Abstract
We describe a high-throughput, quantitative technology for fast identification of all different clones present in selectively enriched phage surface-displayed cDNA libraries. The strategy is based on a combination of phage display and high-density arrays. To demonstrate the utility of the method cDNAs of Aspergillus fumigatus cloned into phagemid pJuFo were expressed on the tip of filamentous M13 phage and affinity-selected on solid phase-immobilized serum IgE from allergic patients. Enriched phagemid libraries were amplified in bacteria, plated and arrayed into 384-well microtitre plates by robotic colony picking. cDNA inserts were amplified by high-throughput PCR and gridded onto high-density filter membranes. Filters were iteratively probed with randomly-sequenced inserts until all clones were identified. Eighty-one different sequences encoding IgE-binding proteins likely to cover a large part of the allergen repertoire of the mould were found. This approach represents a widely applicable method for rapid high-throughput identification of all individual cDNAs present in selectively enriched libraries.
Original language | English (US) |
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Pages (from-to) | 147-154 |
Number of pages | 8 |
Journal | Combinatorial Chemistry and High Throughput Screening |
Volume | 6 |
Issue number | 2 |
DOIs | |
State | Published - Mar 2003 |
Externally published | Yes |
Keywords
- Allergens
- High-density arrays
- Phage display
- Robotics
- cDNA
ASJC Scopus subject areas
- Drug Discovery
- Computer Science Applications
- Organic Chemistry