Molecular cloning and immunological analysis of immunodominant piroplasm surface proteins of Theileria sergenti and T. buffeli.

cDNA libraries of Theileria sergenti and T. buffeli piroplasms were constructed in lambda gt11 and screened with rabbit anti-piroplasm sera. A major antigen of T. sergenti (33 kDa) and that of T. buffeli (34 kDa) was identified from the recombinant phages by using recombinant antigen-selected monospecific antibodies. The reactivities of the cloned proteins with rabbit antisera, infected calf sera and mouse monoclonal antibody suggested that the 33 and 34 kDa proteins expressed species-common and species-specific epitopes. The DNA probes from these recombinant clones showed species-specific hybridizations in Southern blotting with genomic DNA from piroplasms. These results indicate that the Japanese T. sergenti can be distinguishable from the Australian T. buffeli with regard to a polymorphism of the major immunodominant proteins of piroplasm.     

牛瑟氏泰勒虫P33表面蛋白基因的克隆与原核表达

本研究根据GenBank牛瑟氏泰勒虫P33表面蛋白基因设计1对引物,利用全血基因组DNA提取试剂盒提取牛瑟氏泰勒虫全血基因组DNA,PCR扩增得到了大小为786 bp的基因片断,测序分析证明,它与已报道序列的核苷酸同源性可达99%.将该基因与pET-28a(+)载体进行连接,经酶切和PCR鉴定,证明成功构建了含有目的基因片段的重组表达载体pET-28a-P33.将此质粒转化至大肠杆菌Rosetta(DE3)中,用IPTG进行诱导.结果证实,该基因在大肠杆菌中用IPTG诱导4 h时表达量达到高峰,表达产物为分子质量约30.3 ku的融合蛋白,其表达量占菌体总蛋白的43%,以包涵体形式存在;Western blotting试验证明,表达蛋白P33可被牛瑟氏泰勒虫阳性血清所识别,表明该融合蛋白具有较好的反应原性.     

牛瑟氏泰勒虫双拷贝p33表面蛋白基因在原核细胞中的串联表达

为串联融合表达牛瑟氏泰勒虫(Theileria sergenti)p33表面蛋白,本研究根据GenBank中登录的T.sergenti p33基因序列(D87198),在去掉信号肽的部分设计两对引物。PCR扩增出两段相同的p33基因(p331、p332),大小均为684bp,并将两个基因片段按顺序依次插入原核表达载体pGEX-4T-1中构建pGEX-p331-p332(2p33)。将pGEX-2p33重组质粒转化E.coli BL21中进行诱导表达。经SDS-PAGE电泳显示,该融合蛋白获得了高效表达,分子量约为80ku,表达产物以包涵体的形式存在。Western blot试验表明,融合蛋白可被T.sergenti阳性血清识别,具有较好的反应原性。该蛋白的串联融合表达为T.sergenti新型疫苗的研究奠定了基础。     

牛瑟氏泰勒虫P33表面蛋白基因的克隆与序列分析

为分析吉林省流行的牛瑟氏泰勒虫基因序列，根据GenBank上发表的牛瑟氏泰勒虫P33表面蛋白基因序列设计合成一对引物，用PCR方法扩增出牛瑟氏泰勒虫的基因片段，并成功地将该基因纯化后克隆到pGEM-TEasy载体上，将经EcoRⅠ酶切鉴定和PCR鉴定为阳性的重组质粒进行测序。结果表明克隆的基因片段长度为868bp，编码283个氨基酸，有2个潜在的糖基化位点。核苷酸同源性分析表明，该基因片段与韩国株（AF521557）、日本株（AB016280）、俄罗斯株（AB016279）的核苷酸序列同源性分别为99．4％、88.0％、88．1％。     

Characterisation of Theileria parva isolates from Kiambu district, Kenya

Four Theileria parva isolates from Muguga area of Kiambu district, Kenya, were used to establish schizont-infected cell lines. Their protein antigens were then separated by sodium dodecyl sulphate polyacrylamide gel electrophoresis (SDS page). The isolates were subsequently subjected to protein analysis and characterisation by the western immunoblotting technique. Probing for the polymorphic immunodominant molecule (PIM) was done using monoclonal antibody no. 4. SDS page detected up to 20 protein antigens of molecular mass 35,000-180,000 Da. The western blot analysis revealed a greater heterogeneity in the molecular mass (M(r)) of PIM than previously thought. The M(r) of PIM varied between 80 and 90 kDa. The isolates further revealed different densities of surface epitopes with variable reaction to the monoclonal antibody. The implications of these findings to the epidemiology of east coast fever and immunisation programmes are discussed.     

奶牛瑟氏泰勒虫P33表面蛋白基因的克隆及序列分析

研究根据GenBank上发表的牛瑟氏泰勒虫P33表面蛋白的基因序列设计合成1对引物,用PCR方法扩增出了牛瑟氏泰勒虫的基因片段,将该基因纯化后连接到pMDl8-T栽体上,进行序列测定和分析,并用此方法对延边某奶牛场10头奶牛进行了检测.结果表明:10份样品中9份为阳性,所扩增的目的基因核苷酸长为868 bp,共编码283个氨基酸;该段基因片段与牛泰勒虫韩国株核苷酸序列同源性为99.4%,氨基酸同源性为99.3%.     

牛瑟氏泰勒虫P33表面蛋白基因的克隆及在大肠杆菌中的表达

应用PCR方法扩增了牛瑟氏泰勒虫吉林株P33表面蛋白基因片段,并将扩增产物与pMD18-T载体连接,重组质粒经PCR、双酶切鉴定后测序;构建P33重组pGEX-4T-3表达载体,转化大肠杆菌BL-21,经IPTG诱导表达后.进行SDS-PAGE、免疫印记分析.结果显示,获得P33基因完整开放阅读框长868 bp,编码292个氨基酸,与中国株同源性为99.1%;表达的融合蛋白相对分子质量为59 000,能被牛瑟氏泰勒虫阳性血清识别,表明该融合蛋白具有较好的免疫原性.     

Antibodies produced by mice immunized with recombinant vaccinia viruses expressing two different types of a major Theileria sergenti surface antigen (p32) react with the native surface antigen.

A 32 kDa major surface antigen, p32, of Theileria sergenti at the piroplasm stage is the main target of the host immune response. The immunogenic property of the p32 varies in some strains among the population of Theileria sergenti in Japan where the Chitose type and the Ikeda type are the most common varieties. We have constructed vaccinia virus recombinants vv/p32C and vv/p32I which harbor the Chitose and Ikeda types of p32 gene, respectively. It was found that vv/p32C and vv/p32I produced type-specific p32 which did not cross react with the monoclonal antibodies (mAbs) against the other type of p32. When mice were immunized with vv/p32C and vv/p32I, antibodies against p32 were detectable 2 weeks after the immunization, and these antibodies reacted with the native surface antigen in purified T. sergenti merozoite.     

Purification of a 28 kDa Babesia (Theileria) equi antigen and a 29 kDa spurious erythrocyte antigen from in vitro culture through ion exchange chromatography.

An extract of in vitro cultivated Babesia equi was fractionated using a MonoQ anion exchange column. Separation of a 28 kDa B. equi antigen from a 29 kDa spurious erythrocyte antigen, both of which were intensely immunoreactive, was achieved by chromatography of the infected erythrocyte proteins. Using tricine-SDS-PAGE, the 28 kDa antigen of B. equi showed multiple band resolution, while the 29 kDa antigen was consistently resolved as a single band. The 29 kDa antigen was identified in both infected and non-infected erythrocyte extracts. Moreover, B. equi antiserum recognised this antigen in the non-infected erythrocyte extract, and conversely serum from horses not infected with babesia detected the antigen in infected erythrocyte extract. This 29 kDa antigen could represent a horse erythrocyte isoantigen. The purified 28 kDa antigen is specifically recognised by B. equi antisera and therefore could be useful for the production of the recombinant replica and to employ these in further test systems.     

Seroprevalence of antibody to NcSAG1 antigen of Neospora caninum in cattle from Western Java,Indonesia

Neospora caninum can cause fetal abortion and neonatal mortality incattle, and is a cause of economic concern worldwide. This study aimed to determine theprevalence of Neospora caninum-specific antibodies in cattle from WesternJava, Indonesia. Serum samples from 991 cattle from 21 locations were tested forantibodies to N. caninum by using an enzyme-linked immunosorbent assay(ELISA) on the basis of recombinant NcSAG1. The overall seroprevalence was 16.6%, rangingfrom 0 to 87.5% in the sampled locations. The results of this study indicate latentinfection rates of sampled animals were different in each location. Further studies arenecessary to elucidate the relationship between N. caninum infection andabortion in cattle, and to identify risk factors for infection in high-prevalenceenvironments.     

Characterization of bovine coronavirus isolates/from eight different states in the USA.

Bovine coronavirus isolates from eight different states of the USA were compared for their antigenic properties and susceptibility to hygromycin B. Antigenic differences were observed among the isolates in a one-way hemagglutination-inhibition (HI) test using a polyclonal antiserum against the Mebus bovine coronavirus isolate. Differences were observed on isoelectric focusing among viral proteins with isoelectric points between 4.45-4.65. Most of the BCV isolates were susceptible to hygromycin B (0.5 mM) whereas a few hygromycin B resistant isolates were also found.     

Parasites of South African wildlife. II. Helminths of kudu, tragelaphus strepsiceros, from South West Africa/Namibia

A total of 23 kudu, Tragelaphus strepsiceros, were shot at 2-month intervals from June 1983 to April 1984 in the Etosha Game Reserve in the north of South West Africa/Namibia. The parasite survey conducted on these animals yielded 2 cestode and 12 nematode species. Haemonchus vegliai and Cooperia neitzi were the most prevalent nematodes and occurred in 13 animals each, followed by Cooperia acutispiculum and an Onchocerca sp. (9 animals each). The remaining nematodes were present in 4 (17%) or fewer of the antelope. C. neitzi was the most numerous nematode, a total of 3,564 being recovered from all the antelope, followed by C. acutispiculum (2,552) and H. vegliai (1,050). Individual total worm burdens varied from 4-1,326 with 2 kudu harbouring no worms. The mean burden of 399 worms was considered negligible. A single kudu was shot in the Namib-Naukluft Park in the south of the country. This animal harboured no parasites.     

Phylogenetic relationships of Mongolian Babesia bovis isolates based on the merozoite surface antigen (MSA)-1, MSA-2b, and MSA-2c genes

We conducted a molecular epidemiological study on Babesia bovis in Mongolia. Three hundred blood samples collected from cattle grazed in seven different districts were initially screened using a previously established diagnostic polymerase chain reaction (PCR) assay for the detection of B. bovis-specific DNA. Positive samples were then used to amplify and sequence the hyper-variable regions of three B. bovis genes encoding the merozoite surface antigen (MSA)-1, MSA-2b, and MSA-2c. The diagnostic PCR assay detected B. bovis among cattle populations of all districts surveyed (4.4-26.0%). Sequences of each of the three genes were highly homologous among the Mongolian isolates, and found in a single phylogenetic cluster. In particular, a separate branch was formed only by the Mongolian isolates in the MSA-2b gene-based phylogenetic tree. Our findings indicate that effective preventative and control strategies are essential to control B. bovis infection in Mongolian cattle populations, and suggest that a careful approach must be adopted when using immunization techniques.     

Characterization of West Nile virus (WNV) isolates from Assam,India: Insights into the circulating WNV in northeastern India

West Nile virus (WNV) is a mosquito-borne flavivirus that causes subclinical symptoms, febrile illness with possible kidney infarction and encephalitis. Since WNV was first serologically detected in Assam during 2006, it has become recognized as an important etiological agent that causes acute encephalitis syndrome (AES) in addition to endemic Japanese encephalitis virus (JEV). Therefore, isolating and characterizing the currently circulating strain of WNV is important. The virus was isolated from the cerebrospinal fluid (CSF) of two patients that presented with AES. The genotyping of the isolates HQ246154 (WNIRGC07) and JQ037832 (WNIRTC08) based on the partial sequencing of 921 nucleotides (C-prM-E) of the genome placed them within lineage 5 along with other Indian strains isolated prior to 1982, but the present circulating virus formed a distinct subclade. The derived amino acid sequence alignment indicated substitution in A₈₁T and A₈₄P of the capsid region in HQ246154. A cross-neutralization assay suggested substantial antigenic variation between isolates. The pathogenesis in mice that suggested the circulating WNV was neuroinvasive and comparatively more pathogenic than previous strains from India.     

Preparation, assessment and preservation of antigen from Brucella abortus strain 45/20 for use in the rough antigen complement fixation test

Two methods of extraction were used to prepare antigens from Brucella abortus rough strain 45/20. The antigens were assessed for use in the complement fixation test. A suitable antigen was prepared using the saline extraction method of Miller et al. (1976) and used extensively in CF tests. Four methods of preservation were compared; -20 degrees C, -196 degrees C, 0.5% phenol at 4 degrees C, and lyophilisation. The antigen could be stored at -20 degrees C or -196 degrees C for up to 2 years.     

Studies on the parasites of zebras. V. Nematodes of the Burchell's and Hartmann's mountain zebras from the Etosha National Park, South West Africa/Namibia

Nine Burchell's and 6 Hartman's mountain zebras were culled during the 3 climatic periods characteristic of the Etosha National Park, South West Africa/Namibia, and were examined for helminths. The Burchell's zebras ranged in age from 4 1/2 to 19 years and the mountain zebras from 3 1/2 to 13 years. Twenty-five species of nematodes, belonging to the families Atractidae, Strongylidae, Oxyuridae, Onchocercidae and Habronematidae, were recovered. Of the family Cyathostominae, the following species were the most numerous in the Burchell's zebras: Cyathostomum montgomeryi (7 120-67 042), Cylicocyclus triramosus (11-34 540), Cylicostephanus minutus (4 698-40 019) and Cylindropharynx sp. (? intermedia) (3 591-40 018). The atractids present were: Crossocephalus viviparus (20-5 045 212) and Probstmayria vivipara (5 140-3 801 300). Three of the above cyathostome species were also most abundant in mountain zebras: Cylicocyclus triramosus (54-19 782), Cylicostephanus minutus (555-12 396) and Cylindrophrynx sp. (? intermedia) (3-5 325). New reports include Cylicostephanus longiconus in the Burchell's zebras and Cyathostomum alveatum, Cyathostomum montgomeryi, Cylicostephanus bidentatus and Draschia megastoma in the mountain zebra. The overwintering of 4th stage cyathostomes in the gut walls and their emergence which differ in the 2 hosts, are discussed.