LSA was purified from the human liver, and the antibody to the human LSA only reacted with the live extract using the immuno-dotblotting technique. Depending on the immunohistochemical study, the LSA was found to be located within the cytoplasm of hepatocytes. A sensitive and specific sandwich enzyme immunoassay was then developed for the measurement of LSA. The detection limit of human LSA was 1 fmol/tube (52 pg/tube) and this assay was not affected by hemolysis. The LSA levels in serum and blood from health individuals were distributed within a range below the detection limit. The LSA levels in the blood from cadavers whose livers had been damaged were markedly elevated (10 to 140-fold) compared to the normal levels found in other cadavers. No cross-reaction was observed with the liver extracts from several species, including mice, rats, guinea pigs, and rabbits. The results suggest that the measurement of LSA levels in blood will become a useful marker for the detection of liver injury. Figures, tables, photographs, and 14 references (Author abstract modified)