SUBFEMTOMOLE ENZYME-IMMUNOASSAY FOR HUMAN GROWTH-HORMONE USING AFFINITY-CHROMATOGRAPHY AND ENZYME AMPLIFIED DETECTION

被引:7
作者
LEJEUNE, R
THUNUS, L
GOMEZ, F
FRANKENNE, F
CLOUX, JL
HENNEN, G
机构
[1] BIOCODE,B-4000 LIEGE,BELGIUM
[2] UNIV LIEGE,CTR HOSP B23,SERV ENDOCRINOL EXPTL & CLIN,B-4000 LIEGE,BELGIUM
关键词
D O I
10.1016/0003-2697(90)90111-L
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
An immunometric assay is described which allows fast detection of attomole amounts of an antigen. The sensitivity is 100 to 1000 times better than that of classical sandwich immunometric assays. Our system allowed the measurement of human growth hormone in the range of 0.1 amol to 100 fmol in a 4-h time period overall. A chromatography column is sequentially filled with two immunoaffinity resins: SPM1E1Ab1 in the upper half and SPM2E2Ab2 in the lower half, where Ab1 and Ab2 represent complementary antibodies reacting with the antigen to be assayed, E1 and E2 represent enzymes, M1 and M2 represent substances reacting reversibly with E1 and E2, respectively, and SP represents the chromatographic solid phase; the sign - represents covalent linkages and the sign - reversible linkages. The sample solution is passed through the column, resulting in binding of the antigen to the first encountered antibody, yielding the immobilized complex SPM1E1Ab1Ag. The M1 bound is then destabilized by washing with solution of agonist to M1. The freed complex is immediately trapped by the second antibody in the lower part of the column, resulting in the entity SPM2E2Ab2AgAb1E1. After a washing step, an amplified detection allows the measurement of the antigen through the activity of the enzyme E1. The antigen-antibody reactions occur in the presence of a very large excess of antibody. The continuous equilibrium displacement due to the chromatographic procedure enhances the yield of complex formation. These factors explain the extremely low levels (subattomole) capable of being detected with this original technique. © 1990.
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页码:217 / 222
页数:6
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