Sulfadiazine plasma concentrations in women with pregnancy-acquired compared to ocular toxoplasmosis under pyrimethamine and sulfadiazine therapy: a case–control study

This retrospective case–control study covers the period from 1997 until 2011, during which plasma samples had been submitted for drug-level testing from a consecutive series of 89 pregnant women aged 18.8 to 43.8 years (mean 29.6 ± 6.0, [95% confidence interval: 28.4; 30.9]) receiving anti-parasitic treatment for proven or suspected primary Toxoplasma infection (PT) (Table 1). All women had reached or passed the 16^th week of pregnancy when they received the combination therapy according to the following standard dosages: PY 50 mg on the first day, then 25 mg/day and SA 50 mg/kg of body weight/d up to a maximum dosage of 4.0 g/day, divided into three to four doses per day that were supplemented with folinic acid (10–15 mg per week) according to the recommendation of the German federal health authorities, Robert Koch Institute protocol established in 1988 (https://​www.​rki.​de/​DE/​Content/​Infekt/​EpidBull/​Merkblaetter/​Ratgeber_​Toxoplasmose.​html). Drug prescription and patient supervision were effected by their respective obstetricians. Treatment lasted a minimum of 4 weeks and began right after the diagnosis of Toxoplasma infection had been confirmed. Blood or plasma samples were collected approximately 14 days after treatment onset and sent to the Southern German reference laboratory (Laboratory Harald Hlobil, Sindelfingen, Germany) to quantify the plasma concentrations of PY and SA.

Serum samples from 17 HIV-negative women of similar age (17–35, mean 26.1 ± 5.3 [23.6; 28.5] years) who had been treated at the Uveitis Clinic of the University Hospital Bern (Inselspital) for acute symptomatic Toxoplasma retinochoroiditis between 1992 and 2001 were available for comparison (Tables 1 and 2). These patients with OT had initiated treatment with a loading dose of 75 mg PY, followed by 25 mg PY given twice daily, whereas the same SA dosage as in the PT group was given for a minimum of 6 weeks. Blood samples were routinely drawn from all individuals for side effect control approximately 14 days after treatment initiation (range 11–17 days). Unused samples were stored at − 18 °C in a biobank until their analysis in 2011. To confirm the stability of PY and SA in plasma during long-term storage at − 18 °C, we additionally included samples from 10 HIV-negative male patients treated during the same period for acute OT for which the same sampling, storage, and analysis protocols had been followed. Baseline characteristics of this group are displayed in Table 2. More recent blood samples from patients treated after 2001 were not available, since the treatment protocol had been changed from PY/SA to the fix combination pyrimethamine and sulfadoxine (Fansidar®) in 2001 and to the fixed-dose combination of trimethoprim 160 mg and sulfamethoxazole 800 mg twice a day by 2004. Since all individuals were outpatients, no information pertaining to the exact times of drug intake and blood sampling was available. As a result, it was impossible to calculate individual trough-to-peak ratios.

Plasma concentrations of PY and SA were assayed in the same advisory laboratory using chromatography on the day of blood collection (PT) or after thawing of the stored samples (OT). Analysis was done by liquid chromatography–mass spectrometry (HPLC–MS/MS 3200 Q Trap, Sciex, Germany). For this, 50 μl of plasma/serum sample was mixed with 225 μl of methanol (MeOH; Rotisolv HPLC-Grade, Roth Germany), 25 μl of acetonitrile (Rotisolv pestilyse, Roth, Germany) and an internal standard (droperidol) as systematic test performance control and homogenized for 1 min, before the mixture was precipitated for 10 min at 13,000 rpm. In all, 100 µl of the supernatant was used for LC–MS according to the manufacturer’s instructions. Four additional specific internal standards (ISs) were prepared by spiking drug-free serum with known amounts of PY (Sigma Aldrich, Germany, P-7771) or SA (LGC Standards). The concentrations of the ISs for PY were level 1 (200 µg/l), level 2 (400 µg/l), level 3 (1000 µg/l), and level 4 (2000 µg/l) and for SA were level 1 (10 mg/l), level 2 (20 mg/l), level 3 (50 mg/l), and level 4 (100 mg/l). Low positive controls (PY 500 µg/l, SA 25 mg/l) and high positive controls (PY 1200 µg/l, SA 60 mg/l) were added. The described method (hereafter named LC–MS) was validated and proved to be sensitive, selective, and accurate for quantification of PY and SA in human serum/plasma samples. Intra-assay coefficients of variation (CVs) were as follows: for PY control 1 (500 µg/l): CV = 2.0%, and control 2 (1200 µg/l): CV = 0.9% and for SA control 1 (25 mg/l): CV = 2.10% and control 2 (60 mg/l): CV = 0.9%. The ISs were confirmed to be stable under storage at ≤ 16 °C for 1 year. No peaks interfering with quantification were observed throughout the validation process. The assay had lower detection limits of 30 µg/l for PY and 9 mg/l for SA. Calculated intra- and interday CVs remained below 10%.

SPSS (IBM SPSS Statistics for Windows, Version 22.0. Armonk, NY: IBM Corp.) and SAS 9.4. (SAS Institute Inc., Cary, NC, USA) were used to analyse the data. Parametric data (age, days after initiation of therapy) are given in the text with range, mean ± standard deviation (SD) and corresponding 95% confidence intervals (CIs). The non-parametric serum concentrations of PY and SA are shown in the text as medians and corresponding 95% CIs. The 95% CIs of the medians were calculated with SPSS using bootstrapping. Differences between OT and PT were analysed using the t-test for independent samples for age and days after initiation of treatment and the Mann–Whitney U-test for the serum concentration of PY and SA. A p-value < 0.05 was considered significant.