Anti-Müllerian hormone and progesterone levels in human follicular fluid are predictors of embryonic development

The sample size was determined by firstly estimating the minimum change needed to give a difference in P4/AMH follicular fluid concentration. Using results from a previously published paper [9, 18], it was determined that a 15% difference would be the desired minimum change, with a standard deviation of 20%. This gave a difference to be detected of 1.3 SD units (20/15). Using a confidence interval of 95%, 16 participants per group is necessary to provide a significant result. In order to account for data that is not normally distributed, we inflated the sample by 1.16 (Pitman). 16 × 1.16 = 18.56.

Patients undergoing IVF or ICSI cycles at Merrion Fertility Clinic (Dublin) were recruited and provided written informed consent. Patients suffering from PCOS were excluded from the study.

Patients either received a standard GnRH agonist (Buserelin/ Suprecur/ Deceapeptyl) regime or a standard antagonist regime (Orgalutran). Recombinant FSH (Gonal F/Puregon) or human menopausal gonadotrophin (Menopur) stimulation was initiated once down-regulation was confirmed via transvaginal ultrasound and serum oestradiol measurements or on day 2 or 3 of the cycle for antagonist cycles. Final oocyte maturation was achieved using 5000–10,000 iu human chorionic gonadotrophin or an agonist trigger (Buserlin) when at least three follicles had reached a diameter of ≥17 mm. This was administered 36 h before transvaginal oocyte retrieval.

Oocytes were collected by transvaginal ultrasound-guided needle aspiration of the follicles under conscious sedation. To avoid sample contamination, FF was collected from the first follicle aspirated per patient. To minimise the collection of blood or media-contaminated samples, a midstream aspirate was collected for each patient. The follicle was then flushed, using Origio flushing media. If the oocyte was not present in the first aspirate this continued until an oocyte was retrieved from that follicle, this occurred in only two patients.

As part of a larger study, 88 FF samples were collected. None of the oocytes retrieved were immature – this may be due to the fact that the oocyte we collected was from the first follicle aspirated, and generally the largest follicle. None of the patient cycles selected resulted in total fertilisation failure. Samples were selected for analysis in this study based on the developmental competence of the oocyte i.e. follicular fluid from follicles where the oocyte fertilised and developed into a blastocyst as observed on day 5 (Group 1, BLAST; n = 23) and follicular fluid from follicles where the oocyte fertilised but failed to reach blastocyst stage by day 5 (Group 2, FERT; n = 19), as outlined in Fig. 1. In line with standard oocyte assessment in the ART laboratory, the two populations of oocytes were morphologically indistinguishable from each other prior to insemination and fertilisation.

FF AMH levels were measured using enzyme-linked immunosorbent assay (ELISA) (Immunotech Beckman Coulter, Marseille, France). The measurement range was 0.14–21 ng/ml. Intra- and inter-assay coefficients of variation were 12.3 and 14.2%, respectively, with a sensitivity of 0.14 ng/ml. FF progesterone levels were measured using ELISA (ADI-900-011; EnzoLifeSciences). Follicular fluid was diluted by a factor of 10 ⁶. The measurement range was 15.62–500 pg/ml. Intra- and inter-assay coefficients of variation were 7.6 and 6.8%, respectively, with a sensitivity of 8.57 pg/ml.

The cut off for defining AMH threshold concentration corresponded to the round value of the 50th percentile (> 15 pmol/L). The cut off for defining P4 threshold concentration corresponded to the round value of the 75th percentile (> 60 pmol/L). Sensitivity (if you test many blastocysts, the percentage that will have a positive test), specificity (if you test many embryos that fail to reach blastocyst, the percentage that will have a negative test) and prevalence (our test population contained 54% blastocyst samples) were used to calculate positive predictive values and negative predictive values. For AMH the following calculations were used: prior odds = prevalence/(100-Prevalence) = 1.174; likelihood ratio = sensitivity/(100-specificity) = 2.846; posterior odds = prior odds x likelihood ratio = 3.341; posterior probability = posterior odds/(1 + posterior odds) = 0.7696. For P4 the following calculations were used: prior odds = prevalence/(100-Prevalence) = 1.174; likelihood ratio = sensitivity/(100-specificity) = 6.8; posterior odds = prior odds x likelihood ratio = 7.983; posterior probability = posterior odds/(1 + posterior odds) = 0.8887. For AMH and P4 combined the following calculations were used: prior odds = prevalence/(100-Prevalence) = 1.174; likelihood ratio = sensitivity/(100-specificity) = 26; posterior odds = prior odds x likelihood ratio = 30.522; posterior probability = posterior odds/(1 + posterior odds) = 0.9683.

To determine whether the clinical characteristics of the two groups were possible confounding factors, we compared these parameters, as presented in Table 1, between Group 1 (BLAST, n = 23) and Group 2 (FERT, n = 19). No significant differences were observed between the two groups in terms of maternal age, body mass index, previous live births, previous pregnancy loss, number of antral follicles, number of oocytes recovered, IVF:ICSI ratio or percentage of recovered oocytes that fertilised.

To evaluate the possibility of using key reproductive hormones as potential indicators of an oocytes developmental potential, FF levels of AMH and P4 were quantified and compared between the ‘BLAST’ (n = 23) and ‘FERT’ (n = 19) groups. FF AMH levels were significantly increased (P = 0.007) in the ‘BLAST’ group (33.13 ± 28.83 pmol/L) compared to the ‘FERT’ group (13.6 ± 12.3 pmol/L) (Table 2, Fig. 2). Similarly, FF P4 levels were significantly higher (P = 0.013) in the ‘BLAST’ group (59.76 ± 54.38 mg/ml) compared to the ‘FERT’ group (29.25 ± 22.4 mg/ml) (Table 2, Fig. 3).

Twenty-one FF samples had an AMH level > 15 pmol/L, of which 17 related to oocytes that progressed to blastocyst stage; thus providing a sensitivity rate of 74%, a specificity rate of 74% and a prevalence rate of 54% (Table 3). This provides a positive prediction value (PPV) of 76.96%, leaving a 23.04% chance of a false positive. A negative prediction value (NPV) of 70.8% was obtained (i.e. if the sample fertilised but does not reach blastocyst there is a 70.8% chance of a negative test result), leaving a 29.2% chance of a false negative.

Eleven FF samples had a P4 level > 60 mg/ml, of which 10 related to oocytes that progressed to blastocyst stage; thus providing a sensitivity rate of 43%, a specificity rate of 95% and a prevalence rate of 54% (Table 3). This provides a PPV of 90.99%, leaving a 9.01% chance of a false positive. A NPV of 58.67% was obtained, leaving a 41.33% chance of a false negative.

Six samples had an AMH level > 15 pmol/L and a P4 level > 60 mg/ml, of which 100% progressed to blastocyst stage; thus providing a sensitivity rate of 26%, a specificity rate of 99.99% and a prevalence rate of 54% (Table 3). This provides a PPV of 96.83%, leaving a 3.17% chance of a false positive. A NPV of 53.26% was obtained, leaving a 46.74% chance of a false negative.