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从感染巨噬细胞的主要组织相容性复合体II类分子中分离的一种肽指导的杜氏利什曼原虫基因的克隆与表达。

Cloning and expression of a Leishmania donovani gene instructed by a peptide isolated from major histocompatibility complex class II molecules of infected macrophages.

作者信息

Campos-Neto A, Soong L, Cordova J L, Sant'Angelo D, Skeiky Y A, Ruddle N H, Reed S G, Janeway C, McMahon-Pratt D

机构信息

Department of Immunology, University of São Paulo Medical School at Ribeirão Preto, Brazil.

出版信息

J Exp Med. 1995 Nov 1;182(5):1423-33. doi: 10.1084/jem.182.5.1423.

Abstract

The studies reported here describe the isolation of peptides from MHC class II molecules of murine macrophages infected with Leishmania donovani, and the use of the derived peptide sequences to rescue the pathogen peptide donor protein. The isolation of the peptides was carried out by comparing the RP HPLC profile of peptides extracted from infected macrophages with the peptides extracted from noninfected cells. Several distinct HPLC peaks unique to infected macrophages were sequenced. One of the peptides that was not homologous to any known protein was used to instruct the designing of an oligonucleotide sense primer that was used in combination with an oligo dT nucleotide (anti-sense primer) to amplify by PCR a DNA fragment from L. donovani cDNA. The amplified DNA fragment was cloned and used as a probe to screen a L. donovani cDNA library. The cloned gene (Ld peptide gene) has an open reading frame of 525 bp and has no homology with any known protein/gene sequence. Northern blot analyses indicated that the Ld peptide/gene is broadly distributed and expressed among species of the Leishmania genus, in both the amastigote and promastigote life cycle forms. Using the pGEX 2T vector, the gene was expressed and the relationship of the purified recombinant protein with L. donovani was confirmed using both antibody and T cell responses from immunized or infected animals. The gene encodes a 23-kD molecule (Ldp 23) associated with the cell surface of L. donovani promastigotes. In addition, T cells purified from the lymph nodes of BALB/c mice immunized with L. donovani or infected with L. major, and from CBA/J mice infected with L. amazonensis were stimulated to proliferate by the recombinant Ldp 23 and produced high levels of IFN-gamma and no IL 4. This observation suggests that the Ldp 23 is an interesting parasite molecule for the studies concerning the host/parasite interaction because the Th1 pattern of cytokine response that it induces is correlated with resistance to Leishmania infections. These results clearly point to an alternative strategy for the purification of proteins useful for the development of both vaccines and immunological diagnostic tools not only against leishmaniasis but also for other diseases caused by intracellular pathogens.

摘要

本文报道的研究描述了从感染杜氏利什曼原虫的小鼠巨噬细胞的MHC II类分子中分离肽段,以及利用所得肽段序列拯救病原体肽段供体蛋白的过程。肽段的分离是通过比较从感染巨噬细胞中提取的肽段的反相高效液相色谱(RP HPLC)图谱与从未感染细胞中提取的肽段的图谱来进行的。对感染巨噬细胞特有的几个不同的HPLC峰进行了测序。其中一个与任何已知蛋白都不同源的肽段被用于指导设计一个寡核苷酸正义引物,该引物与一个寡聚dT核苷酸(反义引物)结合,通过PCR从杜氏利什曼原虫cDNA中扩增出一个DNA片段。扩增的DNA片段被克隆并用作探针筛选杜氏利什曼原虫cDNA文库。克隆的基因(Ld肽基因)有一个525 bp的开放阅读框,与任何已知的蛋白/基因序列都没有同源性。Northern印迹分析表明,Ld肽/基因在利什曼原虫属的物种中广泛分布并在无鞭毛体和前鞭毛体生命周期形式中都有表达。利用pGEX 2T载体表达该基因,并使用来自免疫或感染动物的抗体和T细胞反应证实了纯化的重组蛋白与杜氏利什曼原虫的关系。该基因编码一个与杜氏利什曼原虫前鞭毛体细胞表面相关的23-kD分子(Ldp 23)。此外,从用杜氏利什曼原虫免疫或感染硕大利什曼原虫的BALB/c小鼠的淋巴结中以及从感染亚马逊利什曼原虫的CBA/J小鼠的淋巴结中纯化的T细胞,被重组Ldp 23刺激而增殖,并产生高水平的IFN-γ且不产生IL 4。这一观察结果表明,Ldp 23是一个在宿主/寄生虫相互作用研究中有趣的寄生虫分子,因为它诱导的细胞因子反应的Th1模式与对利什曼原虫感染的抗性相关。这些结果清楚地指出了一种用于纯化蛋白质的替代策略,这些蛋白质不仅可用于开发针对利什曼病的疫苗和免疫诊断工具,还可用于开发针对其他由细胞内病原体引起的疾病的疫苗和免疫诊断工具。

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