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丝状病毒糖蛋白保守 B 细胞表位的鉴定和有效性:用于埃博拉和可能的马尔堡病毒病的快速诊断检测。

Identity and validity of conserved B cell epitopes of filovirus glycoprotein: towards rapid diagnostic testing for Ebola and possibly Marburg virus disease.

机构信息

Department of Immunology and Molecular Biology, School of Biomedical Sciences, College of Health Sciences, Makerere University, P o Box 7072, Kampala, Uganda.

Arbovirology and Filovirology Laboratories/Centers for Disease Control-CDC, Uganda Virus Research Institute (UVRI), Entebbe, Uganda.

出版信息

BMC Infect Dis. 2018 Oct 3;18(1):498. doi: 10.1186/s12879-018-3409-x.

Abstract

BACKGROUND

Ebolavirus and Marburgvirus are genera of the virus family Filoviridae. Filoviruses cause rare but fatal viral hemorrhagic fevers (VHFs) in remote villages of equatorial Africa with potential for regional and international spread. Point-of-care (POC) rapid diagnostic tests (RDTs) are critical for early epidemic detection, reponse and control. There are 2 RDTs for Zaire ebolavirus (EBOV), but not other Ebolavirus spp. or Marburg marburgvirus (MARV). We validate 3 conserved B cell epitopes of filovirus glycoprotein (GP) using ebola virus diseases (EVD) survivor samples, towards devising pan-filovirus RDTs.

METHODS

In-silico Immuno-informatics:- (a) multiple and basic local alignments of amino-acid sequences of filovirus (4 Ebolavirus spp. & MARV) Gp1, 2 and epitope prediction and conservation analyses within context of ClusterW, BLAST-P and the immune epitope database analysis resource (IEDB-AR); alongside (b) in-vitro enzyme immuno-assays (EIAs) for SUDV Gp1, 2 antigen and host-specific antibodies (IgM and IgG) among 94 gamma irradiated EVD survivor serum and 9 negative controls.

RESULTS

Linear B cell epitopes were present across the entire length of all Gp1, 2, most lying in the region between amino acids positioned 350 and 500. Three seperate epitopes 97/80_GAFFLYDRLAST, 39_YEAGEWAENCY and 500_CGLRQLANETTQALQLFLRATTELR (designated UG-Filo-Peptide- 1, 2 and 3 respectively) were conserved within all studied filovirus species Gp1, 2. Gp1, 2 host specific IgM levels were comparably low (av. ODs < 0.04 [95% CI: 0.02837 to 0.04033]) among the 9 negative controls and 57 survivor samples analyzed. Host specific IgG levels, on the other hand, were elevated (av. ODs > 1.7525 [95% CI: 0.3010 to 3.1352]) among the 92 survivor samples relative to the 9 negative controls (av. ODs < 0.2.321 [95% CI: -0.7596 to 0.5372]). Filovirus Gp1, 2 antigen was not detected [av. ODs < 0.20] within EVD survivor serum relative to recombinant protein positive controls [av. ODs = 0.50].

CONCLUSIONS

These conserved B cell epitopes of filovirus Gp1, 2 and their derivative antibodies are promising for research and development of RDTs for EVD, with potential for extension to detect MVD.

摘要

背景

埃博拉病毒和马尔堡病毒是丝状病毒科的病毒属。丝状病毒在赤道非洲偏远村庄引起罕见但致命的病毒性出血热(VHF),具有在区域和国际传播的潜力。即时检测(POC)快速诊断检测(RDT)对于早期的疫情检测、反应和控制至关重要。有两种针对扎伊尔埃博拉病毒(EBOV)的 RDT,但没有针对其他埃博拉病毒属或马尔堡马尔堡病毒(MARV)的 RDT。我们使用埃博拉病毒病(EVD)幸存者样本验证了丝状病毒糖蛋白(GP)的 3 个保守 B 细胞表位,以开发针对所有丝状病毒的 RDT。

方法

基于计算机的免疫信息学:(a)丝状病毒(4 种埃博拉病毒属和 MARV)GP1、2 的氨基酸序列的多重和基本局部比对,以及在 ClusterW、BLAST-P 和免疫表位数据库分析资源(IEDB-AR)中的表位预测和保守性分析;以及(b)针对 SUDV GP1、2 抗原和宿主特异性抗体(IgM 和 IgG)的体外酶免疫测定(EIA),对 94 名经伽马射线辐照的 EVD 幸存者血清和 9 名阴性对照进行检测。

结果

线性 B 细胞表位存在于所有 GP1、2 的全长,大多数位于氨基酸位置 350 至 500 之间。3 个独立的表位 97/80_GAFFLYDRLAST、39_YEAGEWAENCY 和 500_CGLRQLANETTQALQLFLRATTELR(分别指定为 UG-Filo-Peptide-1、2 和 3)在所有研究的丝状病毒物种的 GP1、2 中保守。GP1、2 宿主特异性 IgM 水平在 9 个阴性对照和 57 个分析幸存者样本中相对较低(平均 OD 值<0.04 [95%CI:0.02837 至 0.04033])。另一方面,宿主特异性 IgG 水平在 92 个幸存者样本中相对 9 个阴性对照(平均 OD 值<0.2.321 [95%CI:-0.7596 至 0.5372])升高。与重组蛋白阳性对照(平均 OD 值=0.50)相比,在 EVD 幸存者血清中未检测到丝状病毒 GP1、2 抗原(平均 OD 值<0.20)。

结论

这些丝状病毒 GP1、2 的保守 B 细胞表位及其衍生抗体有望用于开发针对 EVD 的 RDT 的研究和开发,并有潜力扩展到检测马尔堡病毒。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/196a/6171133/e980c89ff6a8/12879_2018_3409_Fig1_HTML.jpg

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