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本文引用的文献

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Dengue virus-specific human CD4+ T-lymphocyte responses in a recipient of an experimental live-attenuated dengue virus type 1 vaccine: bulk culture proliferation, clonal analysis, and precursor frequency determination.一名实验性1型登革热病毒减毒活疫苗接种者体内的登革热病毒特异性人类CD4+ T淋巴细胞反应:大量培养增殖、克隆分析及前体频率测定
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Immunization of monkeys with baculovirus-dengue type-4 recombinants containing envelope and nonstructural proteins: evidence of priming and partial protection.用含有包膜蛋白和非结构蛋白的杆状病毒-登革4型重组体对猴子进行免疫接种:启动和部分保护的证据。
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Dengue virus-specific, human CD4+ cytotoxic T lymphocytes generated in short-term culture.在短期培养中产生的登革病毒特异性人类CD4 + 细胞毒性T淋巴细胞。
Viral Immunol. 1993 Summer;6(2):143-51. doi: 10.1089/vim.1993.6.143.
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Profound atrophy of the bone marrow reflecting major histocompatibility complex class II-restricted destruction of stem cells by CD4+ cells.骨髓的严重萎缩反映了CD4+细胞对干细胞的主要组织相容性复合体II类限制的破坏。
J Exp Med. 1994 Jul 1;180(1):307-17. doi: 10.1084/jem.180.1.307.
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Recognition of envelope protein by dengue virus serotype-specific human CD4+ CD8- cytotoxic T-cell clones.登革病毒血清型特异性人CD4+ CD8-细胞毒性T细胞克隆对包膜蛋白的识别。
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Overlapping epitopes encompassing a point mutation (12 Gly-->Arg) in p21 ras can be recognized by HLA-DR, -DP and -DQ restricted T cells.包含p21 ras中一个点突变(12甘氨酸→精氨酸)的重叠表位可被HLA - DR、- DP和 - DQ限制性T细胞识别。
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CD4+ human immunodeficiency virus type 1 (HIV-1) envelope-specific cytotoxic T lymphocytes derived from the peripheral blood cells of an HIV-1-infected individual.从一名感染了人类免疫缺陷病毒1型(HIV-1)个体的外周血细胞中分离得到的CD4 + HIV-1包膜特异性细胞毒性T淋巴细胞。
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Dengue virus protein recognition by virus-specific murine CD8+ cytotoxic T lymphocytes.病毒特异性小鼠CD8 + 细胞毒性T淋巴细胞对登革病毒蛋白的识别
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Dengue virus-specific, HLA-B35-restricted, human CD8+ cytotoxic T lymphocyte (CTL) clones. Recognition of NS3 amino acids 500 to 508 by CTL clones of two different serotype specificities.登革病毒特异性、HLA - B35限制的人类CD8 + 细胞毒性T淋巴细胞(CTL)克隆。两种不同血清型特异性的CTL克隆对NS3氨基酸500至508的识别。
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登革4型病毒衣壳蛋白上两个表位的鉴定,这两个表位可被血清型特异性及一组血清型交叉反应性人类CD4+细胞毒性T淋巴细胞克隆识别。

Identification of two epitopes on the dengue 4 virus capsid protein recognized by a serotype-specific and a panel of serotype-cross-reactive human CD4+ cytotoxic T-lymphocyte clones.

作者信息

Gagnon S J, Zeng W, Kurane I, Ennis F A

机构信息

Department of Medicine, University of Massachusetts Medical Center, Worcester 01655, USA.

出版信息

J Virol. 1996 Jan;70(1):141-7. doi: 10.1128/JVI.70.1.141-147.1996.

DOI:10.1128/JVI.70.1.141-147.1996
PMID:8523518
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC189798/
Abstract

We analyzed the CD4+ T-lymphocyte response of a donor who had received an experimental live-attenuated dengue 4 virus (D4V) vaccine. Bulk culture proliferative responses of peripheral blood mononuclear cells (PBMC) to noninfectious dengue virus (DV) antigens showed the highest proliferation to D4V antigen, with lesser, cross-reactive proliferation to D2V antigen. We established CD4+ cytotoxic T-lymphocyte clones (CTL) by stimulation with D4 antigen. Using recombinant baculovirus antigens, we identified seven CTL clones that recognized D4V capsid protein. Six of these CTL clones were cross-reactive between D2 and D4, and one clone was specific for D4. Using synthetic peptides, we found that the D4V-specific CTL clone recognized an epitope between amino acids (aa) 47 and 55 of the capsid protein, while the cross-reactive CTL clones each recognized epitopes in a separate location, between aa 83 and 92, which is conserved between D2V and D4V. This region of the capsid protein induced a variety of CD4+ T-cell responses, as indicated by the fact that six clones which recognized a peptide spanning this region showed heterogeneity in their recognition of truncations of this same peptide. The bulk culture response of the donor's PBMC to the epitope peptide spanning aa 84 to 92 was also examined. Peptides containing this epitope induced proliferation of the donor's PBMC in bulk culture, but peptides not containing the entire epitope did not induce proliferation. Also, PBMC stimulated in bulk culture with noninfectious D4V antigen lysed autologous target cells pulsed with peptides containing aa 84 to 92. These results indicate that this donor exhibits memory CD4+ T-cell responses directed against the DV capsid protein and suggest that the response to the capsid protein is dominant not only in vitro at the clonal level but in bulk culture responses as well. Since previous studies have indicated that the CTL responses to DV infection seem to be directed mainly against the envelope (E) and NS3 proteins, these results are the first to indicate that the DV capsid protein is also a target of the antiviral T-cell response.

摘要

我们分析了一名接种过实验性减毒活登革4型病毒(D4V)疫苗的供体的CD4+ T淋巴细胞反应。外周血单核细胞(PBMC)对非感染性登革病毒(DV)抗原的大量培养增殖反应显示,对D4V抗原的增殖反应最高,对D2V抗原的交叉反应性增殖较低。我们通过用D4抗原刺激建立了CD4+细胞毒性T淋巴细胞克隆(CTL)。使用重组杆状病毒抗原,我们鉴定出七个识别D4V衣壳蛋白的CTL克隆。其中六个CTL克隆在D2和D4之间具有交叉反应性,一个克隆对D4具有特异性。使用合成肽,我们发现D4V特异性CTL克隆识别衣壳蛋白氨基酸(aa)47至55之间的一个表位,而交叉反应性CTL克隆各自在一个单独的位置识别表位,在aa 83至92之间,这在D2V和D4V之间是保守的。衣壳蛋白的这一区域诱导了多种CD4+ T细胞反应,这一事实表明,六个识别跨越该区域的肽的克隆在对该相同肽的截短的识别中表现出异质性。还检测了供体PBMC对跨越aa 84至92的表位肽的大量培养反应。含有该表位的肽在大量培养中诱导供体PBMC增殖,但不包含整个表位的肽不诱导增殖。此外,用非感染性D4V抗原在大量培养中刺激的PBMC裂解了用含有aa 84至92的肽脉冲处理的自体靶细胞。这些结果表明,该供体表现出针对DV衣壳蛋白的记忆性CD4+ T细胞反应,并表明对衣壳蛋白的反应不仅在克隆水平的体外占主导地位,在大量培养反应中也是如此。由于先前的研究表明,对DV感染的CTL反应似乎主要针对包膜(E)和NS3蛋白,这些结果首次表明DV衣壳蛋白也是抗病毒T细胞反应的靶标。