Bioidentical compounded hormones: A pharmacokinetic evaluation in a randomized clinical trial

Maturitas 74 (2013) 375–382

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Bioidentical compounded hormones: A pharmacokinetic evaluation in a randomized clinical trial夽 Richa Sood a,∗ , Roger A. Warndahl b , Darrell R. Schroeder c , Ravinder J. Singh d , Deborah J. Rhodes e , Dietlind Wahner-Roedler f , Rebecca S. Bahn g , Lynne T. Shuster a a

Women’s Health Clinic, Division of General Internal Medicine, Mayo Clinic, 200 First Street SW, Rochester, Minnesota 55905, USA Division of Pharmacy, Mayo Clinic, 200 First Street SW, Rochester, Minnesota 55905, USA c Health Sciences Research, Division of Biomedical Statistics and Informatics, Mayo Clinic, 200 First Street SW, Rochester, Minnesota 55905, USA d Department of Laboratory Medicine and Pathology, Mayo Clinic, 200 First Street SW, Rochester, Minnesota 55905, USA e Executive Health, Division of Preventive and Occupational Medicine, Mayo Clinic, 200 First Street SW, Rochester, Minnesota 55905, USA f Breast Clinic, Division of General Internal Medicine, Mayo Clinic, 200 First Street SW, Rochester, Minnesota 55905, USA g Division of Endocrinology and Metabolism; Mayo Clinic, 200 First Street SW, Rochester, Minnesota 55905, USA b

a r t i c l e

i n f o

Article history: Received 10 December 2012 Received in revised form 11 January 2013 Accepted 12 January 2013

Keywords: Bioidentical Compounded Hormone therapy Pharmacokinetics

a b s t r a c t Objective: Bioidentical compounded hormone therapy is popular among patients, but providers do not have pharmacokinetic information or dosing guidelines for these preparations. Our objective was to compare the pharmacokinetics of the commonly used compounded preparations with conventional hormonal preparations that are considered bioequivalent in practice. Methods: We conducted a randomized, blinded, four-arm 16-day clinical trial of forty postmenopausal women assigned to one of three doses of a compounded estrogen cream (Bi-est (80:20); 2.0, 2.5, or 3.0 mg) + compounded oral progesterone 100 mg, or to a conventional estradiol patch (Vivelle-DotTM 0.05 mg) + PrometriumTM 100 mg. Serum levels of estrone, estradiol, estriol, and progesterone were obtained at multiple time intervals during the first 24-h, and at steady-state. Results: Results were analyzable for 37/40 women. Study medications were well tolerated. The AUC at 24 h and at steady-state for estrogens remained consistently lower for all doses of Bi-est tested relative to the patch. The difference was statistically significant for Bi-est 2.0 mg (AUC-estradiol = 181 vs. 956; p < 0.001) and 2.5 mg (AUC-estradiol = 286 vs. 917; p < 0.001). Estriol levels remained low in all study arms. Serum progesterone levels were comparable in conventional vs. compounded groups. Conclusions: This pharmacokinetic trial showed that the currently used doses of compounded hormones yield lower levels of estrogen compared to the standard-dose estradiol patch. To find comparable doses, further studies are needed. This successfully conducted randomized controlled study attests to the feasibility of using a similar design in the setting of a larger clinical trial. © 2013 Elsevier Ireland Ltd. All rights reserved.

1. Introduction With an aging population globally, the world’s total menopausal population, estimated at 476 million in 1990, is expected to rise to 1.2 billion by 2030 [1]. In the United States, approximately 75%–80% of postmenopausal women report vasomotor symptoms [2]. A large

Abbreviations: CRU, Clinical Research Unit; CVs, coefficient of variations. 夽 Trial registration: linicaltrials.gov identifier: NCT00864214. ∗ Corresponding author at: Women’s Health Clinic, Mayo Clinic, 200 First Street SW, Rochester, Minnesota 55905, USA. Tel.: +1 507 538 7103; fax: +1 507 266 3988. E-mail addresses: [email protected] (R. Sood), [email protected] (R.A. Warndahl), [email protected] (D.R. Schroeder), [email protected] (R.J. Singh), [email protected] (D.J. Rhodes), [email protected] (D. Wahner-Roedler), [email protected] (R.S. Bahn), [email protected] (L.T. Shuster). 0378-5122/$ – see front matter © 2013 Elsevier Ireland Ltd. All rights reserved. http://dx.doi.org/10.1016/j.maturitas.2013.01.010

proportion of these women also experience vaginal dryness [3], urinary incontinence [3], decline in sexual interest and satisfaction [4], mood fluctuations [5,6], sleep disturbances [7–9], and changes in memory and cognition, for which hormone therapy is often sought. The collective impact of these symptoms on women’s well-being is enormous, and the need for safe treatments is compelling [10]. Conventional hormone therapy consisting of Food and Drug Administration (FDA)-approved products is the standard of care in the United States when treatment is indicated for menopausal symptom relief. However, randomized trials such as the Heart and Estrogen/Progestin Replacement Study [11] and Women’s Health Initiative [12] raised concerns about the safety of conventional hormones like PremarinTM and ProveraTM , leading to a marked reduction in their use and creating a demand for safer alternatives. Bioidentical hormones have gained popularity as possible alternatives to conventional hormones. The term “bioidentical”

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Table 1 Study design. No. of patients/arm

Randomization Active intervention

Placebo

Estrogen

Progesterone

10

Bi-est 2.0 mg

Patch

10

Bi-est 2.5 mg

Compounded progesterone 100 mg Compounded progesterone 100 mg

10

Bi-est 3.0 mg

Patch

10

Estradiol 0.05 mg patch (Vivelle-DotTM )

Compounded progesterone 100 mg Micronized progesterone 100 mg capsule (PrometriumTM )

implies a chemical and molecular structure precisely the same as its endogenous human hormone counterpart. Structural similarity by some is believed to correlate with safety, a perception that has led to a sharp increase in the popularity of bioidentical hormones. Currently there are multiple FDA-approved conventional hormone products that are plant-derived and bioidentical in chemical structure [13]. However, likely due to extensive media coverage, requests from women for bioidentical hormones are predominantly for the compounded preparations. In the absence of adequate research, no clear guidelines exist for choosing the most appropriate type, dose, or regimen of bioidentical compounded hormones. Lacking this data, it is challenging to study these preparations for safety and efficacy. To the best of our knowledge, no pharmacokinetic studies have compared conventional with compounded bioidentical hormones. Compounding pharmacists generally consider Bi-est (referring to estriol plus estradiol) in a dose of 2.5 mg (for example, in a ratio of 80% estriol plus 20% estradiol, which consists of 2 mg estriol and 0.5 mg estradiol) as approximately equivalent to a mid-range dose of an estradiol-containing patch such as Vivelle-DotTM 0.05 mg. Thus, using Bi-est with 80% estriol and 20% estradiol, and comparing the calculated estradiol equivalence of the compounded preparations with the daily referenced estradiol dose of the patch, we assigned the three strengths of creams to create a reasonable range for comparison. In order to lay the groundwork for future trials, we conducted a pharmacokinetic study as a randomized, blinded clinical trial. Our intent was to compare estrogen and progesterone levels obtained following the administration of bioidentical compounded hormone therapy preparations both with themselves and with conventional hormone therapy. 2. Methods 2.1. Subjects The study was approved by the Mayo Clinic Institutional Review Board. Since estriol is not an approved product in the United States, an IND (investigational new drug) application was filed with the US-FDA. This was a Phase I, blinded, randomized, four-arm study. Subjects were recruited from Rochester, MN, and surrounding areas through advertisements and news media releases. Eligibility was based on the following criteria:women 40–60 years old, naturally postmenopausal (absence of periods for ≥1 year or amenorrhea for ≥6 months and FSH ≥40 IU/L) or surgically postmenopausal (menopause induced by removal of ovaries), able to understand and sign an informed consent, and willing to stay overnight in a Clinical Research Unit (CRU). Eligible women had normal results on screening tests (AST, creatinine, and TSH within 20% of the upper

Patch

Intervention phase (16 days) Day 1

Days 15 and 16

Serial measurements E1, E2, E3 Baseline and 24 h progesterone level

Serial measurements E1, E2, E3; Single end-of-treatment progesterone level Monitoring for adverse effects

Monitoring for adverse effects

Cream

limit of normal) and a negative mammogram within the last 11 months. Presence or absence of menopausal symptoms was not used as an eligibility criterion. Subjects were excluded using the following criteria: estrogen levels >35 pg/mL; >10 years from last menstrual period; a history of cancer of the breast, uterus or ovary, coronary artery disease, stroke, dementia, migraine, deep venous thromboembolism, active liver or gall bladder disease, uncontrolled hypertension, diabetes, or lupus; currently smoking; alcohol or substance abuse; family history of premenopausal breast or ovarian cancer; or postmenopausal breast cancer in ≥2 relatives. Recent use of hormone therapy was allowed with an adequate washout period (at least 1 week for vaginal hormones, 4 weeks for transdermal hormones, and 8 weeks for oral hormones). Additional exclusions included peanut allergy, current use of isoflavone-containing products, and drugs or herbs that might affect metabolizing enzymes. 2.2. Study treatment Eligible women were randomized to one of four treatment arms in a double-blinded fashion. Three study arms included compounded estradiol–estriol cream (Bi-est) in varying dosage, along with a placebo skin patch, and compounded oral micronized progesterone capsules. The fourth arm included an estradiol-containing patch (Vivelle-DotTM ), placebo cream, and commercially available oral micronized progesterone capsules (Prometrium) (Table 1). Bi-est (80:20) 2.5 mg was chosen as it is considered equivalent to 0.05 mg estradiol patches in compounding practice. Bi-est was compounded in Vanicream and dispensed in premarked individual syringes by an experienced compounding pharmacist (RAW), who was blinded to the participants’ study group assignment. Women in study arm one received Bi-est 2.0 mg (1.6 mg estriol and 0.4 mg estradiol), in arm two Bi-est 2.5 mg (2 mg estriol and 0.5 mg estradiol), and arm three Bi-est 3.0 mg (2.4 mg estriol and 0.6 mg estradiol). Women in study arm four received Vivelle-Dot 0.05 mg patches. On day one of the study, participants were admitted to the hospital in the CRU, where they were instructed to apply their first dose under supervision by trained nurses. The creams were applied to a specified area of the forearm by gentle rubbing for 1 min. The Vivelle-DotTM patch was applied to the skin of the lower abdomen following the manufacturer’s directions. The capsules were administered orally under supervision. Throughout the next 24 h, serial blood samples were obtained at specified intervals to measure the serum levels of estrogen fractions and progesterone (Table 2). After 24 h of the CRU stay, participants were discharged and continued taking study medications as instructed. They returned on the 15th day of the study and were admitted for 12 h during which time serial blood samples were obtained to measure the steady-state

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377

Table 2 Study intervention schedule.

Hours E1, E2, E3 Progesterone Study Coordinator Phone call

Intervention phase Venipuncture Day 1 (hours after initial application of cream/patch) −1 2 5 8 12 18

24

x x

x x

x

x

x

x

x

Days 7 and 13

levels of estrogen and progesterone. Participants returned on day 16 for the last set of blood draws. They returned any remaining supply of medications. Compliance was assessed by counting syringes, patches, and capsules that were returned, as well as by self report. 2.3. Hormone measurements Estrogen fractions (Estrone E1, E2) were measured by liquid chromatography–tandem mass spectrometry (ThermoFisher Scientific, Franklin, MA and Applied Biosystems-MDS Sciex, Foster City, CA). For E1, the intra-assay coefficient of variations (CVs) were 10.9%, 3.4%, 5.1%, and 3.5% at 6.7, 29, 109, and 332 pg/mL respectively, and the inter-assay CVs were 8.1%, 6.9%, 5.2%, 6.3%, and 6.7% at 6.4, 26, 58, 120, and 336 pg/mL respectively. For E2, the intraassay CVs were 12.4%, 3.1%, 5.0%, and 3.5% at 7.2, 29, 109, and 325 pg/mL respectively, and the inter-assay CVs were 9.2%, 8.6%, 9.0%, 6.6%, and 4.8% at 7.0, 24, 61, 125, and 360 pg/mL respectively. The limit of quantitation for both E1 and E2 was 2.5 pg/mL. Values less than 2.5 pg/mL were reported as <2.5 pg/mL. Estriol (E3) was measured by using the Access® Unconjugated Estriol assay, which was a competitive binding immunoenzymatic assay measured on the DxI automated immunoassay system (Beckman Instruments, Chaska, MN). The inter-assay CVs were 6.4%, 4.6%, and 4.9% at 1.04, 2.78, and 5.65 ng/mL respectively, and the lowest reportable result was 0.07 ng/mL. Progesterone was measured by a competitive binding immunoenzymatic assay on the DxI 800 automated immunoassay system (Beckman Instruments, Chaska, MN). The inter-assay CVs were 16.5%, 10.1%, and 7.7% at 0.76, 9.2, and 29.6 ng/mL respectively. The lower limit of the clinically reportable range for progesterone was 0.08 ng/mL. 2.4. Statistical analysis The concentration of each estrogen fraction at the start of the study period (C0 ) and at 24 h after treatment application (C24 ) was measured, as was the difference between the baseline and 24-h concentrations (C24 − C0 ). We also calculated the average concentration and area under the curve (AUC) for each of the three estrogen fractions over the first 24 h. Due to the marked variability observed in the individual concentration–time profile plots, maximum concentration (Cmax ) and time to maximum concentration (Tmax ) were not analyzable. The results from each of the three cream groups were compared with the Vivelle-Dot patch group. Progesterone levels were measured at baseline, 24 h, and at the end of study. We calculated the difference between the mean concentration at 24 h and at the end of the study compared to baseline. The combined results from the compounded micronized progesterone groups were compared against the conventional Prometrium group. Subject characteristics were summarized using mean ± standard deviation, median (min, max) for continuous variables, and frequency counts for categorical variables. E1, E2, and E3 parameters described previously were summarized separately for each of the 4 treatment groups. The rank sum test

Venipuncture Days 15 and16 (hours after final application of cream/patch) −1 2 5 8 12 24 30 x

x

x

x

x x

x

x

x

was used to compare each of the Bi-est groups to the VivelleDot patch group. As a secondary analysis, progesterone levels were summarized and compared between the Bi-est arms and Vivelle-Dot group using the rank sum test. In all cases, two-tailed p-values ≤ 0.05 were considered statistically significant. The frequency of adverse events was summarized according to treatment group and compared across groups using the Fisher exact test. 3. Results 3.1. Participants Fifty-two postmenopausal women were screened; 12 of those were excluded and all 40 women who were randomized into the trial completed the study (Fig. 1). The average age of the study participants was 54 years; their average BMI was 29 kg/m2 (Table 3). The compliance rate for use of Bi-est creams and Vivelle-Dot patch was 100%. Only one participant returned a single unused progesterone capsule. Two participants whose initial screening estradiol levels were in the postmenopausal range had elevated baseline estradiol levels on repeat testing before administration of the study medications (82 pg/mL and 151 pg/mL respectively) and were excluded. A third participant with non-physiologic estradiol levels (1500 pg/mL), presumably from contamination with estrogen cream at the venipuncture site, was excluded after the study medications were administered. Data were analyzable for 37/40 women. 3.2. Estrogen pharmacokinetics Average concentrations and AUC were calculated for estrogen fractions after initial dosing and at steady-state (Tables 4 and 5). The Bi-est cream groups showed a slight trend toward increasing serum levels of estrogen with an increasing dose of estrogen. However, participants had wide fluctuations in their estradiol level with Biest, both after the initial administration as well as at steady-state (Figs. 2 and 3). In contrast, the estrogen absorption with VivelleDot patches was more consistent across the ten participants given the patch, and the pattern was similar to what is reported in the literature (Fig. 2). 3.2.1. Estradiol In the Bi-est groups, for the majority of subjects a peak estradiol level was absent after a single-dose administration (Fig. 2). The 24-h E2-AUC was smaller in all Bi-est groups compared to the estradiol patch group, with the difference being statistically significant for Bi-est 2.0 and 2.5 mg. The steady-state E2-AUC (Days 15, 16) was also smaller for all Bi-est groups compared to the patch, with the difference being statistically significant for the Bi-est 2.0 and 2.5 mg groups (Table 4). 3.2.2. Estrone Estrone (E1) levels in the Bi-est groups remained lower than for the patch, both after initial administration of the medication, as well as at steady-state (Fig. 4). The 24-h E1-AUC and

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Assessed for eligibility n = 52 Excluded (n = 12) Not meeting inclusion criteria (n = 11) Declined to participate (n = 1) Other reasons (n = 0)

Enrollment

Randomized (n = 40)

Allocation

Follow-up

Bi-est 2.0 mg (Arm 1; n = 10)

Bi-est 2.5 mg (Arm 2; n = 10)

Bi-est 3.0 mg (Arm 3; n = 10)

Vivelle-Dot 0.05 mg patch (Arm 4; n = 10)

Discontinued intervention (n =0)

Discontinued intervention (n=3) (2 participants excluded before study drug administration due to elevated repeat baseline estradiol; 1 participant excluded after starting the study medication due to supra-physiologic estrogen levels possibly secondary to contamination)

Discontinued intervention (n =0)

Discontinued intervention (n =0)

Analyzed (n = 10)

Analyzed (n = 7)

Analyzed (n = 10)

Analyzed (n = 10)

Analysis

Fig. 1. Flow diagram.

steady-state E1-AUC were smaller across all Bi-est groups compared to the patch, and the difference was statistically significant for the Bi-est 2.0 and 2.5 mg arms (Table 5). 3.2.3. Estriol Most participants had E3 levels below the lower limit of detection of the assay, both at baseline and at steady-state. All E3 assays were run in triplicate to evaluate the reliability of these results. Acknowledging the limitation of a wide coefficient of correlation

due to very low serum values, average E3 values were comparable at baseline. The 24-h median AUC for the Bi-est 2.0 mg arm and the steady-state median AUC for the Bi-est 2.0 and 2.5 mg arms were significantly lower than the patch (p < 0.05) (Fig. 5). 3.3. Progesterone pharmacokinetics Progesterone levels were analyzed in the 37/40 women whose estrogen levels were confirmed to be menopausal. The levels at

Table 3 Baseline characteristics of study participants. Bi-est 2.0 mg (n = 10)

Bi-est 2.5 mg (n = 7)

Bi-est 3.0 mg (n = 10)

Vivelle-Dot 0.05 mg (n = 10)

Age, years Mean ± SD Median (min, max)

53.7 ± 4.3 54 (44, 59)

55.1 ± 3.6 55 (50, 59)

52.9 ± (3.8) 53 (48, 59)

53.8 ± 2.7 54 (48, 57)

BMI, kg/m2 Mean ± SD Median (min, max)

29.9 ± 5.1 30 (23, 38)

28.8 ± 9.3 27 (18, 42)

29.3 ± 6.5 28 (21, 44)

28.1 ± 5.8 28 (20, 38)

Prior conventional hormone therapy use 6 No 4 Yes

3 4

2 8

2 8

Prior compounded hormone therapy use No 10 0 Yes

7 0

10 0

9 1

Characteristic

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Table 4 Estradiol pharmacokinetics at baseline, 24 h and steady-state in a phase I randomized clinical trial for evaluating estrogen pharmacokinetics. Characteristic

Bi-est 2.0 mg (n = 10)

BASELINE – single dose (all results measured in pg/mL) C0 Mean ± SD 5.7 ± 1.1 5.0 (4.9, 7.7) Median (min, max) C24 Mean ± SD 8.7 ± 3.8a Median (min, max) 8.2 (4.9, 17.0) C24 − C0 Mean ± SD 3.0 ± 3.3a Median (min, max) 1.6 (0.0, 9.4) Average 7.7 ± 2.6a Mean ± SD Median (min, max) 7.0 (5.1, 13.1) AUCd Mean ± SD 193 ± 76a Median (min, max) 181 (124, 381) End of study – steady-state (all results measured in pg/mL) C0 Mean ± SD 9.5 ± 3.2a 9.4 (5.5, 16.0) Median (min, max) C24 Mean ± SD 12.3 ± 8.9a 9.8 (4.9, 36.0) Median (min, max) C24 − C0 Mean ± SD 2.8 ± 8.7c 0.0 (−5.5, 26.0) Median (min, max) Average 11.8 ± 4.9a Mean ± SD Median (min, max) 10.8 (6.3, 24.3) AUCd Mean ± SD 286 ± 118a 269 (149, 592) Median (min, max)

Bi-est 2.5 mg (n = 7)

Bi-est 3.0 mg (n = 10)

Vivelle-Dot 0.05 mg (n = 10)

6.5 ± 2.3 5.2 (4.9, 11.0)

10.0 ± 9.2 5.1 (4.9, 34.0)

8.5 ± 5.8 6.0 (4.9, 23.0)

9.0 ± 3.1a 10.0 (4.9, 12.0)

51.0 ± 90.7b 26.0 (4.9, 306.0)

57.5 ± 28.5 54.5 (19.0, 110.0)

2.5 ± 2.9a 1.0 (0.0, 6.8)

50.0 ± 91.9c 13.6 (0.0, 301.1)

49.0 ± 25.9 44.4 (14.1, 89.1)

7.3 ± 2.5a 6.5 (4.9, 11.9)

26.5 ± 27.7 16.0 (5.1, 96.4)

35.8 ± 19.4 33.2 (10.8, 71.4)

177 ± 62a 153 (118, 293)

730 ± 840 405 (122, 2919)

1043 ± 562 956 (306, 2012)

25.2 ± 34.9b 11.0 (4.9, 103.0)

20.9 ± 14.1b 19.0 (5.4, 52.0)

31.7 ± 21.5 26.0 (13.0, 91.0)

12.7 ± 7.9a 11.0 (6.9, 29.0)

22.2 ± 19.0c 14.5 (5.5, 70.0)

62.7 ± 39.9 51.5 (18.0, 129.0)

−12.6 ± 36.6c −0.6 (−92.0, 19.7)

1.4 ± 11.9c 0 (−26.0, 18.0)

31.0 ± 30.4 26.0 (2.0, 98.0)

17.5 ± 10.7b 12.4 (5.8, 33.8)

32.2 ± 32.4 21.7 (10.4, 117.3)

44.8 ± 26.8 33.0 (12.1, 95.2)

374 ± 199c 337 (143, 641)

728 ± 643 540 (262, 2340)

1247 ± 760 917 (321, 2550)

a

Rank sum test p < 0.001 compared to Vivelle-Dot 0.05 mg. Rank sum test p < 0.05 compared to Vivelle-Dot 0.05 mg. c Rank sum test p < 0.01 compared to Vivelle-Dot 0.05 mg. d At baseline (after a single dose) estrogen fractions were measured at 0, 2, 5, 8, 12, 18, and 24 h. At the end of study (steady-state) estrogen fractions were measured at 0, 2, 5, 8, 12 and 24 h. The area under the curve (AUC) was calculated according to the trapezoidal rule. b

baseline were comparable in all 4 groups. The levels increased comparably at 24 h and at steady-state with administration of both the compounded and conventional bioidentical progesterone preparations; no intergroup differences were noted (Table 6).

coefficient of correlation between BMI and E3 was noted to be −0.33 at steady-state, and the p value was not statistically significant (Fig. 6). 3.5. Safety

3.4. Effect of BMI on estrogen There was wide variability in the BMI of the study participants. Since the enzymes in body fat are involved in estrogen metabolism, we plotted E3 levels against BMI. We used the VivelleDot patch group, as this group had no exogenous E3 administered and thus any rise in E3 was assumed to be from interconversion. The

The study medications were well tolerated. No patient discontinued the study due to medication side effects. The majority (57%) of reported symptoms were deemed to be unrelated to study

Steady State E2 90

Biest 2.5 mg

80

Day 1 E2 90

Biest 2.0 mg

Biest 3.0 mg Vivelle-Dot

70

Biest 2.5 mg

80

Biest 3.0 mg Vivelle-Dot

70

60 50

60 50

40

40

30

30

20

20

10

10 0

Biest 2.0 mg

0 0

5

10

15 Hours

20

25

Fig. 2. Mean estradiol across groups – initial 24-h curves.

30

0

5

10

15

20

25

30

Hours

Fig. 3. Mean estradiol across groups – steady-state (Days 15/16) curves.

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Table 5 Estrone pharmacokinetics at baseline, 24 h and steady-state in a phase I randomized clinical trial for evaluating estrogen pharmacokinetics. Characteristic BASELINE – single dose (all results measured in pg/mL) C0 Mean ± SD Median (min, max) C24 Mean ± SD Median (min, max) C24 − C0 Mean ± SD Median (min, max) Average Mean ± SD Median (min, max) AUCd Mean ± SD Median (min, max) End of study – steady-state (all results measured in pg/mL) C0 Mean ± SD Median (min, max) C24 Mean ± SD Median (min, max) C24 − C0 Mean ± SD Median (min, max) Average Mean ± SD Median (min, max) AUCd Mean ± SD Median (min, max)

Bi-est 2.0 mg (n = 10)

Bi-est 2.5 mg (n = 7)

Bi-est 3.0 mg (n = 10)

Vivelle-Dot 0.05 mg (n = 10)

23.9 ± 5.7 24 (26, 35)

24.6 ± 7.8 23 (24, 37)

31.3 ± 16.8 27.5 (12, 54)

29.2 ± 10.3 26.5 (17, 45)

30.4 ± 10.0a 28.5 (18, 52)

29.7 ± 6.8a 34 (21, 36)

39.8 ± 18.4 40.5 (15, 67)

51.3 ± 16.3 51.5 (27, 89)

6.5 ± 8.8a 2.5 (−2, 27)

5.1 ± 4.7b 4.0 (−3, 11)

8.5 ± 8.4a 8.0 (−1, 27)

22.1 ± 11.6 22 (10, 47)

23.6 ± 6.7c 22.9 (14.7, 33.6)

22.5 ± 8.6c 20.7 (12.3, 35.4)

31.1 ± 16.6 27.2 (12.0, 58.6)

35.1 ± 10.4 32.7 (20.7, 53.0)

563 ± 168a 550 (346, 830)

529.4 ± 219.5c 495 (255, 854)

747 ± 404 656 (283, 1427)

876 ± 254 844 (510, 1339)

28.6 ± 7.4a 27.5 (19, 42)

26.6 ± 9.4c 29 (11, 37)

40.7 ± 21.1 36 (15, 97)

50.7 ± 29.6 42.5 (18, 127)

30.6 ± 8.7b 28 (21, 46)

28.6 ± 7.0b 27 (19, 38)

38.0 ± 16.4c 35.5 (16, 59)

61.7 ± 31.8 56 (31, 146)

2.0 ± 5.1 3 (−5, 10)

2.0 ± 8.1 1 (−11, 15)

−2.7 ± 9.0c −0.5 (−23, 5)

11.0 ± 13.8 13.5 (−13, 29)

26.2 ± 5.8b 25.8 (19.5, 34.8)

25.6 ± 8.7a 26.5 (11.5, 40.2)

36.1 ± 17.0 31.8 (14.0, 62.7)

48.8 ± 23.0 42.4 (20.3, 107.2)

623 ± 137b 625 (476, 854)

615 ± 197a 605 (282, 934)

836 ± 376 757 (334, 1437)

1209 ± 556 1072 (514, 2613)

a

Rank sum test p < 0.01 compared to Vivelle-Dot 0.05 mg. Rank sum test p < 0.001 compared to Vivelle-Dot 0.05 mg. c Rank sum test p < 0.05 compared to Vivelle-Dot 0.05 mg. d At baseline (after a single dose) estrogen fractions were measured at 0, 2, 5, 8, 12, 18, and 24 h. At the end of study (steady-state) estrogen fractions were measured at 0, 2, 5, 8, 12 and 24 h. The area under the curve (AUC) was calculated according to the trapezoidal rule. b

medications (e.g. upper respiratory infection, gastroenteritis). Of the remaining symptoms, most were mild to moderate, and most (71%) resolved by day 23 at the time of final follow-up phone visit. The reported symptoms included abdominal bloating and pain (n = 6, 15%), upper respiratory infection (n = 5, 12.5%), fluid retention (n = 3, 7.5%), gastroenteritis (n = 3, 7.5%), skin irritation (n = 3, 7.5%), progesterone withdrawal bleed (n = 2, 5%), and insomnia, dizziness, fatigue and vaginal discharge in one patient each (n = 1, 2.5% each).

4. Discussion Our study was designed as a comparative prospective pharmacokinetic trial, with the goal to compare the pharmacokinetics of the conventional and compounded hormonal preparations that are considered bioequivalent in clinical practice. To the best of our knowledge, this is the first study of its kind in the literature. Contrary to our expectations, we found that the dose of Bi-est 2.5 mg, commonly prescribed in lieu of the estradiol 0.05 mg patch,

Table 6 Progesterone pharmacokinetics at baseline, 24 h and steady-state in a phase I randomized clinical trial for evaluating estrogen pharmacokinetics. Characteristic C0 Mean ± SD Median (min, max) C24 Mean ± SD Median (min, max) CSteady-state Mean ± SD Median (min, max) C24 − C0 Mean ± SD Median (min, max) Css – C0 Mean ± SD Median (min, max) Note: All results measured in ng/mL.

Bi-est 2.0 mg (n = 10)

Bi-est 2.5 mg (n = 7)

Bi-est 3.0 mg (n = 10)

Vivelle-Dot 0.05 mg (n = 10)

0.38 ± 0.23 0.30 (0.09, 0.80)

0.60 ± 0.52 0.63 (0.09, 1.59)

0.40 ± 0.27 0.32 (0.09, 0.86)

0.65 ± 0.35 0.52 (0.29, 1.37)

1.82 ± 1.85 1.29 (0.56, 6.89)

1.72 ± 0.72 1.73 (0.31, 2.52)

1.71 ± 0.62 1.70 (0.80, 2.59)

1.44 ± 0.50 1.38 (0.92, 2.54)

0.88 ± 0.37 0.90 (0.22, 1.27)

1.01 ± 0.57 1.12 (0.23, 1.87)

0.95 ± 0.40 0.95 (0.44, 1.51)

1.16 ± 0.53 1.18 (0.18, 2.16)

1.43 ± 1.92 0.92 (−0.04, 6.74)

1.12 ± 1.07 1.00 (−0.49, 2.43)

1.31 ± 0.62 1.44 (0.48, 2.28)

0.80 ± 0.69 0.68 (−0.44, 2.08)

0.50 ± 0.47 0.59 (−0.58, 1.09)

0.41 ± 0.93 0.49 (−1.01, 1.68)

0.55 ± 0.39 0.60 (−0.02, 1.20)

0.52 ± 0.74 0.58 (−1.19, 1.24)

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yielded much lower estrogen levels compared to the patch. Even a higher dose of Bi-est 3.0 mg yielded lower estrogen levels than the 0.05 mg Vivelle-Dot patch, although the difference didn’t reach statistical significance. We found that patterns of estrogen absorption with Bi-est creams were highly variable and showed no consistent peak of absorption. Vivelle-Dot, on the other hand, showed a pattern of absorption similar to what is reported in the literature [14]. These differences may be explained by the interindividual variations in skin physiology, blood flow, and hormone metabolism. More importantly, use of different vehicles of administration may also explain these differences, as seen from studies of estrogen in hydroalcoholic gels [14,15]. Our results cannot be compared directly to another cream-based preparation owing to non-availability of any such FDA-approved hormone cream. FDA-approved E3 assays test the high E3 levels of pregnancy. Their reliability in detecting the extremely low postmenopausal E3 levels is unproven. Acknowledging this limitation, our results showed a small rise in E3 in all treatment groups, regardless of whether E3 was administered exogenously or not. We observed a surprising trend toward increased E3 levels in the E2 patch group compared to the E2+E3 cream groups, which may be partly explained by endogenous conversion from higher E2 in the patch group to higher E3 levels. Overall, we observed only a small increase in E3 and hypothesize the possibility of a rapid conversion of E3 to some of its metabolites, or interference in its absorption due to Vanicream. Thus, future studies testing E3 metabolites and utilizing other vehicles of absorption are needed. In our study, progesterone levels were comparable at several time points after initial dosing as well as at steady-state in all groups, thereby suggesting that oral absorption of natural micronized progesterone is comparable across compounded and conventional preparations. From a clinical perspective, the finding of small increments in estradiol levels with low-dose Bi-est formulations raise the question of how much symptomatic benefit attributed to these doses is

30 BMI

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Fig. 5. Steady state E3.

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derived from a placebo effect. Our findings also raise the question as to whether the observed estrogen levels with the compounded formulations in current doses are sufficient to potentiate any bone benefits in menopausal women, which needs to be studied in future clinical trials. There are certain limitations to our study. First, our choice of particular formulations and dosing was empiric because there were no evidence-based guidelines available to direct us. Second, our results can be generalizable to Vanicream-based compounded formulations only. We chose Vanicream as the compounding medium as it is commonly used in the compounding pharmacy at our institution. Third, although we measured E3 levels in triplicate using a state-of-the-art automated immune assay, the test has significant variability and poor reliability at very low postmenopausal levels. Lastly, since we tested multiple medication doses, we chose the multiple arm randomized controlled design without cross-over due to time and cost issues. Our study has several strengths. First, this is the first study of its kind to compare the pharmacokinetics of compounded and conventional bioidentical hormones. Second, the study design was randomized, controlled, and blinded, which optimizes the reliability of results. All study medications were prepared and dispensed by the same experienced compounding pharmacist (RAW),

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thereby minimizing variation in compounding. The study utilized a strict protocol for medication application, thus reducing the potential for variability in results attributable to inconsistent administration of the product. Finally, the successful design and conduct of this study supports the feasibility of conducting research comparing compounded hormone therapies with well-studied, gold-standard hormone therapy products. This is important as the lay public, as well as medical providers, are increasingly seeking reliable information regarding these widely used products. In conclusion, this pharmacokinetic trial provides information regarding bioidentical compounded preparations and bioidentical conventional hormonal preparations that are considered bioequivalent in practice. More studies are needed to evaluate clinical as well as pharmacokinetic differences between compounded formulations, using various vehicles or administration and dosages. The knowledge gained from this study provides the groundwork for future trials to determine the safety and efficacy of bioidentical compounded hormones. This successfully conducted randomized, controlled, blinded multi-group study attests to the feasibility of using a similar design in the setting of a larger clinical trial. Contributors Richa Sood, Lynne Shuster, Darrell Schroeder conceptualized and designed the study. The manuscript was drafted by Richa Sood, Lynne Shuster, Deborah Rhodes, Dietlind Wahner-Roedler, Rebecca Bahn. Laboratory services and analysis were carried out by Ravinder Singh. Pharmaceutical services were provided by Roger Warndahl. Analysis and interpretation of data were done by Richa Sood, Darrell Schroeder, Ravinder Singh, Lynne Shuster, Rebecca Bahn, Deborah Rhodes. Statistical analysis was carried out by Darrell Schroeder. All authors have read and approved the final version of the manuscript. Competing interest The authors declare no conflict of interest. Funding Funding was received by Solvay, an educational grant for Women’s Health Fellowship, for this article.

Role of funding source Solvay was not involved with the study design, data collection and analysis, or writing of the paper. Ethical approval The study was approved by the Mayo Clinic institutional Review Board. References [1] Aso T. Demography of the menopause and pattern of climacteric symptoms in the East Asian region. In: First consensus meeting on menopause in the East Asian Region. 1997. [2] Gracia CR, Freeman EW. Acute consequences of the menopausal transition: the rise of common menopausal symptoms. Endocrinology and Metabolism Clinics of North America 2004;33:675–89. [3] Iosif CS, Bekassy Z. Prevalence of genito-urinary symptoms in the late menopause. Acta Obstetricia et Gynecologica Scandinavica 1984;63:257–60. [4] Gregersen N, Jensen PT, Giraldi AE. Sexual dysfunction in the peri- and postmenopause. Status of incidence, pharmacological treatment and possible risks. A secondary publication. Danish Medical Bulletin 2006;53:349–53. [5] Clayton AH, Ninan PT. Depression or menopause? Presentation and management of major depressive disorder in perimenopausal and postmenopausal women. Primary Care Companion to the Journal of Clinical Psychiatry 2010;12. PCC08r00747. [6] Freeman EW. Associations of depression with the transition to menopause. Menopause 2010;17:823–7. [7] Woods NF, Mitchell ES. Sleep symptoms during the menopausal transition and early postmenopause: observations from the Seattle Midlife Women’s Health Study. Sleep 2010;33:539–49. [8] Landis CA, Moe KE. Sleep and menopause. Nursing Clinics of North America 2004;39:97–115. [9] National Institutes of Health. NIH State-of-the-Science Conference Statement on management of menopause-related symptoms. NIH Consensus and Stateof-the Science Statements 2005;22:1–38. [10] Poniatowski BC, Grimm P, Cohen G. Chemotherapy-induced menopause: a literature review. Cancer Investigation 2001;19:641–8. [11] Hulley S, Grady D, Bush T, et al. Randomized trial of estrogen plus progestin for secondary prevention of coronary heart disease in postmenopausal women. Heart and Estrogen/progestin Replacement Study (HERS) Research Group. Journal of the American Medical Association 1998;280:605–13. [12] Rossouw JE, Anderson GL, Prentice RL, et al. Risks and benefits of estrogen plus progestin in healthy postmenopausal women: principal results from the Women’s Health Initiative randomized controlled trial. Journal of the American Medical Association 2002;288:321–33. [13] Sood R, Shuster L, Smith R, Vincent A, Jatoi A. Counseling postmenopausal women about bioidentical hormones: ten discussion points for practicing physicians. Journal of the American Board of Family Medicine 2011;24:202–10. [14] Jarvinen A, Nykanen S, Paasiniemi L. Absorption and bioavailability of oestradiol from a gel, a patch and a tablet. Maturitas 1999;32:103–13. [15] Kuhl H. Pharmacology of estrogens and progestogens: influence of different routes of administration. Climacteric 2005;8(Suppl. 1):3–63.