Enhancing simultaneous determination of some angiotensin II receptor antagonists and amlodipine in plasma using HPTLC with fluorescence densitometry: Independent fluorescence detection of the co-administrative drugs in the mixture across various pH conditions.

A novel and highly sensitive high-performance thin-layer chromatographic (HPTLC) method was developed and validated to quantify a combination of five pharmaceutical mixtures spiked to human plasma. The compounds comprised Amlodipine (AML) along with five angiotensin II receptor antagonist drugs (AIIRAs), namely Olmesartan (OLM), Telmisartan (TLM), Candesartan (CAN), Losartan (LOS), and Irbesartan (IRB). HPTLC was performed on silica gel 60 F254 plates using a mobile phase of Toluene: ethyl acetate: methanol: acetone: acetic acid (6:1.5:1:0.5:1, v/v/v/v/v). In a pioneering move, a reflectance/fluorescence detection mode was employed to identify two concurrently administered drugs at different pH levels for the first time. This method utilized the same chromatographic system, incorporating a specific measurement for AML at a neutral medium to achieve its maximum fluorescence at a 360 nm excitation wavelength, and measuring emission using a 540 nm optical filter. The process involved obtaining a very low fluorescence response from AIIRA. Subsequently, to enhance AIIRA's fluorescence, the plate was sprayed with perchloric acid to transition to a strong acidic medium, ultimately attaining the maximum fluorescence of AIIRA using various excitation wavelengths and a 400 nm emission filter. Through this strategic process, we could optimize the fluorescence signals of both drugs, thereby elevating the sensitivity of detection for this drug combination. AML demonstrated a linear range of 18-300 ng/band, while AIIRAs drugs exhibited a linear range of 6-150 ng/band. The method satisfied the International Conference on Harmonization (ICH) criteria for recovery, precision, repeatability, and robustness, showcasing exceptional sensitivity. The approach was successfully applied to quantify AML and AIIRAs drugs in both bulk drug and plasma samples, achieving high recovery percentages and minimal standard deviations.

Ultrasensitive TLC determination of montlukast and loratadine mixture in human plasma utilizing fluorescence detection at dual pH values: Toward attaining separate maximum fluorescence intensity.

A novel selective and highly sensitive TLC densitometric method with reflectance/fluorescence detection was developed to separate and quantify montlukast (MONT) and loratadine (LOR). Separation of the studied drugs was performed on precoated silica gel TLC plates using chloroform-ethyl acetate (8 :2 v/v) as a mobile phase. MONT quantification was carried out by measuring emission using 400 nm optical filter after excitation at 340 nm. Enhancement of the week LOR fluorescence was performed through adequate spraying the chromatograms with 0.2 M perchloric acid leading to enhancing sensitivity by 17 folds compared to the reported HPTLC methods with absorbance detection. The scanner was set at 275 nm excitation wavelength and 400 nm optical filter. Detection of both drugs on the same plate separately at different pH conditions was utilized for the first time. Maximum fluorescence was achieved for each of them and this enhances detection sensitivity for both drugs. The linear regression analysis data of the studied drugs produced a good linear relationship with correlation coefficients of 0.996 for MONT and 0.998 for LOR over the concentration range of 6 - 150 ng/band for MONT and 15 - 120 ng/band for LOR. Limit of detection values were 1.7 and 4.5 ng /band for MONT and LOR respectively. The developed method enabled the detection of MONT and LOR in human plasma samples within linear concentrations ranged from 7 to 140 ng/ band and 16 to 50 ng/ band with detection limits of 1.9 and 4.8 ng/band for MONT and LOR respectively. The analytical performance of the proposed method was evaluated according to the International Council for Harmonization (ICH). The method was successfully applied for the analysis of the studied drugs in spiked human plasma and good recovery percentages were obtained indicating that there is no interference from plasma constituents. Therefore the method can be applied for in vivo analysis and pharmacokinetic study.