疟原虫抗原B表位NKND在鼠伤寒沙门氏菌鞭毛蛋白中的表达

疟原虫抗原Ｂ表位ＮＫＮＤ是由本课题组首先报道的一个新的疟疾抗原表位,它是存在于多种不同疟原虫分离株中的保守序列,以减毒沙门菌为载体制备口服活疫苗,方法简单,使用方便,其鞭毛蛋白有较强的免疫原性,有利于激发人体的细胞和体液免疫,人工合成８肽的实验中发现ＮＫＮＤＤ可增强ＮＫＮＤ相应抗体的亲和力,将人工合成的ＮＫＮＤＤ寡核苷酸片段插入鼠伤寒沙门氏菌鞭毛蛋白表达体系中,经Ｗｅｓｔｅｒｎ杂交鉴定,表达出具有     

恶性疟原虫多抗原表位基因的融合与表达

本研究以霍乱毒素B亚基(CT-B)基因为载体,构建了含不同抗原表位的恶性疟原虫的融合基因CTB/ATE和CTB/AWTE。前者除含有恶性疟原虫裂殖子表面主要抗原表位杂合多肽基因SPf66外,还含有很强的T辅助细胞表位CST3和Tc细胞表位;后者在此基础上将我国发现的B细胞表位NKNDD基因经8次串联后融合其中、两种形式的融合基因经测序正确后转入大肠杆菌TK1046中,产量分别为10mg/L及5mg/L。表达产物CTB/AWTE经亲和层析纯化的双抗夹心ELISA测定表明,该融合蛋白在保留了与抗CTB抗体结合的同时,与抗NKNDD单抗的结合效价达1∶8000。     

人精子膜蛋白片段在沙门氏菌中的表达——一种制备抗生育疫苗的途径(英文)

合成编码一种人精子膜蛋白YWK-Ⅱ胞外区的一段多肽片段的双链寡核昔酸链,HSD—2a。用平端连接的方法将其插入到沙门氏菌鞭毛基因fliC(d)的抗原表位IV高变区EcoRV位点,构建了重组质粒pLS408-H1。重组基因在鞭毛负性aroA基因缺失的无致病性沙门氏菌S.dublin SL5928疫苗菌株中表达。经ELISA、电镜免疫胶体金法检测,表明HSD-2a编码的多肽片段成功地在沙门氏菌鞭毛表面表达。融合鞭毛蛋白分子量约为60kD。Western-Blot法检测,提纯的融合鞭毛蛋白与YWK-Ⅱ小鼠抗血清只在60 kD处出现一条结合带。携带重组质粒pLS408—H1的沙门氏菌疫苗菌株极有可能成为抗生育疫苗。     

恶性疟原虫74肽抗原基因在减毒鼠伤寒沙门氏菌的表达和家兔免疫应答

利用减毒鼠伤寒沙门氏菌来表达外源抗原并制备口服活菌苗,是疫苗研究的一个新的突破。作者已在减毒鼠伤寒沙门氏菌SL3261以β—半乳糖苷酶(GZ)融合蛋白的形式表达了人工合成的恶性疟原虫74肽基因HGFC。现报道用活菌SL3261(pWRC)(C组)、SL3261(pWR450-1)(R组)分别免疫新西兰家兔,研究其在家兔体内免疫应答的结果。     

应用噬菌体随机肽库技术筛选鼠疫耶尔森菌F1抗原中和性表位

目的:筛选鼠疫耶尔森菌F1抗原的中和性表位,构建基于鞭毛蛋白佐剂的重组表位疫苗。方法:利用鼠疫菌F1抗原的中和抗体F2H5筛选噬菌体随机12肽库,对得到的阳性克隆采用ELISA进行特异性鉴定,采用竞争抑制ELISA确定具有竞争性的噬菌体单克隆并对其DNA测序,重组表达并纯化获得肽序列与截短型鞭毛蛋白Fli Cdel的融合蛋白,并通过Western印迹和ELISA鉴定重组蛋白与F2H5的结合。结果:获得了2株能够与F1抗原竞争结合F2H5的噬菌体单克隆12-1和12-14,其中12-14的竞争能力较强;通过序列比对,并没有发现这2株噬菌体克隆的插入肽序列与F1抗原序列存在一致性,但这2个插入肽序列与Fli Cdel的重组蛋白在Western印迹和ELISA结果中均显示出能够被抗F1的单克隆抗体识别。结论:F1中和性抗体筛选出的肽序列与截短的鞭毛蛋白融合表达后能够被F2H5特异性识别,为进一步对重组表位抗原进行免疫保护评价奠定了基础。     

恶性疟原虫DNA疫苗免疫效果的评估

以霍乱毒素Ｂ亚基（ＣＴＢ）为载体,由其基因构建了含有不同时期不同抗原表位的恶性疟原虫的融合基因ＣＴＢ～ＡＷＴＥ、ＣＴＢ～ＮＡＮＰ,前者除含有恶性疟原虫裂殖子表面主要抗原表位杂合多肽基因ＳＰｆ６６外,还含有很强的Ｔ辅助细胞表位ＣＳＴ３和Ｔｃ细胞表位,后者含有子孢子期的Ｂ、Ｔｈ细胞表位。将纯化的质粒免疫Ｂａｌｂ．ｃ纯系小鼠,３次免疫后诱导机体产生了体液免疫和细胞免疫,免疫的小鼠进行疟原虫子孢子攻击实验     

沙门菌鞭毛抗原及其多样性研究进展

沙门菌鞭毛蛋白具有抗原性。鞭毛分型抗原有多种,抗原特异性取决于氨基酸序列和种类的不同,抗原表位在鞭毛蛋白二级结构的可变区部位,在分子水平上抗原决定区位于鞭毛基因中间可变区中。利用分型抗原特异性建立起来的免疫学检测被广泛应用。沙门菌属特异性共同抗原具有属特异性,广泛分布于沙门菌全属。共同抗原具有序列保守性和构像稳定性,在沙门菌属内同源性高,ELISA试验表明此抗原免疫原性较好,利用此抗原属特异性建立起免疫学检测沙门菌属已得到应用。     

以ISA720为佐剂甘氨酸作为保护剂的恶性疟疾疫苗AMA1的长期稳定性

<正>恶性疟原虫顶端膜抗原(AMA1)是恶性疟原虫无性繁殖血液期表达的蛋白,是恶性疟疾疫苗的候选抗原。AMA1蛋白是疟原虫FVO和3D7等位基因表达产物,恶性疟疾候选疫苗AMA1-C1/ISA720     

以ISA720为佐剂甘氨酸作为保护剂的恶性疟疾疫苗AMAl的长期稳定性

恶性疟原虫顶端膜抗原（AMA1）是恶性疟原虫无性繁殖血液期表达的蛋白,是恶性疟疾疫苗的候选抗原。AMA1蛋白是疟原虫FVO和3D7等位基因表达产物,恶性疟疾候选疫苗AMA1-C1／ISA720是AMA1抗原与佐剂MontanideISA720按照1：1（质量比）配伍混合合成的。为了将来在大规模人群中接种的需要,     

恶性疟原虫多抗原表位基因表达载体的构建及其在大豆幼胚中的表达

疟疾是当今最需要研究有效疫苗的主要传染病之一。AWTE基因编码恶性疟原虫多种抗原表位基因 ,CTB基因编码霍乱毒素 B亚基 ,是一种既能引起细胞免疫又能引起体液免疫的免疫载体和佐剂。把 AWTE- CTB融合基因构建到植物表达载体 p BVG- ny2上 ,通过基因枪导入法 ,转化大豆幼胚分生组织。 X- glu染色检测到 GUS基因的表达 ;抗原性分析实验结果表明 ,特异表达的融合蛋白可与 CTB和 AWTE抗体结合 ,具有 CTB抗原性。这个实验结果 ,表明疟疾多抗原表位基因首次在转基因大豆幼胚中得到瞬时表达     

疟疾多抗原表位基因表达载体的构建及其在烟草中的表达

本文首次报道疟疾多表位抗原基因在转基因烟草中表达成功。疟疾是当今最需要研究有效疫苗的主要传染病之一。过去的研究表明,ＡＷＴＥ基因编码的疟疾多种抗原表位是有效的抗疟表位,ＣＴＢ基因编码的霍乱毒素Ｂ亚基,是一种既能引起细胞免疫又能引起体液免疫的免疫载体和佐剂。本研究把ＡＷＴＥ－ＣＴＢ融合基因构建到植物表达载体ｐＢＶＧ－ｎｙ１上,采用共转化的方法,通过基因枪导入转化烟草。经ＰＣＲ扩增ＡＷＴＥ－ＣＴＢ基因片段检测,证实了疟疾多表位抗原基因在转基因烟草中的整合。ＳＤＳ－ＰＡＧＥ蛋白电泳结果显示转基因烟草中表达了ＡＷＴＥ－ＣＴＢ融合基因分子量相同的特异蛋白。经抗原性分析实验和Ｗｅｓｔｅｒｎ免疫印迹实验结果表明,特异表达的融合蛋白可与ＣＴＢ和ＡＷＴＥ抗体结合,具有ＣＴＢ和ＡＷＴＥ抗原性。     

Variable wavelength surface plasmon resonance (SPR) in biosensing

In this study, we fabricated a novel variable wavelength surface plasmon resonance (SPR) sensor, which detects resonance conditions such as a maximum attenuation wavelength, measuring change of microscopic refractive index. Such a change was measured to detect a salmonella antigen–antibody reaction and a penicillinase–penicillin reaction. Our experiments were performed after immobilizing a salmonella antibody on the sensor chip. We measured the shift in resonant wavelength during the antigen–antibody reaction for 30 min by injecting 5 × 10⁷ cells/ml concentration of salmonella antigen solution into the sample chamber. Also, after immobilizing penicillinase on the sensor chip, we measured the shift in resonant wavelength during the reaction. Penicillin solution at 10 mM was injected into the sample chamber. The shift of resonant wavelength for each experiment was measured using a white light source, multimode optical fiber, a part of sensor chip and an optical spectrum analyzer.As a result, the resonant wavelength shifted about 0.26 nm/min owing to the salmonella antibody–antigen reaction. Thus, we could detect the change in wavelength (0.8 nm/min) through the interaction of penicillin and penicillinase for 15 min using variable wavelength SPR sensor.     

Generation and characterization of a PhoP homologue mutant of Neisseria meningitidis

Two-component regulatory systems are important regulators of virulence genes in a number of bacteria. Genes encoding a two-component regulator system, with homology to the phoP/phoQ system in salmonella, were identified in the meningococcal genome. Allele replacement was used to generate a meningococcal knock-out mutant of the regulator component of this system, and its phenotype was examined. The mutant displayed many differences in protein profiles compared with wild type, consistent with it being a gene-regulatory mutation. Many of the growth characteristics of the mutant were similar to those of phoP mutants of salmonella: it was unable to grow at low concentrations of magnesium and was sensitive to defensins and other environmental stresses. Magnesium-regulated differences in protein expression were abrogated in the mutant, indicating that the meningococcal PhoP/PhoQ system may, as in salmonella, respond to changes in environmental magnesium levels. These results are consistent with the PhoP homologue playing a similar role in the meningococcus to PhoP in salmonella and suggest that it may similarly be involved in the regulation of virulence genes in response to environmental stimuli in the meningococcus. In support of this conclusion, we found the mutant grew was unable to grow in mouse serum and was attenuated in its ability to traverse through a layer of human epithelial cells. Identification of those genes regulated by the meningococcal PhoP may provide a route towards the identification of virulence genes in the meningococcus.     

Transduction complicates the detection of conjugative ability in lysogenic salmonella strains

When lysogenic salmonella strains were examined for conjugative ability in tri-parental crosses, false positive results were sometimes obtained because phage carried by the lysogenic strains multiplied on the intermediate salmonella recipient strain and then transduced its streptomycin/sulphonamide resistance plasmid to the final salmonella recipient strain. Back transfer of the plasmid to the lysogenic strains was also detected.     

辽宁省鼠伤害沙门氏菌噬菌体分型的研究

本文报道了辽宁省不同来源鼠伤寒沙门氏菌噬菌体型的分布情况。实验结果表明：１５１株鼠伤寒沙门氏菌能分型者１４７株,分型率高达９７．３５％;１４７株鼠伤寒沙门氏菌可分成１４个噬菌体型,其中４７７４型（４６．２６％）、７７７７型（２４．４９％）、６７７４型（１１．５６％）、４０００型（６．８０％）。上述４型为辽宁省鼠伤寒沙门氏菌优势噬菌体型（８９．１２％）。辽宁省各种来源鼠伤寒沙门氏菌均以４７７４型最为常见,肠炎病人和健康带菌者型别众多,医院交叉感染病人型别相对集中,食物中毒鼠伤寒沙门氏菌流行型别为４７７４型和６７７４型。     

Salmonella carrier state and biological characteristics of the infectious agent

Salmonella carrier state (42.6%-S. enteritidis and 34.4%-S. dublin) was demonstrated in subjects after acute salmonellosis as well as in healthy persons infected with salmonella as a result of occupational exposure to poultry (8.8% in humans exposed to chickens and 6.1% in those exposed to ducks) and sheep (2.8%). The carrier state was accompanied by intermittent pain in the epigastrium, diminished appetite, diarrhoea etc. Most of the carrier subjects with a history of salmonellosis exhibited, upon rectoromanoscopy, a varying degree of proctosigmoiditsi. The etiological role of S. typhimurium was proved beyond doubt, as well as its ability to cause salmonellosis outbursts, sporadic cases of the disease and the carrier state. When large industrial facilities specializing in poultry processing were investigated, the salmonella carrier state was revealed in practically healthy poultry--in 16% of chickens and 12% of ducks. The salmonella organisms isolated from carrier persons had, with some exceptions, typical properties, being virulent in that they caused death of experimental animals, seeded their internal organs and induced pathogenicity-associated enzymes. Multiple resistance to antibiotics was demonstrated in salmonella isolated from poultry; also determined was its plasmid nature. Pronounced resistance of the above salmonella subtypes to tetracycline-related antibiotics and streptomycin may be due to the fact that these drugs are used in poultry raising.     

Transfer Agent of Immunity

Detection of the cells which contain antibody was accomplished by a method of immune adherence of human erythrocytes to a single cell, termed SCIA (single cell immune adherence) reaction. Peritoneal exudate cells were collected from mice immunized with flagella of either Salmonella enteritidis or S. tennessee. Serologically specific antibody was detectable in some of the peritoneal exudate cells of such mice. An immune ribonucleic acid (RNA) was extracted from the peritoneal exudate cells of mice immunized with salmonella flagella. When mice were injected intraperitoneally with this preparation, serologically specific antibody was found in some of their peritoneal exudate cells by the SCIA method. This preparation was inactivated by treatment with ribonuclease, but was resistant to proteinases, deoxyribonuclease and anti-flagella antibody, suggesting that this agent is of RNA nature and does not contain antigen or fragment thereof.     

Comparative Studies on Enrichment And Selective Media for Isolation of Salmonellae from Faecal Specimens

Enrichment media (tetrathionate, selenite and Rapp ap ort broths) and selective media (desoxycholate citrate agar and brilliant green agar) were tested in different combinations to ascertain their capacity for isolation of salmonella bacteria. The material consisted of 299 samples of cattle faeces from two herds infected with salmonella (Table 1), and of 111 artificially contaminated samples of pig faeces (Table 3). The tetrathionate and selenite broths were equally useful for the material as a whole, whereas the results varied between different species of salmonella which is of great practical interest. The number of salmonella isolations was much lower when enrichment with Rappaport broth was used. The rate of salmonella isolations can often be increased by parallel enrichments with two different media. Of the selective agar media tested, brilliant green agar was superior to desoxycholate citrate agar.     

Microbially mediated growth suppression and death of salmonella in composted sewage sludge

The role of compost microflora in the suppression of salmonella regrowth in composted sewage sludge was investigated. Microbial inhibition studies of salmonella growth were conducted on nutrient agar, in composts that had been subjected to different temperatures in compost piles, and in radiation sterilized composts inoculated with selected fractions of the compost microflora. Agar assays of inhibition indicated that bacteria and actinomycetes were not suppressive to salmonellae, but a few fungi were. However, compost inoculation assays showed consistently that fungi were not suppressive, but bacteria and actinomycetes were. In compost inoculation assays, microbial antagonists, when present, either killed salmonellae or reduced their growth rate. No suppression of salmonellae occurred in compost taken from 70°C compost-pile zones despite the presence and growth of many types of microbes. With greater numbers and kinds of microbes in 55°C compost, salmonella growth was suppressed 100–10,000-fold. Salmonellae died when inoculated into compost from unheated zones (25–40°C) of piles. Prior colonization of compost with only noncoliform gram-negative bacteria suppressed salmonellae growth 3,000-fold. Coliforms when inoculated prior to salmonellae accounted for 75% of salmonella die-off. Mesophilic curing to allow colonization of curing piles in their entirety by gram-negative bacteria, especially coliforms, should be an effective way to prevent repopulation by salmonellae.     

Inhibition of the Metabolism of Streptococci and Salmonella by Specific Antisera

Streptococcal and salmonella antisera inhibited carbohydrate metabolism for groups A, B, C, and D streptococci and group E salmonella, as measured by the formation of [(14)C]dioxide from [(14)C]glucose metabolism. For salmonella, the inhibition was type specific since group E salmonella were inhibited only by salmonella E antisera and not by anti-salmonella A or C(1). For streptococci, quantitative differences were demonstrated, but major cross-reactivity was observed. At high concentrations, the antisera were bactericidal; at more dilute concentrations, for both salmonella and streptococci, carbohydrate metabolism was suppressed, but subculture on chocolate agar showed abundant growth. Cross-reacting antibodies could be absorbed by incubation with either antigen, e.g., streptococcal antisera versus heat-killed salmonella. The results suggest that the radiometric technique can be more sensitive than either capillary flocculation or visual detection of bacterial growth for detecting the inhibition of streptococci and salmonella by specific antibodies. The use of specific antisera may prove useful for bacterial species identification in an automated system for detection of bacterial growth.