Author: Trirawatanapong, Thaweesak; Chandran, Bala; Putnak, Robert; Padmanabhan, R.
Title: Mapping of a region of dengue virus type-2 glycoprotein required for binding by a neutralizing monoclonal antibody Cord-id: r0f257jv Document date: 1992_7_15
ID: r0f257jv
Snippet: Envelope glycoprotein E of flaviviruses is exposed at the surface of the virion, and is responsible for eliciting a neutralizing antibody (Ab) response, as well as protective immunity in the host. In this report, we describe a method for the fine mapping of a linear sequence of the E protein of dengue virus type-2 (DEN-2), recognized by a type-specific and neutralizing monoclonal Ab (mAb), 3H5. First, an Escherichia coli expression vector containing a heat-inducible λ pl promoter was used to sy
Document: Envelope glycoprotein E of flaviviruses is exposed at the surface of the virion, and is responsible for eliciting a neutralizing antibody (Ab) response, as well as protective immunity in the host. In this report, we describe a method for the fine mapping of a linear sequence of the E protein of dengue virus type-2 (DEN-2), recognized by a type-specific and neutralizing monoclonal Ab (mAb), 3H5. First, an Escherichia coli expression vector containing a heat-inducible λ pl promoter was used to synthesize several truncated, and near-full length E polypeptides. Reactivities of these polypeptides with polyclonal mouse hyperimmune sera, as well as the 3H5 mAb revealed the location of the 3H5-binding site to be within a region of 166 amino acids (aa) between aa 255 and 422. For fine mapping, a series of targeted deletions were made inframe within this region using the polymerase chain reaction (PCR). The hydrophilicity pattern of this region was used as a guide to systematically delete the regions encoding the various groups of surface aa residues within the context of a near-full-length E polypeptide by using PCR. The 3H5-binding site was thus precisely mapped to a region encoding 12 aa (between aa 386 and 397). A synthetic peptide containing this sequence was able to bind to the 3H5 mAb specifically, as shown by enzyme-linked immunosorbent assay. In addition, we show that rabbit Abs raised against the synthetic peptide of 12 aa were able to bind to the authentic E protein, and to neutralize DEN-2 virus in a plaque reduction assay.
Search related documents:
Co phrase search for related documents- aa deletion and aa sequence: 1, 2, 3, 4, 5
- aa peptide and aa residue: 1
- aa peptide and aa sequence: 1, 2, 3, 4, 5, 6, 7, 8, 9
- aa peptide and aa sequence strain: 1
- aa peptide and aa synthetic peptide: 1, 2, 3, 4
- aa residue and aa sequence: 1
Co phrase search for related documents, hyperlinks ordered by date