|
|
;)
454.96
,16
)-.
,16,17-trihydroxypregn-4-ene-3,20-dione cyclic 16,17-acetal with acetone
[3093-35-4].
197K
.
781S:
between +150
and +160.
731—
Dry it in vacuum at 100 for 3 hours: it loses not more than 1.0% of its weight.
281:
not more than 0.2%.
621) coated with a 0.25-mm layer of chromatographic silica gel mixture, into three equal sections, the first two sections to be used for the test solution and the third section for the blank. Apply 100 µL of the test solution to appropriate sections of the plate, drying each solution as it is applied with a current of warm air. Using a continuous elution chromatographic chamber, develop the chromatogram in a solvent system consisting of a mixture of chloroform and ethyl acetate (5:1) for about 2 hours. Remove the plate from the developing chamber, dry in an oven at 90 for 15 minutes, and locate the bands by viewing under short-wavelength UV light. Mark the principal band and any secondary bands. Quantitatively remove the silica gel containing these bands, including a corresponding blank segment, and transfer to separate glass-stoppered, 50-mL centrifuge tubes, combining the impurities if more than one impurity is present. Add 30.0 mL of dehydrated alcohol to the tubes containing the principal band and the corresponding blank, and add 10.0 mL of dehydrated alcohol to the tubes containing the combined impurities and the corresponding blank. Insert stoppers in the tubes, and shake gently on a reciprocating shaker for about 60 minutes. Centrifuge, dilute the principal band eluate and its corresponding blank eluate with an equal volume of dehydrated alcohol, and mix. Determine the absorbances of the clear supernatant eluates in 1-cm cells at the wavelength of maximum absorbance at about 239 nm, with a suitable spectrophotometer, using dehydrated alcohol as the blank. Calculate the percentage of chromatographic impurities by the formula:
467:
meets the requirements.