Cloning, sequencing, expression, and purification of aspartic proteases isolated from two human Demodex species

生物 重组DNA 蛋白酵素 克隆(编程) 分子生物学 生物化学 信号肽 基因 计算机科学 程序设计语言
作者
Hu Li,Chenglin Guan,Yae Zhao,Wanyu Zhang,Rong Chai,Juan Teng,Qiang Tian,Meng Xun,Feng Wu
出处
期刊:International Journal of Biological Macromolecules [Elsevier BV]
卷期号:253: 127404-127404
标识
DOI:10.1016/j.ijbiomac.2023.127404
摘要

Aspartic proteases (ASPs) are important hydrolases for parasitic invasion of host tissues or cells. This was the first study on Demodex ASP. First, the complete coding sequence (CDS) was amplified, cloned and sequenced. Then, the protein physical and chemical properties was analysed. Finally, the recombinant plasmid, expression and purification system was established. Results showed that the lengths of CDS of Demodex folliculorum and D. brevis were 1161 and 1173 bp, respectively. The molecular weight of the protein was approximately 40 KDa. It contained an aspartic acid residue, a substrate-binding site and signal peptide, yet lacked a transmembrane domain and was located in the membrane or extracellular matrix. The phylogenetic and conserved motif analyses showed that D. folliculorum and D. brevis clustered separately and then formed a single branch, which finally clustered with other Acariformes species. The prokaryotic expression systems for recombinant ASP with His-tag (rASP-His) and GST-tag (rASP-GST) were constructed. The inclusion bodies of rASP-His were renaturated by gradient urea and purified using NI beads, while those of rASP-GST were renaturated by sarkosyl and Triton X-100 and purified using GST beads. Conclusively, the prokaryotic expression and purification system of Demodex rASP was successfully established for further pathogenic mechanism research.
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