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一种新的微小隐孢子虫模块化蛋白,具有蓖麻毒蛋白B和LCCL结构域,在子孢子侵入阶段表达。

A new modular protein of Cryptosporidium parvum, with ricin B and LCCL domains, expressed in the sporozoite invasive stage.

作者信息

Tosini Fabio, Agnoli Alessia, Mele Raffaella, Gomez Morales Maria Angeles, Pozio Edoardo

机构信息

Department of Infectious, Parasitic and Immunomediated Diseases, Istituto Superiore di Sanità, viale Regina Elena 299, 00161 Rome, Italy.

出版信息

Mol Biochem Parasitol. 2004 Mar;134(1):137-47. doi: 10.1016/j.molbiopara.2003.11.014.

Abstract

The recombinant SA35 peptide has been described as an antigenic portion of a larger Cryptosporidium parvum protein. We identified and characterized the encoding Cpa135 gene and the entire protein, Cpa135. The Cpa135 gene was found to consist of a single exon of 4671 bp, and the mRNA transcribed in the sporozoites was identified. The predicted 1556 amino-acid protein showed the presence of domains which are widely conserved also in other unrelated phylogenetic groups (i.e. a ricin B and a LCCL motif). Comparison of Cpa135 sequence with genomic and protein databases revealed many related genes in other apicomplexan species and high homology with CCP2 protein from Plasmodium yoelii and Plasmodium berghei. The Cpa135 protein was identified and localized by using a monoclonal antibody (Mab) directed against the SA35 antigen (anti-SA35). In oocyst-sporozoite lysate, the anti-SA35 MAb recognized a 135 kDa protein that forms a protein complex larger than 200 kDa, which is mediated by disulfide bridges. Cpa135 synthesis was up-regulated during the excystation process. After host-cell invasion, Cpa135 gene expression was undetectable up to 48 h, whereas mRNA synthesis was newly observed at 72 h post-infection. The Cpa135 protein was localized in the apical complex, and it was found to be secreted by sporozoites during their gliding. Cpa135 persisted during the intracellular stages of the parasite, and it defined the boundaries of the parasitophorous vacuole in the infected cells. The unique array of domains and the homology with other apicomplexan proteins indicate that the Cpa135 protein is representative of a new family of proteins.

摘要

重组SA35肽已被描述为一种较大的微小隐孢子虫蛋白的抗原部分。我们鉴定并表征了编码Cpa135基因及整个Cpa135蛋白。发现Cpa135基因由一个4671 bp的单一外显子组成,并鉴定了在子孢子中转录的mRNA。预测的1556个氨基酸的蛋白显示存在在其他不相关的系统发育组中也广泛保守的结构域(即蓖麻毒素B和LCCL基序)。将Cpa135序列与基因组和蛋白质数据库进行比较,发现其他顶复门物种中有许多相关基因,并且与约氏疟原虫和伯氏疟原虫的CCP2蛋白具有高度同源性。通过使用针对SA35抗原的单克隆抗体(Mab)(抗SA35)鉴定并定位了Cpa135蛋白。在卵囊-子孢子裂解物中,抗SA35单克隆抗体识别一种135 kDa的蛋白,该蛋白形成大于200 kDa的蛋白复合物,由二硫键介导。在脱囊过程中Cpa135的合成上调。宿主细胞入侵后,直到48小时都检测不到Cpa135基因表达,而在感染后72小时新观察到mRNA合成。Cpa135蛋白定位于顶端复合体,并且发现它在子孢子滑行过程中由子孢子分泌。Cpa135在寄生虫的细胞内阶段持续存在,并确定了感染细胞中寄生泡的边界域的独特排列以及与其他顶复门蛋白的同源性表明Cpa135蛋白代表了一个新的蛋白家族。

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