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百日咳毒素S4亚基上B细胞表位的鉴定

Identification of B-cell epitopes on the S4 subunit of pertussis toxin.

作者信息

Ibsen P H, Holm A, Petersen J W, Olsen C E, Heron I

机构信息

Bacterial Vaccine Department, Statens Seruminstitut, Copenhagen, Denmark.

出版信息

Infect Immun. 1993 Jun;61(6):2408-18. doi: 10.1128/iai.61.6.2408-2418.1993.

Abstract

The main purpose of the present study was to identify B-cell epitopes on the S4 subunit of pertussis toxin (PT) by the synthetic peptide approach. Two strategies were followed: (i) screening of two series of overlapping peptides (12- and 25-residue peptides) covering the entire S4 sequence by a panel of murine monoclonal anti-PT antibodies and various polyclonal anti-PT antisera in an enzyme-linked immunosorbent assay (ELISA), and (ii) analysis of the S4 amino acid sequence by a predictive algorithm followed by synthesis and immunization of mice with the predicted peptides coupled to diphtheria toxoid. The anti-peptide conjugate antisera were tested in an ELISA for cross-reactivity with native PT, B oligomer, and S4. Screening of the free peptides in an ELISA by the PT antisera indicated the presence of six B-cell epitope-containing domains covered by residues 18 to 32, 33 to 46, 39 to 52, 51 to 65, 71 to 84, and 91 to 106. None of the peptides, however, were recognized by the monoclonal anti-PT antibodies in an ELISA. Immunization with six computer-predicted peptides (B1 to B6) and three potential T-cell epitopes (T1 to T3) gave rise to very high antibody responses towards the homologous conjugates. With the exception of the anti-T1/diphtheria toxoid antisera, all anti-peptide conjugate antisera cross-reacted with PT in an ELISA at different levels. None of these anti-peptide conjugate antisera, however, showed any PT-neutralizing effect as measured by the Chinese hamster ovary cell assay and the leukocytosis-promoting activity test. The results of the present study suggest that discontinuous epitopes are predominant in the S4 subunit of native PT.

摘要

本研究的主要目的是通过合成肽方法鉴定百日咳毒素(PT)S4亚基上的B细胞表位。采用了两种策略:(i)在酶联免疫吸附测定(ELISA)中,用一组鼠单克隆抗PT抗体和各种多克隆抗PT抗血清筛选覆盖整个S4序列的两个系列重叠肽(12个和25个残基的肽);(ii)通过预测算法分析S4氨基酸序列,然后合成预测肽并将其与白喉类毒素偶联后免疫小鼠。在ELISA中检测抗肽偶联物抗血清与天然PT、B寡聚体和S4的交叉反应性。用PT抗血清在ELISA中筛选游离肽,结果表明存在6个含B细胞表位的结构域,分别由第18至32、33至46、39至52、51至65、71至84和91至106位残基覆盖。然而,在ELISA中没有一种肽能被单克隆抗PT抗体识别。用6种计算机预测肽(B1至B6)和3种潜在T细胞表位(T1至T3)免疫后,对同源偶联物产生了非常高的抗体反应。除抗T1/白喉类毒素抗血清外,所有抗肽偶联物抗血清在ELISA中均与PT发生不同程度的交叉反应。然而,通过中国仓鼠卵巢细胞试验和白细胞增多促进活性试验测定,这些抗肽偶联物抗血清均未显示出任何PT中和作用。本研究结果表明,天然PT的S4亚基中不连续表位占主导地位。

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Annu Rev Immunol. 1984;2:67-101. doi: 10.1146/annurev.iy.02.040184.000435.
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Immune response to the B oligomer of pertussis toxin.对百日咳毒素B寡聚体的免疫反应。
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