beta-Amyloid peptide (beta A) is a major fibrillar component of neuritic plaques in Alzheimer's disease (AD) brains and is related to the pathogenesis of the disease. In this study, using electron microscopy, we describe herein the results concerning the efficacy of compounds that can dissolve preformed beta A fibrils in vitro. For such a purpose, two hydrosoluble and biocompatible polymers such as polyethylene glycol and poly-L-lysine were used. The poly-L-lysine appears as a potent dissolver of preformed beta A fibrils in vitro. Its efficiency is instantaneous. Poly-L-lysine can be used as a universal dissolver of all types of oligomeric beta-sheet conformation, precursor of the fibrils. This finding provides the basis for future investigation of the therapeutic potential of poly-L-lysine in terms of preventing and/or retarding amyloidogenesis in AD and other types of amyloid-related disorders.
Repetitive determinations using injection of the sample containing the sought-for species (substrate, S) into a continuously circulated reagent mixture (enzyme + buffer), is described. The glucose oxidase-catalyzed oxidation of ßo-glucose has been chosen to illustrate methods of substrate determination based on:
FFSCYT ME GQEYP APL Two XI-ets-J gene transcripts of 4.4 kb (major species) and 7.5 kb (minor species) were detected in the poly(A)+ fraction from the early stages of the oogenesis to the late stages of embryogenesis. They appear to decline regularly during embryogenesis. They were not at all detected in several adult organs, except in spleen where the larger transcript (7.5 kb) is the major one.
By exploiting the kinetics of NADH consumption in the enzyme system creatinine amidohydrolase + creatine kinase + pyruvate kinase + lactate dehydrogenase, one can determine creatinine in serum in the range of 1 to 90 mg/L. By using the conditions defined here, this determination can be made with a single measurement of the rate of disappearance of NADH. The analytical rate measurement is made at a fixed time (2 min) after the sample is introduced into the enzyme solution. For this fixed time, the interferences of creatine and pyruvate are eliminated. Results so obtained for creatinine in human blood serum samples correlated well (r = 0.98) with those obtained by the classical Jaffé-reaction method. Run-to-run reproducibility (CV) was 3%, and the limit of detection was 1 mg/L.
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