Development, validation and application of an ultra-sensitive two-site enzyme immunoassay for human follistatin

Recent studies have found follistatin to be an important regulator of activin bioactivity. Whilst a number of assay formats have been described, all are of limited sensitivity and require the use of isotopes. Many use polyclonal antibodies. Furthermore, a wide range of follistatin preparations have been used as standards, complicating inter-laboratory comparison. We now describe an ultra-sensitive two-site enzyme immunoassay using a pair of mouse monoclonal antibodies raised against follistatin 288. The presence of sodium deoxycholate and Tween 20 in the diluent gave results for total (free and activin-dissociated) follistatin. The assay had a detection limit of <19 pg/ml and recovery of spiked follistatin 288 from amniotic fluid, serum seminal plasma, human follicular fluid and granulosa cell conditioned medium averaged 100.7 +/- 7.5%, 89.1 +/- 5.5%, 98 +/- 4.9%, 96 +/- 7.2% and 123.9 +/- 11% respectively. The intra- and interplate coefficients of variation were < 5%. An excess of activin-A (50 ng/ml) prior to assay did not affect follistatin recovery. Inhibin-A, inhibin-B, activin-A, activin-B and activin-AB had minimal cross-reactivity (<0.3%). However, follistatin 315 had a significant cross-reaction (9.9%). Serially diluted human samples gave dose-response curves parallel to the standard. Pooled human follicular fluid contained high concentrations of follistatin (approximately 242 ng/ml). Follistatin was also found in maternal serum during pregnancy (first trimester approximately 0.8 ng/ml, third trimester approximately 2.8 ng/ml), normal male serum (approximately 0.45 ng/ml), amniotic fluid (sixteen week approximately 3.63 ng/ml, term approximately 0.89 ng/ml), seminal plasma (2.4-30 ng/ml) and human granulosa cell conditioned media (approximately 0.44 ng/ml). Serial serum samples taken throughout the menstrual cycle of ten women showed fluctuating follistatin concentrations (approximately 0.62 ng/ml) with no apparent relationship to the stage of the cycle. Interestingly, pooled serum from postmenopausal women appeared to have higher follistatin levels than any of the normal women (approximately 1.4 ng/ml). The possible presence in certain samples of mixtures of follistatin isoforms with different immunoreactivities poses major problems of interpretation in this and all other current follistatin immunoassays. Further work is needed to identify the major immunoreactive forms in different tissues and fluids. Nevertheless, the new assay has a number of advantages over previous assays and should prove a useful tool for various clinical and physiological studies.

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EP859 Endocrine-disrupting chemicals present in human follicular fluid disrupt granulosa cell tumors E2 secretion dependent on estrogen metabolism potential

10.1136/ijgc-2019-esgo.908 ◽

2019 ◽

Author(s):

J Gogola ◽

M Hoffmann ◽

S Nimpsz ◽

A Ptak

Keyword(s):

Granulosa Cell ◽

Follicular Fluid ◽

Endocrine Disrupting Chemicals ◽

Estrogen Metabolism ◽

Human Follicular Fluid ◽

Granulosa Cell Tumors ◽

Endocrine Disrupting

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A Mixture Reflecting Polybrominated Diphenyl Ether (PBDE) Profiles Detected in Human Follicular Fluid Significantly Affects Steroidogenesis and Induces Oxidative Stress in a Female Human Granulosa Cell Line

Endocrinology ◽

10.1210/en.2016-1106 ◽

2016 ◽

Vol 157 (7) ◽

pp. 2698-2711 ◽

Cited By ~ 11

Author(s):

Pavine L. C. Lefevre ◽

Mike Wade ◽

Cindy Goodyer ◽

Barbara F. Hales ◽

Bernard Robaire

Keyword(s):

Oxidative Stress ◽

Cell Line ◽

Granulosa Cell ◽

Follicular Fluid ◽

Chronic Exposure ◽

Flame Retardants ◽

Culture Medium ◽

Oxygen Species ◽

Human Follicular Fluid ◽

Human Granulosa Cell

Brominated flame retardants are incorporated into consumer products to prevent flame propagation. These compounds leach into the domestic environment, resulting in chronic exposure. Pregnancy failure is associated with high levels of polybrominated diphenyl ethers (PBDEs), a major class of brominated flame retardants, in human follicular fluid, raising serious questions regarding their impact on female fertility. Our goal was to elucidate the effects of a mixture of PBDEs, similar to the profile found in human follicular fluid, on an immortalized human granulosa cell line, the KGN cell line. We showed that cell viability was altered and oxidative stress was induced as reflected by increased reactive oxygen species formation at 100 μM of the PBDE mixture. Transcriptomic analysis revealed that PBDE treatments of 1, 5, and 20 μM altered the expression of several genes involved in the reactive oxygen species signaling pathway. Significant dose-dependent reductions in progesterone and estradiol levels in the culture medium were measured after PBDE treatment; in parallel, the expression of genes involved in estradiol metabolism, namely CYP1A1, was up-regulated by 5 and 20 μM of the PBDE mixture. Treatment with 20 μM PBDE also increased the expression and secretion of the proinflammatory factor, IL-6, into the KGN cell culture medium. Our results demonstrate that PBDEs can alter human granulosa cell functions by inducing oxidative stress and disrupting steroidogenesis. These results indicate that PBDEs may be detrimental to ovarian functions and thus may adversely affect female reproductive health after chronic exposure.

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Levels of Environmental Contaminants in Human Follicular Fluid, Serum, and Seminal Plasma of Couples Undergoing In Vitro Fertilization

Archives of Environmental Contamination and Toxicology ◽

10.1007/s00244-001-0048-8 ◽

2002 ◽

Vol 43 (1) ◽

pp. 121-126 ◽

Cited By ~ 157

Author(s):

E. V. Younglai ◽

W. G. Foster ◽

E. G. Hughes ◽

K. Trim ◽

J. F. Jarrell

Keyword(s):

In Vitro Fertilization ◽

Seminal Plasma ◽

Follicular Fluid ◽

Environmental Contaminants ◽

Human Follicular Fluid ◽

Vitro Fertilization

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Co-incubation of spermatozoa with human follicular fluid reduces sperm DNA fragmentation by mitigating DNase activity in the seminal plasma

Journal of Assisted Reproduction and Genetics ◽

10.1007/s10815-019-01643-2 ◽

2019 ◽

Vol 37 (1) ◽

pp. 63-69

Author(s):

Monica Dorado-Silva ◽

Javier Bartolomé-Nebreda ◽

Pascual Sánchez-Martín ◽

Stephen Johnston ◽

Jaime Gosálvez

Keyword(s):

Dna Fragmentation ◽

Seminal Plasma ◽

Follicular Fluid ◽

Dnase Activity ◽

Sperm Dna Fragmentation ◽

Human Follicular Fluid ◽

Sperm Dna

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Dimeric inhibins and activin A in human follicular fluid and oocyte–cumulus culture medium

Human Reproduction ◽

10.1093/humrep/14.10.2525 ◽

1999 ◽

Vol 14 (10) ◽

pp. 2525-2530 ◽

Cited By ~ 28

Author(s):

C.P. Lau ◽

W.L. Ledger ◽

N.P. Groome ◽

D.H. Barlow ◽

S. Muttukrishna

Keyword(s):

Follicular Fluid ◽

Culture Medium ◽

Activin A ◽

Human Follicular Fluid

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Human follicular fluid stimulation of granulosa cell steroid secretion

Acta Endocrinologica ◽

10.1530/acta.0.114s147 ◽

1987 ◽

Vol 116 (3_Suppl) ◽

pp. S147

Author(s):

J. DITTMANN ◽

S. CHARI ◽

U. DEICHERT ◽

G. STURM ◽

E. DAUME

Keyword(s):

Granulosa Cell ◽

Follicular Fluid ◽

Human Follicular Fluid ◽

Steroid Secretion ◽

Stimulation Of

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Development and application of a two-site enzyme immunoassay for the determination of 'total' activin-A concentrations in serum and follicular fluid

Journal of Endocrinology ◽

10.1677/joe.0.1480267 ◽

1996 ◽

Vol 148 (2) ◽

pp. 267-279 ◽

Cited By ~ 178

Author(s):

P G Knight ◽

S Muttukrishna ◽

N P Groome

Keyword(s):

Human Serum ◽

Enzyme Immunoassay ◽

Follicular Fluid ◽

Biological Fluids ◽

Activin A ◽

Β Subunit ◽

Serum Samples ◽

Response Curves ◽

Inhibin A ◽

Α Subunit

Abstract The performance of existing immunoassays and bioassays for activins is compromised by the presence of activin-binding proteins such as follistatin and α2 macroglobulin (α2M) in biological fluids. To overcome this problem we have developed a novel two-site enzyme immunoassay procedure for activin-A which incorporates an analyte denaturation and oxidation step. The optimized assay is sensitive (detection limit ∼10 pg/well), precise (mean within- and between-plate coefficients of variation 4·9 and 9·1% respectively) and accurate (activin-A recovery values of 102 ± 3 and 96 ± 5% for bovine follicular fluid (FF) and human serum respectively). In specificity tests, high concentrations of follistatin (500 ng/ml) and α2M (100 μg/ml) did not interfere with the response signal to activin-A. In addition, no significant cross-reactivity was observed with a range of related molecules including inhibin-A, inhibin-B, activin-B (all <0·5%), bovine pro-αC and follistatin (both <0·1%). Response curves parallel to the activin-A standard curve were obtained for a variety of test samples including bovine, human, ovine and porcine FF, human sera and conditioned medium from cultured bovine and human granulosa cells. Fractionation of bovine FF by SDS-PAGE confirmed assay specificity since only one peak of activin-A immunoreactivity was detected (Mr ∼25 k) in eluted gel slices. However, gel-permeation chromatography showed that under physiological conditions all of the detectable activin-A in bovine FF eluted with apparent Mr values of >700 and 60–200 k reflecting its association with binding protein(s). Analysis of bovine FF samples (n=76) from morphologically dominant follicles during the luteal phase showed that activin-A levels were positively correlated with inhibin-A (r=+0·54; P<0·001) and total β subunit immunoreactivity (r=+0·32; P<0·005) but not with total α subunit immunoreactivity (r= −0·09). Classification of these follicles according to oestrogenic status showed that activin-A, inhibin-A and total β subunit levels were highest in oestrogen-inactive follicles (P<0·01) whereas total α subunit levels were lowest in these follicles (P<0·001). Activin-A levels were measurable in all human serum samples analysed, ranging from 128 pg/ml during the normal menstrual cycle, 210 pg/ml in women undergoing ovarian hyperstimulation and ∼ 500 pg/ml in postmenopausal women to over 4000 pg/ml during pregnancy. In conclusion, the present assay provides a reliable method for quantitating total (i.e. bound+free) activin-A concentrations in a variety of biological samples and should prove useful for further in vivo and in vitro studies in a range of species including man. Journal of Endocrinology (1996) 148, 267–279

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