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Is an immunoassay available for the measurement of bioactive LH in serum?

作者信息

Rosenfield R L, Helke J

机构信息

Department of Pediatrics, University of Chicago, Pritzker School of Medicine, Wyler Children's Hospital, Illinois 60637-1470.

出版信息

J Androl. 1992 Jan-Feb;13(1):1-10.

PMID:1551801
Abstract

An in vitro bioassay for luteinizing hormone (LH) is in our opinion the "gold standard" bioassay. The rodent interstitial cell testosterone assay (RICT) is specific for bioactive LH and very sensitive, accurate, and reproducible. Diverse LH standards consistently display parallel dose-response characteristics. Sera also manifest parallel dose-response characteristics throughout reproductive life, with the exception of basal samples from prepubertal children. This indicates that all known hormones with LH bioactivity have a similar bioactive site. The in vivo bioassays for LH used for calibration of World Health Organization standards are more cumbersome and less precise and accurate than the in vitro bioassay. The ovarian ascorbic acid depletion assay corresponds better than the seminal vesicle weight assay with in vitro bioassay. Variation in the ratio of bioactive to immunoreactive LH (B/I) principally reflects variation in LH immunoassay dose-response characteristics, rather than a change in the bioactive moiety of LH. The varying B/I ratio is due to molecular heterogeneity at multiple levels. Different LH standards contain different proportions of nonbioactive but immunoreactive material. The immunoreactive LH isoforms in serum contain different proportions of bioactive material and the isoform distribution differs with reproductive status. Furthermore, the antibodies comprising the various immunoassay systems detect heterogeneous epitopes on LH, which are not necessarily bioactive. B/I ratio disparities indicate lack of specificity of immunoassays for bioactive LH. Polyclonal antibody-based radioimmunoassay requires the use of purified reagents, including a bioactive tracer, in order to achieve high specificity for bioactive LH. The new generation of monoclonal antibody-based immunometric assays yields results that are lower than, but correlate with, LH measured by the in vitro bioassay. The purest of standards, even a recombinant standard, yields results that differ up to 50% or more from one immunoassay to another. Serum LH levels also differ up to two-fold among assays. The immunometric assays have the advantage of being more sensitive and more specific for low levels of LH in serum than radioimmunoassays, but B/I ratio discrepancies remain great. An immunoassay specific for the bioactive "docking site" of human LH isoforms is still needed.

摘要

相似文献

1
Is an immunoassay available for the measurement of bioactive LH in serum?
J Androl. 1992 Jan-Feb;13(1):1-10.
2
The changing ratio of bioactive to immunoreactive luteinizing hormone (LH) through puberty principally reflects changing LH radioimmunoassay dose-response characteristics.
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LH levels in women with polycystic ovarian syndrome: have modern assays made them irrelevant?多囊卵巢综合征女性的促黄体生成素水平:现代检测方法是否使其变得不再重要?
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Biologically active luteinizing hormone (LH) in plasma. V. A re-analysis of the differences in the ratio of biological to immunological LH activities during the menstrual cycle.血浆中的生物活性促黄体生成素(LH)。V. 月经周期中生物活性LH与免疫活性LH活性比值差异的重新分析。
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Radioimmunoassay for luteinizing hormone in human plasma or serum: physiological studies.人血浆或血清中促黄体生成素的放射免疫测定:生理学研究
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