Abstract

A selective, specific and stability-indicating gradient reverse phase high-performance liquid chromatographic (HPLC) method was developed for the determination of Ranitidine in presence of its impurities, forced degradation products and placebo substances such as saccharide and parabens. Ultraviolet detection was performed at 230 nm. Separate portions of the drug product and ingredients were exposed to stress conditions to induce oxidative, acidic, basic, hydrolytic, thermal and photolytic degradation. Ranitidine was found to degrade significantly at acidic, basic and oxidative stress conditions but was stable at heat and humidity. The developed method was validated as per International Conference on Harmonization (ICH) guidelines. The method was validated over this range for (i) system suitability (ii) specificity, (iii) precision, (iv) limit of detection and limit of quantification, (v) linearity, (vi) accuracy, (vii) robustness. The method was found to be precise, accurate, linear and robust. The proposed method was successfully employed for estimation of Ranitidine impurities in pharmaceutical preparations.

Highlights

  • Ranitidine hydrochloride (HCl), USP, is a histamine H2-receptor antagonist

  • Many analytical approaches are available for the related substances of ranitidine in tablet formulations and drug substances [1,2,3]

  • Now-a-days, pharmaceutical industry is forced to assess a strict control of impurities when manufacturing drug substance and drug products

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Summary

A Validated Stability-Indicating

Liquid-Chromatographic Method for Ranitidine Hydrochloride in Liquid Oral Dosage Form. Nitish SHARMA * 1,2, Surendra Singh RAO 1, Namala Durga Atchuta KUMAR 1, Pingili Sunil REDDY 1, Annarapu MALLESWARA REDDY 1. Published: Accepted: February 12th 2011 February 10th 2011 doi:10.3797/scipharm.1101-06. © Sharma et al.; licensee Österreichische Apotheker-Verlagsgesellschaft m.

Introduction
Method Validation
Method Development and Optimization
Conclusions
Full Text
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