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恰菲埃立克体的可变长度PCR靶蛋白在富含酸性丝氨酸的串联重复序列中含有主要的种特异性抗体表位。

A variable-length PCR target protein of Ehrlichia chaffeensis contains major species-specific antibody epitopes in acidic serine-rich tandem repeats.

作者信息

Luo Tian, Zhang Xiaofeng, Wakeel Abdul, Popov Vsevolod L, McBride Jere W

机构信息

Department of Pathology, University of Texas Medical Branch, Galveston, TX 77555-0609, USA.

出版信息

Infect Immun. 2008 Apr;76(4):1572-80. doi: 10.1128/IAI.01466-07. Epub 2008 Jan 22.

Abstract

Ehrlichia chaffeensis and E. canis have a small subset of tandem repeat (TR)-containing proteins that elicit strong host immune responses and are associated with host-pathogen interactions. In a previous study, we molecularly characterized a highly conserved 19-kDa major immunoreactive protein (gp19) of E. canis and identified the corresponding TR-containing ortholog variable-length PCR target (VLPT) protein in E. chaffeensis. In this study, the native 32-kDa VLPT protein was identified and the immunodeterminants defined in order to further understand the molecular basis of the host immune response to E. chaffeensis. Synthetic and/or recombinant polypeptides corresponding to various regions of VLPT were used to localize major antibody epitopes to the TR-containing region. Major antibody epitopes were identified in three nonidentical repeats (R2, R3, and R4), which reacted strongly with antibodies in sera from an E. chaffeensis-infected dog and human monocytotropic ehrlichiosis patients. VLPT-R3 and VLPT-R2 reacted most strongly with antibody, and the epitope was further localized to a nearly identical proximal 17-amino-acid region common between these repeats that was species specific. The epitope in R4 was distinct from that of R2 and R3 and was found to have conformational dependence. VLPT was detected in supernatants from infected cells, indicating that the protein was secreted. VLPT was localized on both reticulate and dense-core cells, and it was found extracellularly in the morula fibrillar matrix and associated with the morula membrane.

摘要

查菲埃立克体和犬埃立克体有一小部分含串联重复序列(TR)的蛋白质,这些蛋白质能引发强烈的宿主免疫反应,并与宿主 - 病原体相互作用相关。在之前的一项研究中,我们对犬埃立克体一种高度保守的19 kDa主要免疫反应蛋白(gp19)进行了分子特征分析,并在查菲埃立克体中鉴定出了相应的含TR的直系同源可变长度PCR靶标(VLPT)蛋白。在本研究中,我们鉴定了天然的32 kDa VLPT蛋白并确定了免疫决定簇,以便进一步了解宿主对查菲埃立克体免疫反应的分子基础。与VLPT不同区域相对应的合成和/或重组多肽被用于将主要抗体表位定位到含TR的区域。在三个不同的重复序列(R2、R3和R4)中鉴定出了主要抗体表位,这些表位与来自感染查菲埃立克体的犬和人类单核细胞埃立克体病患者血清中的抗体强烈反应。VLPT - R3和VLPT - R2与抗体反应最强,表位进一步定位到这些重复序列之间一个几乎相同的近端17氨基酸区域,该区域具有种属特异性。R4中的表位与R2和R3的不同,且具有构象依赖性。在感染细胞的上清液中检测到了VLPT,表明该蛋白被分泌。VLPT定位于网状细胞和致密核心细胞上,并且在桑葚体纤维状基质中细胞外被发现,并与桑葚体膜相关。

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