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一种用于检测循环免疫复合物中杜氏利什曼原虫抗原的聚乙二醇酶联免疫吸附测定法。

A PEG-ELISA for the detection of Leishmania donovani antigen in circulating immune complexes.

作者信息

Azazy A A, Devaney E, Chance M L

机构信息

Biomedical Science Division, Liverpool School of Tropical Medicine, UK.

出版信息

Trans R Soc Trop Med Hyg. 1994 Jan-Feb;88(1):62-6. doi: 10.1016/0035-9203(94)90502-9.

Abstract

Leishmanial antigen in circulating immune complexes (CIC) from sera of cotton-rats experimentally infected with Leishmania donovani and visceral leishmaniasis patients (VLP) was detected using a polyethylene glycol (PEG) enzyme-linked immunosorbent assay (PEG-ELISA). The immune complexes were precipitated in the cold with 12% PEG (average M(r) 6000) and then dissociated with glycine-HCl buffer. The dissociated antigen bound to the plate was then detected by peroxidase-labelled rabbit antibody raised to either amastigotes or to CIC. Serum samples from either controls or patients infected with heterologous organisms were used to define the sensitivity and specificity of the test. Leishmanial antigen was detected in the CIC from all experimentally infected animals (100% sensitivity) and in 22 of 25 of the CIC from VLP (88% sensitivity), using either conjugate. Immunoblotting of PEG-precipitated CIC from infected animals with both rabbit antisera revealed multiple antigen components. Antigens of 40, 42 and 45 kDa appeared to be specifically recognized by both antibodies; the components of 40 and 42 kDa were common to amastigote extracts and CIC from infected animals.

摘要

采用聚乙二醇(PEG)酶联免疫吸附测定法(PEG-ELISA)检测了实验感染杜氏利什曼原虫的棉鼠血清以及内脏利什曼病患者(VLP)血清中循环免疫复合物(CIC)中的利什曼原虫抗原。免疫复合物在低温下用12%的PEG(平均相对分子质量6000)沉淀,然后用甘氨酸 - 盐酸缓冲液解离。解离后结合在平板上的抗原随后用抗无鞭毛体或抗CIC的过氧化物酶标记兔抗体进行检测。使用来自对照或感染异源生物体患者的血清样本确定该检测方法的敏感性和特异性。使用任何一种结合物,在所有实验感染动物的CIC中均检测到利什曼原虫抗原(敏感性100%),在25例VLP患者的CIC中有22例检测到(敏感性88%)。用两种兔抗血清对感染动物的PEG沉淀CIC进行免疫印迹分析,发现了多种抗原成分。40、42和45 kDa的抗原似乎能被两种抗体特异性识别;40和42 kDa的成分在无鞭毛体提取物和感染动物的CIC中都有。

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