Cloning, Expression, and Functional Analysis of the Full-Length cDNA ofAcetyl-CoA C-acetyltransferase (AACT) Genes Related to TerpenoidSynthesis in Platycodon grandiflorus

基因 分子生物学 互补DNA 生物 重组DNA 克隆(编程) 亚细胞定位 免疫印迹 表达式向量 基因表达 生物化学 计算机科学 程序设计语言
作者
Mengli Liu,Hanwen Yu,Jing Li,Nan Dong,Bowen Chen,Rui Xu,Junxian Wu,Xiangwei Chang,Jutao Wang,Huasheng Peng,Liangping Zha,Shuangying Gui
出处
期刊:Protein and Peptide Letters [Bentham Science]
卷期号:29 (12): 1061-1071 被引量:7
标识
DOI:10.2174/0929866529666220831114920
摘要

Abstract: Platycodon grandiflorus is a well-known and widely distributed traditional herbal medicine and functional food in Asia, with triterpenoids as the main bioactive component in its roots. Acetyl-CoA C-acetyltransferase (AACT) is the initiation enzyme in the mevalonate pathway and plays an important role in the biosynthesis of terpenoids. Objective: The objective of this study was to clone and identify the PgAACT function in P. grandiflorus. Method: The full-length sequence of PgAACT genes was isolated and cloned from P. grandiflorus by polymerase chain reaction (PCR). The recombinant plasmid was constructed using the pET-32a vector and expressed in E. coli Transetta (DE3) cells. Subcellular localization of AACT was observed in the epidermal cells of N. tabacum. Quantitative reverse transcription-PCR (qRT-PCR) was used to identify the PgAACT gene transcription levels. After MeJA treatment, the changes in AACT gene expression were observed, and UHPLC-Q-Exactive Orbitrap MS/MS was used to detect the changes in P. grandiflorus saponins. Results: In this study, two full-length cDNAs encoding AACT1 (PgAACT1) and AACT2 (PgAACT2) were isolated and cloned from P. grandiflorus. The deduced PgAACT1 and PgAACT2 proteins contain 408 and 416 amino acids, respectively. The recombinant vectors were constructed, and the protein expression was improved by optimizing the reaction conditions. Sodium dodecyl sulphate-polycrylamide gel electrophloresis and western blot analysis showed that the PgAACT genes were successfully expressed, with molecular weights of the recombinant proteins of 61 and 63 kDa, respectively. Subcellular localization showed that the PgAACT genes were localized in the cytoplasm. Tissue specificity analysis of P. grandiflorus from different habitats showed that PgAACT genes were expressed in the roots, stems, and leaves. After MeJA treatment, the expression level of PgAACT genes and the content of total saponins of P. grandiflorus were significantly increased, suggesting that PgAACT genes play an important role in regulating plant defense systems. Conclusion: Cloning, expression, and functional analysis of PgAACT1 and PgAACT2 will be helpful in understanding the role of these two genes in terpene biosynthesis.
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