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Cellular responses to Plasmodium falciparum erythrocyte membrane protein-1: use of relatively conserved synthetic peptide pools to determine CD4 T cell responses in malaria-exposed individuals in Benin,West Africa
Authors:Latifu?A?Sanni,Catherine?EM?Allsopp,Lieke?Reubsaet,Ambaliou?Sanni,Chris?Newbold,Virander?S?Chauhan,Jean?Langhorne  author-information"  >  author-information__contact u-icon-before"  >  mailto:jlangho@nimr.mrc.ac.uk"   title="  jlangho@nimr.mrc.ac.uk"   itemprop="  email"   data-track="  click"   data-track-action="  Email author"   data-track-label="  "  >Email author
Affiliation:(1) Division of Parasitology, National Institute for Medical Research, The Ridgeway, NW7 1AA Mill Hill, London, UK;(2) Molecular Parasitology Group, Institute of Molecular Medicine, John Radcliffe Hospital, OX3 9DS Oxford, UK;(3) Laboratory of Biochemistry and Molecular Biology, National University of Benin, Cotonou, Benin;(4) International Centre for Engineering and Biotechnology, Aruna Asaf Ali Marg, 110067 New Delhi, India
Abstract:

Background

Plasmodium falciparum erythrocyte membrane protein-1, a variant antigen of the malaria parasite, is potentially a target for the immune response. It would be important to determine whether there are CD4 T cells that recognise conserved regions. However, within the relatively conserved region, there is variation. It is not possible to test T cell responses from small field samples with all possible peptides.

Methods

We have aligned sequences that are relatively conserved between several PfEMP1 molecules, and chosen a representative sequence similar to most of the PfEMP1 variants. Using these peptides as pools representing CIDRα, CIDRβ and DBLβ-δ domains, DBLα domain, and EXON 2 domain of PfEMP1, we measured the CD4 T cell responses of malaria-exposed donors from Benin, West Africa by a FACS based assay.

Results

All the three peptide pools elicited a CD4 T cell response in a proportion of malaria-exposed and non-exposed donors. CD4 T cell proliferation occurs at a relatively higher magnitude to peptide pools from the DBLα and EXON 2 in the malaria-exposed donors living in Benin than in the UK malaria-unexposed donors.

Conclusions

These findings suggest that an immunological recall response to conserved peptides of a variant antigen can be measured. Further testing of individual peptides in a positive pool will allow us to determine those conserved sequences recognised by many individuals. These types of assays may provide information on conserved peptides of PfEMP1 which could be useful for stimulating T cells to provide help to P. falciparum specific B cells.
Keywords:
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