广藿香醇合酶PcPTS互作蛋白的筛选与鉴定分析  被引量：1

作　　者：陈立凯 吴带娣 CHEN Likai;WU Daidi(School of Pharmaceutical Sciences,Guangzhou University of Chinese Medicine,Guangzhou 510006,China;Key Laboratory of Chinese Medicinal Resource from Lingnan,Ministry of Education(Guangzhou University of Chinese Medicine),Guangzhou 510006,China)

机构地区：[1]广州中医药大学中药学院,广东广州510006 [2]岭南中药资源教育部重点实验室(广州中医药大学),广东广州510006

出　　处：《广东农业科学》2024年第5期1-15,共15页Guangdong Agricultural Sciences

基　　金：国家自然科学基金(82373976);广东省乡村振兴战略专项资金种业振兴项目(GDNK20230331);云浮市科技创新战略专项(202301)。

摘　　要：【目的】广藿香[Pogostemon cablin(Blanco)Benth.]是临床常用的芳香化湿药,其质量指标成分广藿香醇具有良好的抗病毒、抗炎症等活性。广藿香醇合酶(Patchouli alcohol synthase,PcPTS)在广藿香醇生物合成途径中起关键作用,但其在蛋白互作层面调控广藿香醇合成的机制尚不清楚。旨在筛选PcPTS的互作蛋白,以揭示PcPTS在广藿香醇生物合成途径中的调控机制和功能。【方法】利用酵母双杂交技术和GST pull-down联合液相色谱-串联质谱(LC-MS/MS)技术筛选可能与PcPTS互作的蛋白,利用MASCOT软件和BLAST分析注释互作蛋白,选取有文献报道参与其他蛋白互作、影响蛋白转运、修饰或降解、参与次生代谢调控的蛋白,利用酵母双杂交技术初步验证它们与PcPTS蛋白的互作关系并对互作蛋白进行生物信息学分析。【结果】通过PCR技术成功克隆了PcPTS的cDNA序列,开放阅读框(ORF)为1659 bp,编码522个氨基酸。构建了广藿香cDNA初级文库和酵母杂交文库,初级和次级文库容量分别为7.6×10^(6) CFU和8.6×10^(6) CFU,初级和次级文库的重组率均为100%,且插入片段平均长度均大于800 bp。构建的诱饵载体pGBKT7-PcPTS对酵母菌株不产生毒性,且无自激活活性。利用酵母双杂交筛选得到阳性克隆并进行测序和BLAST分析,获得17个候选蛋白。成功构建了GST-PcPTS表达载体,诱导表达纯化获得GST-PcPTS诱饵蛋白,利用诱饵蛋白从广藿香总蛋白中捕获互作蛋白,共鉴定出98个候选互作蛋白。从候选蛋白中筛选14个可能与PcPTS互作的蛋白,利用酵母双杂交进行点对点验证,结果发现PcC3H6、PcENO3、PcACR11和PcHAD与PcPTS存在相互作用。生物信息分析表明,四者分别属于CCCH锌指蛋白家族、烯醇化酶蛋白、ACR亚家族和HAD-like超家族。【结论】初步筛选验证获得与PcPTS存在相互作用的4个蛋白PcC3H6、PcENO3、PcACR11和PcHAD,有助于揭示PcPTS在广藿香醇生物合成【Objective】Pogostemon cablin(Blanco)Benth.is a frequently-used aromatic herb eliminating dampness in clinical settings,with its primary bioactive compound,patchouli alcohol,demonstrating potent antiviral and anti-inflammatory and other beneficial properties.Patchoulialcohol synthase(PcPTS)plays an essential role in the biosynthesis pathway of patchouli alcohol.However,the precise mechanisms by which PcPTS modulates patchouli alcohol production at the level of protein-protein interactions is still unclear.This study aims to identify interacting proteins of PcPTS in order to elucidate its regulatory mechanisms and functions in the biosynthesis pathway of patchouli alcohol.【Method】The yeast two-hybrid technique and GST pull-down combined with liquid chromatography-tandem mass spectrometry(LC-MS/MS)were employed to identify potential interacting proteins of PcPTS.The annotation of these interacting proteins was conducted by the MASCOT software and BLAST analysis.Proteins known to be involved in protein translocation,modification,degradation and regulation of secondary metabolism were selected for further analysis.Their interactions with PcPTS proteins were initially confirmed through yeast two-hybrid technology,and subsequently analyzed by using bioinformatics tools.【Result】The cDNA sequence of PcPTS was successfully cloned by PCR,resulting in an open reading frame(ORF)of 1659 bp,encoding 552 amino acids.The primary cDNA library and the yeast hybrid cDNA library were constructed and obtained,with capacities of 7.6×10^(6) and 8.6×10^(6) colony-forming units(CFU),respectively.Both libraries achieved a 100%recombination rate,with an average length of the inserted fragment greater than 800 bp.The constructed bait vector pGBKT7-PcPTS exhibited no toxicity towards yeast strains and did not exhibit any self-activating activity in yeast cells.The positive clones identified through yeast two-hybrid screening were subjected to sequencing and BLAST analysis,resulting in the identification of 17 candidate proteins.

关 键 词：药用成分 生物合成调控 植物代谢 酵母双杂交 广藿香醇合酶 互作蛋白 

分 类 号：S567.239[农业科学—中草药栽培]