair and amino acid sequence between strains NCTC11637, SS1, CCS9809 were 99.6% and 98.9%, respectively; (2) The homology of base pair and amino acid sequence between CCS9803 and CCS9810 was 97.7% and 99.1%; (3) That of the rest strains, CCS9801, CCS9802, CCS9806, CCS9813, MGl, MG3, MG9 reached 99.4% and 98.4%; (4) The base pair homologies between all hpaA fragments of different sources were higher than 94.6%, therefore the correspondence of deduced amino acid sequence was higher than 96.8% between each other. CONCLUSION: The gene hpaA from different H pylori strains revealed variation, and this might provide an effective method for molecular epidemiological survey of H pylori.

幽门螺杆菌hpaA基因RFLP研究

用限制性片段长度多态性 (RFLP)的方法评价幽门螺杆菌不同菌株鞭毛粘附素基因(hpaA)的变异性。PCR扩增 9株幽门螺杆菌 710bp的hpaA基因 ,用HhaⅠ、HaeⅢ限制性内切酶对该基因片段进行酶切分析。hpaA基因HaeIII单酶切可见 4种带型 ,HhaI单酶切出现 5种带型。从临床分离的H pylori菌株hpaARFLP互有差异 ,且不同于国际标准菌株 ;临床分离株感染动物后分离得到的动物适应株其hpaA基因也发生了变异。不同H pylori菌株间hpaA基因表现出明显的多态性 ,为开展H

抗幽门螺杆菌粘附素HpaA卵黄抗体的制备

目的研制高效价特异性的抗幽门螺杆菌黏附素鸡卵黄抗体免疫球蛋白抗体。方法用纯化重组幽门螺杆菌黏附素(Helicobacter pyloriadhesin A,rHpaA)抗原免疫22周龄罗曼鸡,母鸡免疫应答后,在卵黄中产生抗幽门螺杆菌黏附素抗体;经硫酸铵法初步纯化浓缩后;以间接ELISA鉴定抗体效价及免疫学活性;采用Bradford法测定蛋白含量;并用SDS-PAGE法测定分子量及鉴定抗体纯度。结果母鸡初次免疫第10d即有抗体产生,初次免疫后75d左右抗体效价超过1∶10000;最高可达为1∶12800。卵黄抗体经硫酸铵法纯化后,用SDS-PAGE分析,出现两条蛋白带,纯度达95%以上。其含量为10.56mg/ml蛋黄。结论本研究首次研制并鉴定抗黏附素卵黄抗体,开拓了我国预防幽门螺杆菌感染的新领域,分析了抗体在产蛋期卵黄液中表达的进度,为今后该抗体的持续、高质量诱导奠定基础。有望获得高效价、高产量的抗黏附素的IgY抗体(IgY-HpaA),为制备口服制剂开辟了广阔前景。

血清幽门螺杆菌HpaA抗体与胃癌风险关系的研究

目的探讨幽门螺杆菌感染人群中血清黏附素(HpaA)与胃癌风险之间的关系,为早期胃癌的筛查提供了理论依据,并为胃癌的病因研究提供了新的线索。方法采用以医院为基础的病例对照研究方法,检测重组目的蛋白HpaA在两组人群血清中抗体的水平并分析其抗体水平与胃癌之间的关系。结果全部的研究人群和幽门螺杆菌阳性以及阴性人群中HpaA与胃癌的发病风险有关联(P <0. 001); HpaA的抗体水平与胃癌的发病风险存在剂量反应关系(P <0. 001)。受试者工作特征曲线确定KatA筛查胃癌的最佳截断值为0. 3471时,对应的灵敏度和特异度分别为81. 40%和63. 40%,其曲线下面积为0. 762。结论血清幽门螺杆菌HpaA抗体与胃癌的发病风险有关。

特异性结合幽门螺杆菌黏附蛋白A(HpaA)核酸适配子的筛选及鉴定

目的通过指数富集的配体系统进化技术(SELEX)筛选特异性结合幽门螺杆菌(H.pylori)黏附蛋白A(HpaA)的核酸适配子,并鉴定其结合特性。方法构建pET28a/HpaA原核表达质粒并诱导表达纯化重组HpaA蛋白;以重组HpaA蛋白为靶标利用SELEX技术筛选出能够与HpaA具有高特异性、高亲和力结合的核酸适配子。随后利用筛选所得HpaA适配子通过体外实验验证与H.pylori菌体的结合以及对临床胃黏膜切片中H.pylori的检测效能。结果本研究培养并提取ATCC26695菌株基因组,通过PCR扩增HpaA部分基因长度约699 bp,并成功克隆构建了原核表达质粒pET28a/HpaA。经异丙基β-D-半乳糖苷(IPTG)诱导表达、纯化获得纯度约98%的重组HpaA蛋白作为筛选靶标。利用SELEX技术通过10轮正向筛选和5轮的负向筛选,获得6条与HpaA高亲和力的适配子分别命名为HA1~HA6。其中适配子HA6具有较高的亲和力和特异性,且适配子HA6核心序列在体外仍表现出与H.pylori菌体较高的结合力;利用羟基荧光素(FAM)标记的HA6适配子对166例H.pylori感染的患者胃黏膜中H.pylori进行检测,检出率为94.58%,高于同批次快速脲酶检测法的检出率(87.95%)。结论本研究筛选出的特异性结合H.pylori菌体表面HpaA的适配子,可能作为一种新的方法应用于胃黏膜组织中H.pylori的检测。

抗幽门螺杆菌黏附素蛋黄抗体与HP1188蛋黄抗体在小鼠体内防治幽门螺杆菌感染的比较

目的比较抗幽门螺杆菌黏附素(Helicobacter pylori adhesin A,HpaA)蛋黄抗体(immunoglobulin yolk,IgY)(HpaA-IgY)及抗H.pylori HP1188 IgY(HP1188-IgY)在BALB/c小鼠体内预防和治疗H.pylori感染的最低浓度,并评价治疗效果。方法Western blot鉴定HpaA-IgY及HP1188-IgY抗原特异性。制备1×10^9 CFU/mL H.pylori菌液,将BALB/c小鼠随机分为阳性对照组(灌喂H.pylori菌液0.5 mL)、阴性对照组(以布氏肉汤替换H.pylori)、预防组(先灌喂1、3、5 mg/mL HpaA-IgY或HP1188-IgY及PBS各1 mL,再灌喂H.pylori菌液0.5 mL)、治疗组(先灌喂H.pylori菌液0.5 mL,再灌喂1、3、5 mg/mL HpaA-IgY或HP1188-IgY及PBS各1 mL)。处理完成后,取各组小鼠胃组织进行H.pylori培养、快速尿素酶试验(rapid urease test,RUT)及组织学检查,观察H.pylori定植及炎症反应情况。结果经Western blot分析,HpaA-IgY及HP1188-IgY分别与重组HpaA和HP1188蛋白发生特异性结合。阳性及PBS对照组小鼠感染率均为100%。与PBS对照组比较,5 mg/mL HpaA-IgY及3 mg/mL HP1188-IgY预防组和治疗组感染率均降低,RUT、H.pylori定植及炎症程度评分均显著降低(P均<0.05),均达到较理想的预防和治疗效果。结论HpaA-IgY及HP1188-IgY对感染H.pylori小鼠均有预防和治疗双重作用,剂量选择HP1188-IgY优于HpaA-IgY。本文为制备防治H.pylori感染的口服生物制品提供了参考。