Gentamicin and Hydrocortisone Acetate Ear Drops

Aminoglycoside antibacterial (Gentamicin Sulfate); corticosteroid (Hydrocortisone Acetate).

Gentamicin and Hydrocortisone Acetate Ear Drops contain Gentamicin Sulfate and Hydrocortisone Acetate suspended in a suitable vehicle.

The ear drops comply with the requirements stated under Ear Preparations and with the following requirements.

95.0 to 105.0% of the stated amount.

A. Carry out the method for thin-layer chromatography, Appendix III A, using the following solutions.

(1) Dilute a volume of the ear drops, if necessary, with sufficient water to produce a solution containing the equivalent of 0.3% w/v of gentamicin, filter and use the filtrate.

(2) 0.5% w/v of gentamicin sulfate BPCRS in water.

(a) Use a silica gel precoated plate (Merck silica gel 60 plates are suitable).

(b) Use the mobile phase as described below.

(c) Apply 10 µL of each solution.

(d) Develop the plate to 15 cm.

(e) After removal of the plate, allow it to dry in air, spray with ninhydrin solution R1 and heat at 105° for 2 minutes.

The lower layer obtained by shaking together equal volumes of 13.5m ammonia, dichloromethane and methanol and allowing to separate.

The three principal spots in the chromatogram obtained with solution (1) are similar in position, colour and size to those in the chromatogram obtained with solution (2).

B. Comply with the test for Composition of gentamicin sulfate.

C. Filter 20 mL of the well-mixed ear drops (Whatman No. 1 filter paper is suitable), wash the residue with the minimum amount of water, dry at 105° and dissolve 50 mg of the residue obtained in 50 mL of ethanol (96%). Add 2 mL of sulfuric acid to 2 mL of the resulting solution; an intense yellow colour is produced which exhibits a green fluorescence which is particularly intense when viewed under ultraviolet light (365 nm). Add the solution to 10 mL of water and mix; the fluorescence under ultraviolet light (365 nm) does not disappear.

D. In the Assay for hydrocortisone acetate, the chromatogram obtained with solution (1) shows a peak with the same retention time as the principal peak in the chromatogram obtained with solution (2).

pH, 6.0 to 7.0, Appendix V L.

Carry out the method for liquid chromatography, Appendix III D, using the following solutions.

(1) Add 5 mL of methanol to 10 mL of a solution prepared by diluting a suitable volume of the ear drops with water to contain the equivalent of 0.045% w/v of gentamicin. Swirl and add 4 mL of phthalaldehyde reagent, mix and add sufficient methanol to produce 25 mL, heat in a water bath at 60° for 15 minutes and cool. If the solution is not used immediately, cool to 0° and use within 4 hours.

(2) Prepare in the same manner as solution (1) but using 10 mL of a 0.065% w/v solution of gentamicin sulfate BPCRS in place of 10 mL of the preparation being examined.

(a) Use a stainless steel column (12.5 cm × 4.6 mm) packed with end-capped octadecylsilyl silica gel for chromatography (5 µm) (Hypersil ODS and Kromasil C18 are suitable).

(b) Use isocratic elution and the mobile phase described below.

(c) Use a flow rate of 1.5 mL per minute.

(d) Use an ambient column temperature.

(e) Use a detection wavelength of 330 nm.

(f) Inject 5 µL of each solution.

0.025m sodium heptanesulfonate monohydrate in a mixture of 5 volumes of glacial acetic acid, 25 volumes of water and 70 volumes of methanol.

When the chromatograms are recorded under the prescribed conditions the retention time of component C₂ is 10 to 20 minutes. The retention times relative to component C₂ are: about 0.13 (reagent); about 0.27 (component C₁); about 0.65 (component C_1a); about 0.85 (component C_2a).

The test is not valid unless, in the chromatogram obtained with solution (2), the resolution factor between the peaks due to components C_2a and C₂ is at least 1.3.

Using the chromatogram obtained with solution (1) calculate the percentage content of components C₁, C_1a, C₂ and C_2a in the ear drops by normalisation. The proportions are within the following limits:

C₁, 25.0 to 50.0%;

C_1a, 10.0 to 35.0%;

C₂ plus C_2a, 25.0 to 55.0%.

Dilute a volume of the ear drops containing the equivalent of 15 mg of gentamicin to 50 mL with sterile phosphate buffer pH 8.0 and dilute 10 mL of the resulting solution to 50 mL with the same solvent. Carry out the microbiological assay of antibiotics, Appendix XIV A. The precision of the assay is such that the fiducial limits of error are not less than 95% and not more than 105% of the estimated potency.

Calculate the content of gentamicin in the ear drops, taking each 1000 IU found to be equivalent to 1 mg of gentamicin. The upper fiducial limit of error is not less than 90.0% and the lower fiducial limit of error is not more than 120.0% of the stated content.

Carry out the method for liquid chromatography, Appendix III D, using the following solutions.

(1) Shake a quantity of the ear drops containing 0.1 g of Hydrocortisone Acetate with 25 mL of methanol, add sufficient methanol to produce 100 mL and dilute 10 mL of this solution to 50 mL with the mobile phase.

(2) Dilute 10 mL of a 0.1% w/v solution of hydrocortisone acetate BPCRS in methanol to 50 mL with the mobile phase.

(a) Use a stainless steel column (12.5 cm × 4.6 mm) packed with octadecylsilyl silica gel for chromatography (5 µm) (Spherisorb ODS 1 is suitable).

(b) Use isocratic elution and the mobile phase described below.

(c) Use a flow rate of 2 mL per minute.

(d) Use an ambient column temperature.

(e) Use a detection wavelength of 256 nm.

(f) Inject 20 µL of each solution.

400 volumes of water and 600 volumes of methanol.

Calculate the content of C₂₃H₃₂O₆ in the ear drops using the declared content of C₂₃H₃₂O₆ in hydrocortisone acetate BPCRS.

Gentamicin and Hydrocortisone Acetate Ear Drops should not be allowed to freeze.

The quantity of Gentamicin Sulfate is stated in terms of the equivalent amount of gentamicin.