Differentiation of keratein from bovine and canine hair by passive hemagglutination.

The possibility of keratein species differentiation was examined using the passive hemagglutination test. To the knowledge of the author this approach has not previously been attempted. Keratein was obtained by solubilizing hairs cut from a Jersey cow and a cross-bred dog in disodium sulfide and urea ( 1934). After precipitation with acetic acid the kerateines were redissolved in 0.1 N-NaOH and dialyzed for 48 hrs. against 0.1 M-NaHPO, pH 9.0. The nitrogen content was determined by micro Kjeldahl analysis and the keratein content calculated by multiplying the nitrogen figure with the factor 6.25. Antisera against the 2 kerateines were produced in adult rabbits. These were injected with approx. 5 mg keratein once a week for 3 weeks. A 5 mg booster dose was given 4 weeks after the third injection. The potency of the antisera was tested by immuno double diffusion in 1 % agar gel. Suitable sera were used for the passive hemagglutination test ( 1954). Goat erythrocytes were coated with the 2 respective kerateines using approx. 0.1 mg keratein per ml of a 2.5 % erythrocyte suspension. After inactivation at 56°C for 30 min. and absorption with 2 volumes of packed goat erythrocytes the antisera were absorbed 3 times with equal volumes of the heterologous keratein containing approx. 0.5 mg protein per ml. Serial 2-fold dilutions of the respective antisera were prepared in 1 % normal rabbit serum in 0.85 % saline. The keratein coated erythrocytes were then suspended in the absorbed and diluted homologous and heterologous antisera. The tests were read after incubation at 20°C for 3 to 4 hrs. From the results listed in Table 1 it may be seen that the hemagglutination titers of the homologous systems are more than 100-fold above their heterologous counterparts.