Standard solutions
Transfer 0.5 mL of the
Test solution to a 100-mL volumetric flask, dilute with acetone to volume, and mix
(Standard solution A). Dissolve 10 mg, accurately weighed, of
USP Ethylparaben RS in 1 mL of the
Test solution, and dilute with acetone to 10 mL
(Standard solution B).
Procedure
Separately apply 2 µL of the
Test solution and 2 µL of each
Standard solution to a thin-layer chromatographic plate (see
Chromatography 621) coated with a 0.25-mm layer of chromatographic octadecylsilanized silica gel mixture. Develop the chromatogram in a solvent system consisting of a mixture of methanol, water, and glacial acetic acid (70:30:1) until the solvent front has moved about three-fourths of the length of the plate. Remove the plate from the chamber, mark the solvent front, and allow the solvent to evaporate. Examine the plate under short-wavelength UV light, and compare the intensities of any secondary spots observed in the chromatogram of the
Test solution with that of the principal spot in the chromatogram of
Standard solution A: the intensity of any individual secondary spot in the chromatogram of the
Test solution is not greater than that of the principal spot obtained in the chromatogram of
Standard solution A (0.5%). The test is not valid unless the chromatogram obtained with
Standard solution B shows two clearly separated principal spots.