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一种在组织包囊基质中大量表达的65千道尔顿刚地弓形虫抗原的分子特征

Molecular characterization of a 65-kilodalton Toxoplasma gondii antigen expressed abundantly in the matrix of tissue cysts.

作者信息

Parmley S F, Yang S, Harth G, Sibley L D, Sucharczuk A, Remington J S

机构信息

Department of Immunology and Infectious Diseases, Palo Alto Medical Foundation, CA 94301.

出版信息

Mol Biochem Parasitol. 1994 Aug;66(2):283-96. doi: 10.1016/0166-6851(94)90155-4.

Abstract

We describe the cloning and characterization of a novel antigen expressed in the bradyzoite stage of Toxoplasma gondii. A cDNA library was constructed in bacteriophage lambda gt11 Sfi-Not using messenger RNA molecules isolated from cysts of the ME49 strain of T. gondii. The recombinant phage library was subjected to screening with polyclonal antibodies against bradyzoite antigens. This screening identified a recombinant antigen that was recognized strongly by polyclonal antibodies against bradyzoite antigens as well as by sera from mice chronically infected with T. gondii. The native antigen is a protein of 65 kDa that localized to the matrix of the cyst and the cyst wall surrounding the bradyzoites. The antigen was found to be expressed abundantly in cysts but could not be detected in tachyzoites or within the parasitophorous vacuole of tachyzoite infected host cells. Genomic and cDNA sequence of the gene revealed an open reading frame encoding 452 amino acids interrupted by 2 introns: a 503-bp intron located in the 5' untranslated region preceding the protein coding sequence and a 110-bp intron located 95 bp downstream of the first ATG.

摘要

我们描述了一种在刚地弓形虫缓殖子阶段表达的新型抗原的克隆和特性。使用从刚地弓形虫ME49株包囊中分离的信使RNA分子,构建了噬菌体λgt11 Sfi-Not cDNA文库。用抗缓殖子抗原的多克隆抗体对重组噬菌体文库进行筛选。该筛选鉴定出一种重组抗原,它能被抗缓殖子抗原的多克隆抗体以及来自慢性感染刚地弓形虫小鼠的血清强烈识别。天然抗原是一种65 kDa的蛋白质,定位于包囊基质和围绕缓殖子的包囊壁。发现该抗原在包囊中大量表达,但在速殖子或速殖子感染的宿主细胞的寄生泡内无法检测到。该基因的基因组和cDNA序列显示一个编码452个氨基酸的开放阅读框,被2个内含子打断:一个503 bp的内含子位于蛋白质编码序列之前的5'非翻译区,一个110 bp的内含子位于第一个ATG下游95 bp处。

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