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Novel phage display-based subtractive screening to identify vaccine candidates of Brugia malayi.


ABSTRACT: This study describes a novel phage display method based on an iterative subtraction strategy to identify candidate vaccine antigens of Brugia malayi. A cDNA library of the infective larval stage of B. malayi expressed on the surface of T7 phage was sequentially screened with sera samples from human subjects showing different manifestations of the disease. Antigens that selectively and specifically bind to immune sera were then enriched using a multi-step panning procedure. This strategy identified five antigens, four of which were previously reported (ALT-2, TPX-2, VAH and COX-2) and the other one was a novel cuticular collagen (Col-4). Sera from immune individuals specifically recognized all the five antigens. However, ALT-2 appeared to be the most predominantly recognized antigen by the immune sera. Therefore, it was decided to evaluate the vaccine potential of recombinant ALT-2 (rALT-2) in a mouse and jird model. The results presented show that immunization with rALT-2 conferred over 73% protection against a challenge infection in the jird model and over 64% protection in the mouse model. The present study suggests that phage display-based cDNA screening may be a powerful tool to identify candidate vaccine antigens of infectious agents.

SUBMITTER: Gnanasekar M 

PROVIDER: S-EPMC470678 | biostudies-literature | 2004 Aug

REPOSITORIES: biostudies-literature

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Novel phage display-based subtractive screening to identify vaccine candidates of Brugia malayi.

Gnanasekar Munirathinam M   Rao Kakaturu V N KV   He Yi-Xun YX   Mishra Pankaj K PK   Nutman Thomas B TB   Kaliraj Perumal P   Ramaswamy Kalyanasundaram K  

Infection and immunity 20040801 8


This study describes a novel phage display method based on an iterative subtraction strategy to identify candidate vaccine antigens of Brugia malayi. A cDNA library of the infective larval stage of B. malayi expressed on the surface of T7 phage was sequentially screened with sera samples from human subjects showing different manifestations of the disease. Antigens that selectively and specifically bind to immune sera were then enriched using a multi-step panning procedure. This strategy identifi  ...[more]

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