Analysis of T- and B-cell epitopes of capsid protein of rubella virus by using synthetic peptides

Ou, Dawei; Chong, Pele; Tripet, Brian; Gillam, Shirley

doi:10.1128/jvi.66.3.1674-1681.1992

Cited by 38 publications

(19 citation statements)

References 49 publications

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“…We have synthesized 49 synthetic peptides comprising approximately 95% of the amino acid sequences of the structural proteins El (23 peptides), E2 (15 peptides), and C (1 1 peptides) of RV strain M33 (Clarke et a/., 1987) and initiated a series of experiments to search for peptide-specific T cell responses in individuals naturally infected with RV. We have showed that C peptides such as C5 (residues 96-l 23), C6 (residues 119-152), C9 (residues 205-233) or Cl 1 (residues 255-280) can induce significant proliferation of T cells in short-term cultured T cell lines from some RV-seropositive donors (Ou et a/., 1992). The T cell clones used in this study were initially established from the T cell lines of two RV seropositive donors (Ou et a/., 1992).…”

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confidence: 99%

“…We have showed that C peptides such as C5 (residues 96-l 23), C6 (residues 119-152), C9 (residues 205-233) or Cl 1 (residues 255-280) can induce significant proliferation of T cells in short-term cultured T cell lines from some RV-seropositive donors (Ou et a/., 1992). The T cell clones used in this study were initially established from the T cell lines of two RV seropositive donors (Ou et a/., 1992). A total of 36 clones were isolated by the method a A total of 2 X 1 O4 T cells from each clone was tested for their proliferative response to each synthetrc peptide at a final concentration of 5 pg/ml in the presence of y-irradiated (3000 rad) autologous PBMC 5 X 1 O4 as APC.…”

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confidence: 99%

“…' Underlined numbers represent significant cell proliferation values of limiting dilution (Celis et al, 1988a,b) and their RV specificity was tested in proliferation assays (Ou et al, 1992). To further identify the capacity of these T cell clones to recognize the T cell epitopes of the structural proteins of RV, their responses to 49 synthetic peptides were tested in proliferation assays.…”

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confidence: 99%

“…On the other hand, C9, or Cl l-reactive T cell clones, are located at the B Cell lines used as targets were incubated with or without peptide C9 at 5 &ml overnight before addition of T cells. b Cytotoxicity was determined using the T cell clone Al 1 at an effectorkarget ratio of 5. peak region of the a-helix index within the C6, C9, or Cl 1 peptide sequences according to the profiles of a-helix, P-turn and hydrophilicity of the C protein of RV (Ou et a/., 1992). We have analyzed the T cell motif (second model) structures within C6, C9, and Cl 1 sequences (Ou et a/., 1992).…”

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confidence: 99%

“…b Cytotoxicity was determined using the T cell clone Al 1 at an effectorkarget ratio of 5. peak region of the a-helix index within the C6, C9, or Cl 1 peptide sequences according to the profiles of a-helix, P-turn and hydrophilicity of the C protein of RV (Ou et a/., 1992). We have analyzed the T cell motif (second model) structures within C6, C9, and Cl 1 sequences (Ou et a/., 1992). C6E is located in the region between two T cell motif structures.…”

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confidence: 99%

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Characterization of the specificity and genetic restriction of human CD4+ cytotoxic T cell clones reactive to capsid antigen of rubella virus

Chong²,

McVeish³

et al. 1992

Virology

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Using 11 overlapping synthetic peptides covering more than 95% of the amino acid sequence of capsid protein of rubella virus, 7 CD4+ T cell clones (R10, R11, R18, A2, A10, A11, and A12) isolated from 2 rubella seropositive donors reacted strongly to rubella capsid peptides C6 (residues 119-152), C9 (residues 205-233), or C11 (residues 255-280), respectively, in both proliferation and cytotoxicity assay. Truncated peptides C6E (residues 125-139), C9B (residues 205-216), and C11E (residues 260-272) were shown to be involved directly to the T cell determinants of C6, C9, and C11, respectively. Genetic restriction of these T cell clones was analyzed by using human cell lines with various HLA-DR phenotypes as targets and/or antigen-presenting cells in cytotoxicity assay and/or proliferation assays. The results indicated that the recognition of peptide C6 by T cell clones (R11 and R18) was associated with DRw9 molecule, while the HLA restriction element of the responses of other T cell clones (A2 and A11, A10, and A12) that reacted with peptide C9 or C11 was DR4 molecule. However, there may be a cross-recognition by the T cell clone (A12) between DR1 and DR4 subtypes.

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confidence: 99%

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confidence: 99%

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confidence: 99%

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confidence: 99%

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confidence: 99%

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Characterization of the specificity and genetic restriction of human CD4+ cytotoxic T cell clones reactive to capsid antigen of rubella virus

Chong²,

McVeish³

et al. 1992

Virology

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Rubella

Best

Cooray

Banatvala

2010

Topley &Amp; Wilson's Microbiology and Microbial Infections

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Viral hemagglutinin augments peptide‐specific cytotoxic T cell responses

et al. 1993

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In attempt to increase the induction of peptide-specific cytolytic T cells (CTL) we investigated the effect of the Newcastle disease virus (NDV) hemagglutinin-neuraminidase (HN) gene product on the activation of peptide-specific CTL. Spleen cells of CH3 mice immunized against the influenza nucleoprotein peptide 50-63 (NP 50-63) were restimulated in vitro (i) with peptide-pulsed syngeneic fibroblast cells (Ltk-) as antigen-presenting cells, which were in addition (ii) infected with NDV or (iii) stably transfected with the HN cDNA of NDV. A greater than sixfold increase in peptide-specific CTL responses was observed in cultures restimulated with peptide-pulsed Ltk- cells which co-expressed viral hemagglutinin due to either infection or transfection. A similar augmentation was seen in CTL responses against other types of antigen (major histocompatibility complex alloantigens, minor histocompatibility antigens or tumor antigens) when suboptimal cultures were stimulated with the respective antigen-presenting cells modified by NDV infection. These findings suggest that NDV or viral HN expressed on antigen-presenting cells or tumor cells can exert a T cell co-stimulatory function.

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Analysis of T- and B-cell epitopes of capsid protein of rubella virus by using synthetic peptides

Cited by 38 publications

References 49 publications

Characterization of the specificity and genetic restriction of human CD4+ cytotoxic T cell clones reactive to capsid antigen of rubella virus

Characterization of the specificity and genetic restriction of human CD4+ cytotoxic T cell clones reactive to capsid antigen of rubella virus

Rubella

Viral hemagglutinin augments peptide‐specific cytotoxic T cell responses

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