Radioimmunoassay for the detection of leptin in human serum

 

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Summary

Human leptin, which is encoded by the obese (ob) gene, is secreted specifically from adipocytes and is involved in the regulation of satiety and energy consumption. We developed a radioimmunoassay for the determination of leptin in human serum using polyclonal antibodies generated in rabbits against a C-terminal fragment of leptin, leptin_(126–140), coupled to hemocyanin. The sensitivity of the assay was app. 5 pmol/l leptin_(126–140) equivalent to 0.5 fmol/tube. The intra-assay variation at 100 pmol/l was less than 4.8% and the interassay variation less than 8.3%. Dilution curves of serum samples containing high levels of leptin_(126–140) were parallel to the standard curve. Following G-50 Sephadex chromatograpy a single specific peak was detected at app. 16 kd. The assay procedure compared well to a commercially available assay (Lineo, St. Louis, USA) using polyclonal antibodies directed against the intact recombinant protein (R=0.96; p < 0.0001). Serum levels were significantly higher than plasma levels (app. 20%) over a wide range of the standard curve.

Levels of serum leptin_126–140 immunoreactivity were not altered by meals and no day-to-day variation was found. In a group of 148 healthy female and 108 healthy male subjects with a BMI between 18.2 and 40 kg/m² there was a significant difference between sexes with higher circulating serum levels in female than in male subjects when tested for identical BMI (p < 0.001). Serum leptin levels in both male and female subjects were positively related to BMI (p < 0.001) when analysed for lean and obese subjects whereas in lean subjects this relation was not apparent. No relation of serum leptin levels and age was detectable in subjects with a BMI up to 30 kg/m². These data support an important role of leptin in the regulation of body fat stores and BMI which is modulated by gender specific factors.