ADJUVANT EFFECT OF PERTUSSIS TOXIN ON THE PRODUCTION OF ANTI-OVALBUMIN IGE IN MICE AND LACK OF DIRECT CORRELATION BETWEEN PCA AND ELISA

被引：23

作者：

LINDSAY, DSJ ^{[1
]}

PARTON, R ^{[1
]}

WARDLAW, AC ^{[1
]}

机构：

[1] UNIV GLASGOW,DEPT MICROBIOL,GLASGOW G12 8QQ,LANARK,SCOTLAND

来源：

INTERNATIONAL ARCHIVES OF ALLERGY AND IMMUNOLOGY | 1994年 / 105卷 / 03期

关键词：

IGE ENZYME-LINKED IMMUNOSORBENT ASSAY; OVALBUMIN; PASSIVE CUTANEOUS ANAPHYLAXIS; PERTUSSIS TOXIN;

D O I：

10.1159/000236770

中图分类号：

R392 [医学免疫学];

学科分类号：

100102 ;

摘要：

In studies designed to optimize the production and detection of anti-ovalbumin (anti-Oa) IgE in Ham/ICR mice, a range of doses of both Oa and pertussis toxin as the IgE adjuvant was explored. As determined by 48-hour passive cutaneous anaphylaxis (PCA) tests, the highest titre of anti-Oa IgE was obtained in a three-injection protocol with 0.1 mu g Oa and 1 mu g pertussis toxin for the priming dose, followed by two further doses of 0.1 mu g Oa alone. In single-dose immunizations, the highest PCA responses were obtained in sera from mice given 20 mu g Oa and 1 mu g pertussis toxin. These data confirm that murine IgE production to Oa depends on particular combinations of immunization variables. There was no direct correlation between the PCA and anti-IgE enzyme-linked immunosorbent assay (ELISA) titres of the PCA-positive sera; indeed there was a significant negative correlation. This relationship was not due to interference by IgG1, as there was no correlation between the anti-Oa IgG1 and anti-Oa IgE ELISA titres of the sera. These results highlight the need for caution in assuming that serum IgE levels as measured by ELISA will necessarily correlate positively with IgE biological activity as measured by allergen challenge in vivo.

引用

页码：281 / 288

页数：8

共 26 条

[1] IGE SUPPRESSOR FACTOR INDUCED BY PHYTOHEMAGGLUTININ
ASTORQUIZA, MI
CISTERNAS, C
[J]. INTERNATIONAL ARCHIVES OF ALLERGY AND APPLIED IMMUNOLOGY, 1990, 92 (03): : 223 - 225
[2] NEW AND SIMPLE RADIOIMMUNOASSAY METHOD FOR DETERMINATION OF IGE
CESKA, M
LUNDKVIST, U
[J]. IMMUNOCHEMISTRY, 1972, 9 (10): : 1021 - +
[3] CLAUSEN C, 1970, J IMMUNOL, V1004, P312
[4] CLAUSEN CR, 1969, J IMMUNOL, V103, P768
[5] ENGVALL E, 1972, J IMMUNOL, V109, P129
[6] A COMPARISON OF 5 DIFFERENT METHODS FOR THE DETECTION OF TNP SPECIFIC MOUSE IGE - ELISA, ELISA ON CELLS, ROSETTING, GRANULE ENZYME-RELEASE ASSAY AND PASSIVE CUTANEOUS ANAPHYLAXIS
GAVERIAUX, C
RENARD, P
CAMMISULI, S
LOOR, F
[J]. JOURNAL OF IMMUNOLOGICAL METHODS, 1986, 93 (01) : 107 - 114
[7] STUDIES ON MURINE IGE WITH MONOCLONAL-ANTIBODIES .1. CHARACTERIZATION OF RAT MONOCLONAL ANTI-IGE ANTIBODIES AND THE USE OF THESE ANTIBODIES FOR DETERMINATIONS OF SERUM IGE LEVELS AND FOR ANAPHYLACTIC REACTIONS
HIRANO, T
MIYAJIMA, H
KITAGAWA, H
WATANABE, N
AZUMA, M
TANIGUCHI, O
HASHIMOTO, H
HIROSE, S
YAGITA, H
FURUSAWA, S
OVARY, Z
OKUMURA, K
[J]. INTERNATIONAL ARCHIVES OF ALLERGY AND APPLIED IMMUNOLOGY, 1988, 85 (01): : 47 - 54
[8] COMPARISON OF GUINEA-PIG IGE ANTIBODIES ESTIMATED BY ELISA WITH THOSE ESTIMATED BY PASSIVE CUTANEOUS ANAPHYLAXIS
ITO, K
ISHII, A
YAMASHITA, N
MIYAMOTO, T
WATANABE, N
[J]. INTERNATIONAL ARCHIVES OF ALLERGY AND APPLIED IMMUNOLOGY, 1988, 87 (04): : 424 - 429
[9] JARRETT EEE, 1980, CLIN EXP IMMUNOL, V39, P183
[10] LEHRER SB, 1977, IMMUNOLOGY, V32, P507

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