The purpose of this work is to provide a simple, accurate quantitative assay for Lymphocyte Stimulating Hormone (LSH) by using the routine clinical microzone electrophoresis method. This new method has two keystone: one is using Dr. Robey's pure extraction of LSH crystal as an identified reference, the other is using chymotrypsinogen standard curve to determine the LSH quantitative concentration of separation point on membrane. we obtain the same Rf value from the extraction of animal thymus gland and that of human serum as Dr. Robey's product. This assay provides a simple rapid precise and high sensitive routine method for studying LSH protein.