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本文引用的文献

1
Size variation of the major immunodominant protein of Cowdria ruminantium.反刍动物立克次氏体主要免疫显性蛋白的大小变异
Clin Diagn Lab Immunol. 1994 Nov;1(6):744-6. doi: 10.1128/cdli.1.6.744-746.1994.
2
Development of a single dilution ELISA to detect antibody to Dermatophilus congolensis in goat and cattle sera.用于检测山羊和牛血清中刚果嗜皮菌抗体的单稀释酶联免疫吸附测定法的开发。
Vet Microbiol. 1993 Jan;34(1):47-62. doi: 10.1016/0378-1135(93)90006-s.
3
Standardisation and validation of enzyme-linked immunosorbent assay techniques for the detection of antibody in infectious disease diagnosis.用于传染病诊断中抗体检测的酶联免疫吸附测定技术的标准化与验证
Rev Sci Tech. 1993 Jun;12(2):435-50. doi: 10.20506/rst.12.2.691.
4
An immunoblotting diagnostic assay for heartwater based on the immunodominant 32-kilodalton protein of Cowdria ruminantium detects false positives in field sera.一种基于反刍动物考德里氏体免疫显性32千道尔顿蛋白的牛心水病免疫印迹诊断检测方法在现场血清中检测到假阳性。
J Clin Microbiol. 1993 Oct;31(10):2729-37. doi: 10.1128/jcm.31.10.2729-2737.1993.
5
The immunodominant 32-kilodalton protein of Cowdria ruminantium is conserved within the genus Ehrlichia.反刍动物考德里氏体的免疫显性32千道尔顿蛋白在埃立克体属内保守。
Rev Elev Med Vet Pays Trop. 1993;46(1-2):145-52.
6
The sero-diagnosis of heartwater: a comparison of five tests.心水病的血清学诊断:五种检测方法的比较
Rev Elev Med Vet Pays Trop. 1993;46(1-2):123-9.
7
Detection of antibodies to Cowdria ruminantium in the serum of domestic ruminants by indirect ELISA.用间接酶联免疫吸附测定法检测反刍家畜血清中抗反刍兽立克次氏体的抗体
Rev Elev Med Vet Pays Trop. 1993;46(1-2):115-20.
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Heartwater in Guadeloupe and in the Caribbean.瓜德罗普岛及加勒比地区的心水病
Rev Elev Med Vet Pays Trop. 1993;46(1-2):109-14.
9
Molecular cloning, sequence analysis, and expression of the gene encoding the immunodominant 32-kilodalton protein of Cowdria ruminantium.反刍动物考德里氏体免疫显性32千道尔顿蛋白编码基因的分子克隆、序列分析及表达
Infect Immun. 1994 Apr;62(4):1451-6. doi: 10.1128/iai.62.4.1451-1456.1994.
10
Correlation between antibodies to Cowdria ruminantium (rickettsiales) in cattle and the distribution of Amblyomma vector ticks in Zimbabwe.津巴布韦牛体内反刍动物考德里氏体(立克次氏体目)抗体与钝缘蜱传播媒介蜱分布的相关性
Exp Appl Acarol. 1993 Nov;17(11):799-810. doi: 10.1007/BF00225853.

在血清学检测中使用反刍动物考德里氏体MAP1蛋白上的特定免疫原性区域。

Use of a specific immunogenic region on the Cowdria ruminantium MAP1 protein in a serological assay.

作者信息

van Vliet A H, van der Zeijst B A, Camus E, Mahan S M, Martinez D, Jongejan F

机构信息

Department of Bacteriology, Faculty of Veterinary Medicine, Utrecht University, The Netherlands.

出版信息

J Clin Microbiol. 1995 Sep;33(9):2405-10. doi: 10.1128/jcm.33.9.2405-2410.1995.

DOI:10.1128/jcm.33.9.2405-2410.1995
PMID:7494037
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC228424/
Abstract

Currently available serological tests for cowdriosis (Cowdria ruminantium infection) in domestic ruminants are hampered by their low specificities because of cross-reactivity with Ehrlichia spp. The use of recombinant major antigenic protein (MAP1) of C. ruminantium for serodiagnosis was investigated. Overlapping fragments of the MAP1 protein were expressed in Escherichia coli and were reacted with sera from sheep infected with either C. ruminantium or Ehrlichia ovina. Two immunogenic regions on the MAP1 protein, designated MAP1-A and MAP1-B, were identified. MAP1-A was reactive with C. ruminantium antisera, E. ovina antisera, and three MAP1-specific monoclonal antibodies, whereas MAP1-B reacted only with C. ruminantium antisera. An indirect enzyme-linked immunosorbent assay (ELISA) based on MAP1-B was further developed and validated with sera from animals experimentally infected with C. ruminantium or several Ehrlichia spp. Antibodies raised in sheep, cattle, and goats against nine isolates of C. ruminantium reacted with MAP1-B. Cross-reactivity with MAP1-B was limited to Ehrlichia canis and Ehrlichia chaffeensis, two rickettsias which do not infect ruminants. Antibodies to Ehrlichia spp. which do infect ruminants (E. bovis, E. ovina, and E. phagocytophila) did not react with MAP1-B. Antibody titers to C. ruminantium in sera from experimentally infected cattle, goats, and sheep were detectable for 50 to 200 days postinfection. Further validation of the recombinant MAP1-B-based ELISA was done with sera obtained from sheep raised in heartwater-free areas in Zimbabwe and from several Caribbean islands. A total of 159 of 169 samples which were considered to be false positive by immunoblotting or indirect ELISA did not react with MAP1-B. In conclusion, recombinant MAP1-B may be a suitable antigen for a sensitive serological test for cowdriosis, with dramatically improved specificity.

摘要

目前用于家畜牛心水病(反刍动物立克次氏体感染)的血清学检测,因与埃立克体属存在交叉反应,特异性较低而受到阻碍。本研究对反刍动物立克次氏体的重组主要抗原蛋白(MAP1)用于血清诊断进行了调查。MAP1蛋白的重叠片段在大肠杆菌中表达,并与感染反刍动物立克次氏体或绵羊埃立克体的绵羊血清发生反应。在MAP1蛋白上鉴定出两个免疫原性区域,分别命名为MAP1 - A和MAP1 - B。MAP1 - A与反刍动物立克次氏体抗血清、绵羊埃立克体抗血清以及三种MAP1特异性单克隆抗体发生反应,而MAP1 - B仅与反刍动物立克次氏体抗血清反应。基于MAP1 - B进一步开发了间接酶联免疫吸附测定(ELISA),并用实验感染反刍动物立克次氏体或几种埃立克体属的动物血清进行了验证。在绵羊、牛和山羊体内针对九株反刍动物立克次氏体分离株产生的抗体与MAP1 - B发生反应。与MAP1 - B的交叉反应仅限于犬埃立克体和恰菲埃立克体,这两种立克次氏体不感染反刍动物。感染反刍动物的埃立克体属(牛埃立克体、绵羊埃立克体和吞噬细胞埃立克体)的抗体不与MAP1 - B反应。在实验感染的牛、山羊和绵羊血清中,感染后50至200天可检测到针对反刍动物立克次氏体的抗体滴度。利用从津巴布韦无牛心水病地区以及几个加勒比岛屿饲养的绵羊获得的血清,对基于重组MAP1 - B的ELISA进行了进一步验证。在169个通过免疫印迹或间接ELISA被认为是假阳性的样本中,共有159个不与MAP1 - B反应。总之,重组MAP1 - B可能是一种适用于牛心水病敏感血清学检测的抗原,其特异性有显著提高。