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抗麻疹病毒血凝素的单克隆抗体与合成肽发生反应。

Monoclonal antibodies against measles virus haemagglutinin react with synthetic peptides.

作者信息

Mäkelä M J, Salmi A A, Norrby E, Wild T F

机构信息

Department of Virology, University of Turku, Finland.

出版信息

Scand J Immunol. 1989 Aug;30(2):225-31. doi: 10.1111/j.1365-3083.1989.tb01205.x.

DOI:10.1111/j.1365-3083.1989.tb01205.x
PMID:2474850
Abstract

The ability of 17 monoclonal antibodies (MoAb) against measles virus haemagglutinin (MV-H) to bind to 10 selected MV-H-specific synthetic peptides was tested in an enzyme immunoassay (EIA). Three peptides representing residues 126-135 (close to the NH2 terminus), 309-318 (middle), and 587-596 (C-terminal) reacted with MoAb designated 48, I29, and 18, respectively. Binding of MoAb I29 to purified virus was abolished after pre-incubation with the peptide 309-318. Similarly, MoAb 48 did not bind to the virus after absorption with the peptide 126-135. Longer peptides of 19 residues from the regions reacting with the MoAb were also synthesized and tested in EIA. None of the MoAb recognized these longer peptides when the latter were bound as free peptides on solid phase. However, MoAb I29 binding to purified virus was blocked equally well by peptides 304-322 and 309-318. In contrast, peptide 121-139 absorbed the reactivity of the MoAb 48 much more weakly than the shorter peptide 126-135, suggesting that the conformation of the longer peptide in solution is different. To analyse affinities in the antigen-antibody reactions, the plates were washed with buffers of varying pH after absorption of the MoAb to MV or peptides. The MoAb I29 bound both to MV and peptide 309-318 with equal affinity, but MoAb 48 and 18 bound to the peptides 126-135 and 587-596 with lower affinity than to the virus. This study indicates that regions corresponding to amino acids 126-135, 309-318, and 587-596 define antigenic sites of the H protein.

摘要

采用酶免疫测定法(EIA)检测了17种抗麻疹病毒血凝素(MV-H)的单克隆抗体(MoAb)与10种选定的MV-H特异性合成肽结合的能力。三种肽分别代表第126 - 135位残基(靠近NH2末端)、第309 - 318位残基(中间位置)和第587 - 596位残基(C末端),它们分别与编号为48、I29和18的MoAb发生反应。用肽309 - 318预孵育后,MoAb I29与纯化病毒的结合被消除。同样,用肽126 - 135吸收后,MoAb 48不再与病毒结合。还合成了与MoAb反应区域的19个残基的更长肽段,并进行EIA检测。当这些更长的肽段以游离肽形式结合在固相上时,没有一种MoAb能识别它们。然而,肽304 - 322和309 - 318对MoAb I29与纯化病毒结合的阻断效果相同。相反,肽121 - 139对MoAb 48反应性的吸收比短肽126 - 135弱得多,这表明溶液中更长肽段的构象不同。为了分析抗原 - 抗体反应中的亲和力,在MoAb与MV或肽结合后,用不同pH的缓冲液洗涤平板。MoAb I29以相同亲和力与MV和肽309 - 318结合,但MoAb 48和18与肽126 - 135和587 - 596的结合亲和力低于与病毒的结合亲和力。这项研究表明,对应于氨基酸126 - 135、309 - 318和587 - 596的区域确定了H蛋白的抗原位点。

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