Method 1—

pH 6.8 PHOSPHATE BUFFER—Mix 64 mL of 0.2 M monobasic sodium phosphate and 61 mL of 0.1 M dibasic sodium phosphate in a 1-liter volumetric flask, dilute with water to volume, and mix.

MOBILE PHASE —Prepare a filtered and degassed mixture of methanol and pH 6.8 phosphate buffer (625:375). Make adjustments if necessary (see System Suitability under Chromatography 621).

CHROMATOGRAPHIC SYSTEM (see Chromatography 621)—The liquid chromatograph is equipped with a 3.9-mm × 30-cm column that contains 10-µm packing L1. It is also equipped with a flow-through gamma ray detector having a cell volume of about 10 µL. A constant flow rate of about 1 mL per minute is maintained, and counts are recorded and charted at about 5-second intervals.

PROCEDURE —Constitute the Injection, and allow to stand for 15 minutes. Chromatograph a volume of Injection, with activity of 0.6 to 15 MBq (16 to 400 µCi), and record the chromatogram. The resolution between the secondary characteristic peak, eluting at about 3.5 minutes, and the principal peak, eluting at about 6 minutes, is not less than 1.5. The time interval between the elution of the Tc 99m pertechnetate peak, at about 2 minutes, and the principal peak is not less than 3.0 minutes. If the foregoing criteria are met, record the counts for the pertechnetate Tc 99m peak, the two complex peaks, a representative baseline segment, and the total counts for the chromatogram. Calculate the percentage of complexed radioactivity in the two characteristic peaks taken by the formula: in which C is the count of the complex peak of interest, T is the total count, and P is the pertechnetate peak count, each being corrected for the corresponding baseline count. The complexed radioactivity is not less than 90.0% in the principal peak and between 1% and 6% in the second characteristic peak. Calculate the percentage of all other complexed radioactivity (this excludes the main, secondary, and free pertechnetate peaks) taken by the formula: in which K is the sum of all other peaks, and T and P are as defined above. Record the result for use in the calculation as directed under Method 2.

Method 2—

CHROMATOGRAPHIC SYSTEM A (see Chromatography 621)—Prepare a 1.0- × 12.5-cm silicic acid-impregnated glass microfiber strip by dipping it in a 10% sodium chloride solution and removing the excess liquid by blotting. Dry the strip by heating in an oven at about 80. Apply about 5 µL of the Injection with activity of about 3.7 MBq (100 µCi) about 1.5 cm from one end of the strip, and immediately develop the chromatogram in a chromatographic chamber containing saturated sodium chloride solution until the solvent front reaches a level about 1 cm from the top of the strip. Remove the strip from the chamber, and allow to air-dry. Separate the top and bottom portions of the chromatogram by cutting the strip in half, and record the counts separately for each portion. Calculate the percentage of unreduced pertechnetate taken by the formula: in which P is the count from the top half of the strip, and C is the count from the bottom half of the strip.

CHROMATOGRAPHIC SYSTEM B —Proceed as directed under Chromatographic system A except to use a 1.0- × 12.5-cm silica gel-impregnated glass microfiber strip, without preliminary treatment, and a mixture of acetonitrile and water (3:1) as the developing solvent. Calculate the percentage of reduced hydrolyzed Tc 99m taken by the formula: in which R is the count from the bottom half of the strip, and D is the count from the top half of the strip. The sum of the percentage of unreduced pertechnetate from System A, the percentage of reduced hydrolyzed Tc 99m from System B, and the percentage of other complexed radioactivity determined from Method 1 is not greater than 10.0%.

100(A/B),