Butyrylcholinesterase in Human Brain and Acetylcholinesterase in Human Plasma: Trace Enzymes Measured by Two-Site Immunoassay

A novel and sensitive noncompetitive enzyme immunoassay (hetero-two-site enzyme immunoassay) for a-human atrial natriuretic peptide (a-hANP) in plasma, which uses only one monoclonal IgG for the ring structure of a-hANP, is described. Plasma was filtered through polysaccharide membrane to separate p

a-Human atrial natriuretic polypeptide (a-was 30-90 fg (10-30 attomo1es)ltube and hANP) in plasma was directly measured 0.6-2.3 ng (0.2-0.75 pmol)/L using 0.04without extraction by sensitive sandwich 0.05 ml of plasma. The lower detection enzyme immunoassay. Polystyrene balls limit was obtained usin

We reassessed the enzyme immunoassay (EIA) system for hEGF previously developed by our laboratory ( C h ChimActa 15651-60, 1985), since it appeared that the reported EIA system detected not only hEGF but also pS2 protein owing to minor contamination by pS2 protein in the hEGF sample used for immuniz

## Abstract A simple, fast, and reliable immunoassay has been developed to detect and measure Alzheimer's disease‐associated proteins (ADAPs) in human brain tissue. This assay, called ALZ‐EIA (brain), was developed for Abbott's quantum system, in which 1/4‐in. beads are used as solid phase. The bea

A noncompetitive enzyme immunoassay (hetero-two-site enzyme immunoassay) for p-melanocyte-stimulating hormone (@-MSH) was developed. p-MSH (1-12) was biotinylated, trapped onto an anti-e-MSH (1-12) IgG-coated polystyrene bead, eluted at pH 1 after washing to eliminate other biotinylated substances,

A highly sensitive and specific two-site enzyme immunoassay for parathyroid hormone (1-34) (PTH(1-34)) and its usability for the pharmacokinetic study are described. Plasma samples were incubated simultaneously with 2,4-dinitrophenylated anti-PTH(1-34) IgG and anti-PTH(1-34) Fab´β-D-galactosidase co