Rapid and Microdetermination of Carbon Monoxide in Blood using Oxygen Electrode and Light Irradiation Apparatus

Abstract

The authors deviced a rapid microdetermination carbon monoxide (CO) in blood using polarographic oxygen (O₂) electrode and light irradiation apparatus. This method consists of following procedures; (1) 15μl of the CO-biood was aded into 1 ml of O₂-depleted water (O₂: 4-5 μg/ml) in the closed glass cell fixed O₂ electrode. By this step, deoxyhemoglobin (HHb) in the CO-blood was saturated with dissolved O₂ in the O₂-depleted water to become oxyhemoglobin (HbO₂). The amount (a) of oxygen corresponding to [HbO₂ (a') formed from HHb and HbO₂ (a') already existed] in the sample was recorded by addition of 10 μl of 10% K₃Fe (CN)₆.(2) The same CO-blood diluted with water was bubbled by O₂ gas under light irradiation. By this procedure, HHb and HbCO in the CO blood were completely changed into HbO₂ The quantity (b) of O₂ combined with total Hb was determined by addition of 10 μl of 10% K₃Fe (CN)₆, successively. The value, [(b-a)/b] ×100, indicates the per cent of HbCO on the total Hb of the CO-blood tested. This method requires only 35 μl of the CO-blood and 6-7 min for each determination. Results showed excellent agreement with those obtained by spectrophotometry (r=0.993, y=0.95× ±2.14). Within-run precision was measured from 30 blood samples containing 50.0% HbCO, and the standard deviation and coefficient of variation were ±1.3% HbCO and 2.6%, respectively.