cDNA cloning of galectins from third stage larvae of the parasitic nematode Teladorsagia circumcincta

A monoclonal antibody raised to a Teladorsagia circumcincta 31–33 kDa doublet antigen was used to immunoscreen a T. circumcincta cDNA expression library. Sheep antibodies eluted from the proteins expressed by two clones immunopositive with the monoclonal antibody specifically recognised the doublet...

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Bibliographic Details
Published in:Molecular and biochemical parasitology 1997-06, Vol.86 (2), p.143-153
Main Authors: Newton, Susan E, Monti, Jennifer R, Greenhalgh, Christopher J, Ashman, Keith, Meeusen, Els N.T
Format: Article
Language:English
Subjects:
Amino Acid Sequence
amino acid sequences
animal parasitic nematodes
Animals
antigens
Antigens, Helminth - analysis
Antigens, Helminth - immunology
Base Sequence
beta-galactoside binding lectin like proteins
binding proteins
Carrier Proteins - chemistry
Carrier Proteins - genetics
Carrier Proteins - isolation & purification
cloning
Cloning, Molecular
complementary DNA
DNA, Complementary - genetics
DNA, Complementary - immunology
Galactosides - chemistry
Galactosides - genetics
Galactosides - isolation & purification
Galectin
Galectins
genbank/u67147
genbank/u67148
Hemagglutinins - chemistry
Hemagglutinins - genetics
Hemagglutinins - isolation & purification
Larva - chemistry
Larva - genetics
Larva - growth & development
lectins
Lectins - chemistry
Lectins - genetics
Lectins - isolation & purification
messenger RNA
Molecular Sequence Data
Nematode
nematode larvae
nucleotide sequences
Onchocerca volvulus
Ostertagia
purification
Sequence Analysis, DNA
Spliced leader
spliced leader rna
Teladorsagia circumcincta
Trichostrongyloidea - chemistry
Trichostrongyloidea - genetics
Trichostrongyloidea - immunology
β-galactoside-binding
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Description
Summary:A monoclonal antibody raised to a Teladorsagia circumcincta 31–33 kDa doublet antigen was used to immunoscreen a T. circumcincta cDNA expression library. Sheep antibodies eluted from the proteins expressed by two clones immunopositive with the monoclonal antibody specifically recognised the doublet antigen on Western blots of third stage larval extract, confirming that these clones coded for the antigen. Database searches revealed high levels of similarity with β-galactoside-binding lectin-like proteins (GalBPs or galectins) from Caenorhabditis elegans and Onchocerca volvulus. By analogy with these sequences, both T. circumcincta cDNA clones contain the full-length protein coding region. The native doublet proteins could be preferentially extracted from homogenates of third stage larvae with lactose and could be affinity purified on an asialofetuin column, confirming the identity of these bands as galectins. Reverse transcriptase-polymerase chain reaction amplification using a primer based on the C. elegans Spliced Leader SL1 sequence showed that the corresponding T. circumcincta mRNAs are also trans-spliced at their 5′ ends. While there are considerable nucleotide differences between the two clones, the majority are located in the non-coding regions. Within the coding region there are 87 nucleotide differences but only three of these result in amino acid substitutions.
ISSN:0166-6851
1872-9428
DOI:10.1016/S0166-6851(97)02834-X