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蠕形螨组织蛋白酶L的鉴定及遗传特征分析

Identification and genetic characterisatin of cathepsin L in Demodex.

作者信息

Li Hu, Chenglin Guan, Yae Zhao, Wanyu Zhang, Rong Chai

机构信息

Department of Pathogenic Biology and Immunology, School of Basic Medical Sciences, Xi'an Jiaotong University Health Science Center, No.76 Yanta West Road, Xi'an, 710061, Shaanxi Province, China.

出版信息

Exp Appl Acarol. 2023 Apr;89(3-4):329-344. doi: 10.1007/s10493-023-00789-0. Epub 2023 Apr 14.

Abstract

Owing to difficulties in obtaining functional gene sequences, molecular pathogenic mechanisms in Demodex have been understudied. In this study, overlap extension PCR was used to obtain the sequences of cathepsin L (CatL), a pathogenicity-related gene, to provide a foundation for subsequent functional research. Demodex folliculorum and Demodex brevis mites were obtained from the face skin of Chinese individuals, and Demodex canis mites were isolated from the skin lesions of a dog. RNA was extracted and used to synthesise double-stranded cDNA. PCR amplification, cloning, sequencing, and bioinformatics analysis of CatL were performed. CatL gene sequences of 1005, 1008, and 1008 bp were successfully amplified for D. brevis, D. folliculorum, and D. canis, respectively. These sequences showed 99.9 or 100% identity with templates previously obtained by RNA-seq. The Maximum Likelihood (ML) phylogenetic tree showed that D. folliculorum clustered with D. canis first, then with D. brevis, and finally with other Acariformes mite species. The three Demodex species had nine similar motifs to those of Sarcoptes scabies, Dermatophagoides pteronyssinus, and Dermatophagoides farinae, and motifs 10-13 were valuable for identification. CatL proteins of Demodex species were predicted to be approximately 38 kDa, be located in lysosomes, have a signal peptide but no transmembrane region, and have two functional domains, I29 and Pept_C1. However, interspecific differences were observed in secondary and tertiary protein structures. In conclusion, we successfully obtained CatL sequences of three Demodex species by overlap extension PCR, which creates conditions for further pathogenic mechanism studies.

摘要

由于获取功能基因序列存在困难,毛囊蠕形螨的分子致病机制研究较少。在本研究中,采用重叠延伸PCR技术获取了与致病性相关的组织蛋白酶L(CatL)序列,为后续功能研究奠定基础。从中国个体的面部皮肤获取毛囊蠕形螨和皮脂蠕形螨,从一只狗的皮肤病变中分离出犬蠕形螨。提取RNA并用于合成双链cDNA。对CatL进行PCR扩增、克隆、测序及生物信息学分析。分别成功扩增出皮脂蠕形螨、毛囊蠕形螨和犬蠕形螨的CatL基因序列,长度分别为1005、1008和1008 bp。这些序列与先前通过RNA测序获得的模板显示出99.9%或100%的同一性。最大似然(ML)系统发育树显示,毛囊蠕形螨首先与犬蠕形螨聚类,然后与皮脂蠕形螨聚类,最后与其他真螨目螨类物种聚类。这三种蠕形螨物种与疥螨、尘螨和粉螨有九个相似的基序,其中基序10-13对鉴定有价值。预测蠕形螨物种的CatL蛋白约为38 kDa,位于溶酶体中,有信号肽但无跨膜区域,有两个功能域,即I29和Pept_C1。然而,在蛋白质二级和三级结构上观察到种间差异。总之,我们通过重叠延伸PCR成功获得了三种蠕形螨物种的CatL序列,为进一步研究致病机制创造了条件。

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