8% for AT and accuracy of 92 9% and precision less than 5 4% for

8% for AT and accuracy of 92.9% and precision less than 5.4% for EZ. The stability of the two drugs under various conditions is shown in Table 4. Under all conditions tested, the two drugs proved to be stable. All results were within the acceptance criteria of ±15% deviation from the nominal concentration. The mean plasma level of AT and EZ in both products A and B are shown in Fig. 4a and b. Table 5 shows the parameters for the non-compartmental pharmacokinetic

analysis. According to ANOVA results there is no significant sequence effect for both cmax and AUC0–72 h indicating that the crossover design was properly performed. The parametric point estimates and the 90% confidence intervals for ln-transformed AUC0–t, AUC0–∞, and cmax, ( Table 6) were within commonly accepted bioequivalence range of 80–125% range, thus the results reveal Protein Tyrosine Kinase inhibitor Adriamycin price that the bioequivalence between products A and B could be concluded. A rapid, sensitive,

and simple method for determining AT and EZ levels in human plasma was developed and validated. The UPLC–MS/MS method described herein reveals significant advantages over other techniques, including LC–MS/MS, due to the inherently increased column efficiency of UPLC, which resulted in complete analysis within 1.2 min with significantly lower limits of quantitation (0.1 ng mL−1). To the best of our knowledge, this is the first UPLC–MS/MS method for the simultaneous determination of AT and EZ in human plasma. This fully validated method was an ideal tool for high-throughput Phosphatidylinositol diacylglycerol-lyase analysis of plasma samples used in pharmacokinetic and bioequivalence study of AT and EZ between two market products. All authors have none to declare. Special thanks to Prof. Dr. Meselhy Ragab Meselhy for allowing the performance of this research in the “Center of Applied Research and Advanced Studies” (CARAS), Faculty of Pharmacy, Cairo University. “
“Treatment of tuberculosis is now very complex because of the emergence of multi drug resistant bacteria, which are resistant to first-line anti-tuberculosis drugs, pyrazinamide, isoniazid and rifampin.1 Pyrazinamide (Fig. 1) is used extensively

in the treatment of tuberculosis together with rifampicin, isoniazid and ethambutol.2 The structure of pyrazinamide is given by Fig. 1 and the structure of metronidazole is given by Fig. 2. It has a plasma half-life of 3–4 h, and is quickly absorbed from the gastrointestinal tract with peak serum concentrations of 6–8 μg/ml occurring 1.5–2.0 h after administration.3 The determination of PZA levels in biological fluids was carried out earlier by spectroscopic methods,4, 5 and 6 colorimetric methods7 and gas chromatographic–mass spectrometric technique.8 A survey of literature revealed that HPLC technique has been used for the determination of pyrazinamide in pharmaceuticals.9 A HPLC technique reported earlier had a step of very tedious extraction.

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