Preparation ofEntamoeba histolyticaantigens without enzymatic inhibitors

Author:

FLORES M. S.,TAMEZ-TREVIÑO E.,CASTAÑEDA F.,TIJERINA-MENCHACA R.,GALAN-WONG L.,RANGEL R.

Abstract

The goal of this work is to report a novel assay that preserves antigenicity of extracts with high protease content without using enzymatic inhibitors. A great reduction of proteolytic activity in the insoluble chloroform/methanol and heated amoebic fraction (IC[ratio ]MC) was obtained by this method, even in the presence of sodium dodecyl sulphate and 2-mercaptoethanol. The substrates azo-casein and the hide powder azure were used to determine the reduction of proteolytic activity of IC[ratio ]MC compared with the activity of crude extract and crude extract with iodoacetamide. The IC[ratio ]MC SDS-PAGE pattern shows a higher quantity of bands than extract with the inhibitor iodoacetamide or than crude extract. In addition, anti-Entamoeba histolyticaantibodies from amoebic liver abscess patients recognized a richer antigenic Western blot pattern in the IC[ratio ]MC fraction than in crude extract alone or with inhibitor. The described method has proved to be suitable to preserve amoebic antigens for its use in diagnostic tests and it can be used for immunological response studies againstE. histolyticaantigens. Furthermore we propose that this method to obtain the IC[ratio ]MC fraction can be applied for the study of other microorganisms or cells with high enzymatic content.

Publisher

Cambridge University Press (CUP)

Subject

Infectious Diseases,Animal Science and Zoology,Parasitology

Reference20 articles.

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4. A single step duplex PCR to distinguishEntamoeba histolyticafromEntamoeba dispar

5. FLORES-CASTAÑEDA, M. S. (1999).Procedure to preserve antigens of Entamoeba histolytica without enzymatic inhibitors and their use in immunological methods. United States Patent 5 861 263.

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