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一种编码具有免疫诊断潜力的结构抗原的疥螨cDNA的鉴定及异源表达。

Identification and heterologous expression of a Sarcoptes scabiei cDNA encoding a structural antigen with immunodiagnostic potential.

作者信息

Casais Rosa, Prieto Miguel, Balseiro Ana, Solano Paloma, Parra Francisco, Martín Alonso José M

机构信息

Servicio Regional de Investigación y Desarrollo Agroalimentario, Laboratorio de Sanidad Animal, Jove, Gijón, Asturias, Spain.

出版信息

Vet Res. 2007 May-Jun;38(3):435-50. doi: 10.1051/vetres:2007007. Epub 2007 Mar 13.

Abstract

The mite Sarcoptes scabiei causes sarcoptic mange (or scabies), a disease of considerable human and veterinary significance. An S. scabiei cDNA clone of about 2 kb was isolated from a S. scabiei var. hominis expression library by immunological screening using blood serum from a naturally infected chamois (Rupicapra rupicapra). The nucleotide sequence of the identified cDNA contains an open reading frame of 1930 bp that encodes a 642 amino acid polypeptide. This polypeptide shows tandem repeats of a glycine-serine rich 20 residue sequence followed by a unique C-terminal glutamate rich 54 residue sequence. The cDNA or the deduced polypeptide did not show significant similarities to any of the sequences in the databases. A carboxyl-terminal fragment of this polypeptide (residues 380 to 642) was efficiently expressed in Escherichia coli as a fusion with Glutathione S-transferase and then was used to produce a specific antiserum. The antigen encoded by the cDNA was located at the integument of the mite's epidermis and the cavities surrounding its vital organs. Western blot analysis of mite extracts using the specific antiserum against the recombinant protein identified antigens larger that 60 kDa indicating that the isolated cDNA did not contain the full ORF. Moreover, we designed a diagnostic assay based on the carboxyl-terminal fragment of the antigen for the identification of infected animals.

摘要

疥螨可引发疥螨性 mange(或疥疮),这是一种对人类和兽医都具有重要意义的疾病。通过使用来自自然感染岩羚羊(岩羚羊)的血清进行免疫筛选,从人疥螨变种的表达文库中分离出一个约 2 kb 的疥螨 cDNA 克隆。所鉴定 cDNA 的核苷酸序列包含一个 1930 bp 的开放阅读框,编码一个 642 个氨基酸的多肽。该多肽显示出富含甘氨酸 - 丝氨酸的 20 个残基序列的串联重复,随后是独特的富含谷氨酸的 C 末端 54 个残基序列。该 cDNA 或推导的多肽与数据库中的任何序列均无显著相似性。该多肽的羧基末端片段(第 380 至 642 位残基)在大肠杆菌中作为与谷胱甘肽 S - 转移酶的融合蛋白有效表达,然后用于制备特异性抗血清。由 cDNA 编码的抗原位于螨表皮的体表及其重要器官周围的腔中。使用针对重组蛋白的特异性抗血清对螨提取物进行 Western 印迹分析,鉴定出大于 60 kDa 的抗原,表明分离的 cDNA 不包含完整的开放阅读框。此外,我们基于抗原的羧基末端片段设计了一种诊断方法,用于鉴定感染动物。

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