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6.6 - Differentiation between parasite species by agglutination and detection of parasite surface carbohydrates, using non-conjugated lectins

Published online by Cambridge University Press:  05 June 2012

G. A. Ingram
Affiliation:
Department of Biological Sciences
D. W. Halton
Affiliation:
Queen's University Belfast
J. M. Behnke
Affiliation:
University of Nottingham
I. Marshall
Affiliation:
Liverpool School of Tropical Medicine
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Summary

Aims and objectives

Using commercial lectins, these two exercises are designed to:

  1. Distinguish between different species of parasites and two strains of the same parasite species.

  2. Determine the type of carbohydrate present on the parasite surface membrane.

Introduction

Lectins (often referred to as agglutinins) are proteins or glycoproteins that bind specifically to carbohydrates, usually present as glycoconjugates, on cell or tissue surfaces or in cell tissue fluids (Sharon & Lis, 1989; Jacobson, 1994). Lectin reactivity is generally designated according to the monosaccharides or oligosaccharides that cause inhibition of lectin-mediated agglutination of cells or adherence to cell membranes.

Lectins have been widely used in parasitology to detect and determine the types of saccharide moieties on the surface of trypanosomatids, e.g. Crithidia (Petry et al., 1987), Leishmania (Schottelius & Aisen, 1994) and Trypanosoma species (Maraghi et al., 1989), to demonstrate differences between parasite growth and stationary phases (Jacobson & Schnur, 1990) and to distinguish between the different stages of the trypanosomatid life cycle (Rudin et al., 1989). In addition, lectins have been employed to differentiate between parasite species (Schottelius & Aisen, 1994) and in the identification of various strains (Schnur & Jacobson, 1989) and stocks (Schottelius, 1987) of these flagellates. The following methods are applied to kinetoplastid flagellates but can be adapted to study other unicellular parasites.

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Publisher: Cambridge University Press
Print publication year: 2001

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