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日本血吸虫病肠相关与卵相关抗原血症检测的诊断互补性初报
引用本文:陆萍,邱东川,钱宗立. 日本血吸虫病肠相关与卵相关抗原血症检测的诊断互补性初报[J]. 中国寄生虫学与寄生虫病杂志, 1995, 0(1)
作者姓名:陆萍  邱东川  钱宗立
作者单位:上海第二医科大学寄生虫学教研室(陆萍),四川省寄生虫病防治研究所(邱东川),莱登大学寄生虫学研究室(钱宗立)
摘    要:应用经羟基磷灰石纯化,偶联长链生物素BACH(Biotinaminocaprylhydrazide)的两株主要识别卵相关不同表位的单克隆抗体建立检测灵敏度达微微克水平的硷性磷酸酶抗原捕获酶联试验(BA-APELISA),对粗制日本血吸虫卵抗原SEAj-TCA的检测极限,2H10-ELISA可达1—0.3ng/ml,仅有效地检出日本血吸虫种特异的卵抗原表位分子;而2H1-ELISA则达3.2ng/ml,亦能灵敏地检示曼氏血吸虫的卵抗原组分。两组试验反复试用于日本血吸虫病例及正常人群血样检测,显示有非常明显的OD消光读数差异。同时采用已建立的1B10-APELISA检测肠相关CAA系列,以平行检测的健康对照组消光OD均值+3SD为阳性界值,对3组采自不同流行区的慢性或混合型病例同批血样进行肠相关CAA及卵相关2H10和2H1的二联或三联叠加检测,其累计检出率都得到不同程度的提高,尤以低度流行区的慢性病例组更为明显。

关 键 词:循环抗原  抗原血症  血吸虫表位血清学  单克隆抗体  互补检测

A PRELIMINARY REPORT ON DIAGNOSTIC COMPLEMENTARITY OF GUT ASSOCIATED AND EGG ASSOCIATED ANTIGENEMIA IN SCHISTOSOMIASIS JAPONICA
Lu Ping ,Qiu Dongchuan ,Qian Zongli ,Andre M Deelder. A PRELIMINARY REPORT ON DIAGNOSTIC COMPLEMENTARITY OF GUT ASSOCIATED AND EGG ASSOCIATED ANTIGENEMIA IN SCHISTOSOMIASIS JAPONICA[J]. Chinese Journal of Parasitology and Parasitic Diseases, 1995, 0(1)
Authors:Lu Ping   Qiu Dongchuan   Qian Zongli   Andre M Deelder
Affiliation:Lu Ping 1,Qiu Dongchuan 2,Qian Zongli 1,Andre M Deelder 3 1 Department of parasitology,Shanghai Second Medical University,Shanghai 200025 2 Sichuan Provincial Institute of Parasitic Diseases,Chengdu 610041 3 Labora
Abstract:With Hyroxylapatite purified preparations and BACH(biotin aminocapryl hydrazide) biotinylated McAbs, 274 2H10 and 273 2H1,recognizing different egg associated epitopes, biotin avidin(BA)involved alkaine phosphatase (AP) ELISA with detecting sensi tivities reaching nanogram levels (10 -9 ) were set up. The detectable limit for crude preparations of Schistosoma japonicum SEAJ TCA in 2H10 ELISA achieved 1.0 3.2 ng/ml, in which only S. japonicum specific egg antigens were efficiently detected, whereas with 2H1 ELISA, which could detect SEA TCA of both S. japonicum and S. mansoni species, an end point of detecting 3.2 ng/ml was obtained. Repeated tests with human serum groups revealed very significant differences of extinction OD readings between patients and normal individuals. For detection combinations, a previously established anti CAA homologous AP ELISA system was parallelly used for gut associated antigenemia determinations. Taking the mean extinction OD reading of a parallel normal serum group plus 3 SD as corresponding cut off values, 3 patient groups (n=82,52,39) from different areas of transmission intensity were subjected to accumulating determinations for egg and gut associated antigenemiae. Improved detectabilities to variable extent were achieved in either of the 2 or 3 combinations. The study thus demonstrated that the diagnostic efficiency for human schistosomiasis could be improved by multi epitope detections for more than one target molecule using corresponding McAbs, especially in areas where the transmission intensity of the disease is comparatively lower.
Keywords:Circulating antigen   antigenemia   schistosome epitope serology   monoclonal antibody   complementary detection  
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