Specific rotation 
781S
:
between +84
and +89
.
Test solution:
5 mg per mL, in a pH 7 buffer. Prepare the pH 7 buffer solution as follows. Dissolve 5 g of monobasic potassium phosphate and 11 g of dibasic potassium phosphate in 900 mL of water, adjust with phosphoric acid or 5 N sodium hydroxide to a pH of 7, dilute with water to 1000 mL, and mix.
Loss on drying (see Thermal Analysis 891)—
[NOTE—The quantity taken for the determination may be adjusted, if necessary, for instrument sensitivity. Weight loss occurring at temperatures above about 160
, indicative of decomposition, is not to be interpreted as
Loss on drying.
] Determine the percentage of volatile substances by thermogravimetric analysis on an appropriately calibrated instrument, using 5 to 10 mg of Imipenem, accurately weighed. Heat the specimen under test at a rate of 20
per minute under vacuum. Record the thermogram to 200
, and calculate the weight loss at the plateau or inflection point at about 150
: it loses not less than 5.0% and not more than 8.0% of its weight.
Solvents—
Internal standard solution—
Add 1 mL of n-propyl alcohol to 2000 mL of water, and mix.
Standard preparation—
Transfer 1.0 mL of acetone and 2.0 mL of isopropyl alcohol to a 1000-mL volumetric flask, dilute with water to volume, and mix. Transfer 1.0 mL of this solution and 5.0 mL of Internal standard solution to a 25-mL volumetric flask, dilute with water to volume, and mix. Each mL of this Standard preparation contains 31.6 µg of acetone and 63.2 µg of isopropyl alcohol.
Test preparation—
Transfer about 250 mg of Imipenem, accurately weighed, to a 10-mL volumetric flask, add 4.0 mL of 1 N ammonium hydroxide, and dissolve by swirling. Add 2.0 mL of Internal standard solution, dilute with water to volume, and mix.
Chromatographic system
(see
Chromatography 621)—The gas chromatograph is equipped with a flame-ionization detector and a 3-mm × 1.8-m column containing 10% phase G16 on support S5. The column temperature is programmed to operate at 70
for 8 minutes, then to increase at a rate of 32
per minute to 170
, and to maintain the temperature at 170
for 8 minutes. The injection port is maintained at 200
, the detector is maintained at 250
, and helium is used as the carrier gas at a flow rate of about 19 mL per minute. Chromatograph the
Standard preparation, and record the peak responses as directed under
Procedure: the relative retention times are about 0.3 for acetone, 0.5 for isopropyl alcohol, and 1.0 for
n-propyl alcohol, and the relative standard deviation of each of the ratios of the response of the respective analyte peak to the response of the
n-propyl alcohol peak for replicate injections is not more than 5%.
Procedure—
[NOTE—Use peak areas where peak responses are indicated.
] Separately inject equal volumes (about 2 µL) of the
Standard preparation and the
Test preparation into the chromatograph, using the solvent (water) flush technique, record the chromatograms, and measure the responses for the acetone, isopropyl alcohol, and
n-propyl alcohol peaks. Calculate the percentages of acetone and isopropyl alcohol in the portion of Imipenem taken by the same formula:
(C / W)(RU / RS),
in which
C is the concentration, in µg per mL, of the appropriate analyte in the
Standard preparation; W is the quantity, in mg, of Imipenem taken to prepare the
Test preparation; and
RU and
RS are the ratios of the peak response of each of the corresponding analytes to the peak responses of
n-propyl alcohol obtained from the
Test preparation and the
Standard preparation, respectively. Add the percentages of acetone and isopropyl alcohol found: the total is not more than 0.25%.
Assay—
Mobile phase—
Dissolve 0.54 g of monobasic potassium phosphate in 3600 mL of water, adjust with 0.5 N sodium hydroxide or 0.5
M phosphoric acid to a pH of 6.8 ± 0.1, dilute with water to make 4000 mL of solution, and mix. Filter this solution through a filter of 0.5-µm or finer porosity, and degas. Make adjustments if necessary (see
System Suitability under
Chromatography 621).
Standard preparation—
Dissolve an accurately weighed quantity of
USP Imipenem Monohydrate RS in
Mobile phase to obtain a solution having a known concentration of about 0.4 mg per mL. Store this solution in an ice bath, and discard after 8 hours.
Assay preparation—
Transfer about 100 mg of Imipenem, accurately weighed, to a 250-mL volumetric flask, dissolve in and dilute with Mobile phase to volume, and mix. Store this solution in an ice bath, and discard the unused portion after 8 hours.
Chromatographic system (see Chromatography 621)—
The liquid chromatograph is equipped with a 300-nm detector and a 4.6-mm × 30-cm column that contains packing L1, and is maintained at a temperature of 30 ± 1.0
. The flow rate is about 1.5 mL per minute. Chromatograph the
Standard preparation, and record the peak responses as directed for
Procedure: the column efficiency determined from the analyte peak is not less than 600 theoretical plates, and the relative standard deviation for replicate injections is not more than 1.0%.
Procedure—
Separately inject equal volumes (about 10 µL) of the
Standard preparation and the
Assay preparation into the chromatograph, record the chromatograms, and measure the responses for the major peaks. Calculate the quantity, in mg, of imipenem monohydrate (C
12H
17N
3O
4S·H
2O) in the portion of Imipenem taken by the formula:
(317.36 / 299.35)(0.25CP)(rU / rS),
in which 317.36 and 299.35 are the molecular weights of imipenem monohydrate and anhydrous imipenem, respectively;
C is the concentration, in mg per mL, of
USP Imipenem Monohydrate RS in the
Standard preparation; P is the content, in µg per mg, of anhydrous imipenem (C
12H
17N
3O
4S) in
USP Imipenem Monohydrate RS; and
rU and
rS are the imipenem peak responses obtained from the
Assay preparation and the
Standard preparation, respectively.
;)
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