昆虫学报 ›› 2021, Vol. 64 ›› Issue ( 2): 141-148.doi: 10.16380/j.kcxb.2021.02.001

• 研究论文 •    下一篇

RNAi抑制小菜蛾Br-Z2/3基因对下游细胞凋亡基因表达及化蛹的影响

胡晓汉1, 田素芬1, 李亚勍1, 林硕2,3, 陈艺欣2,3, 魏辉2,3顾晓军1,2,*, 黄劲飞1,2,*, 王曦莹1, 李志华1   

  1. (1. 福建农林大学植物保护学院, 福州350002; 2. 福建省农业科学研究院, 福建省作物有害生物监测与治理重点实验室,
    福州350003; 3. 福建省农业科学研究院, 农业农村部福州作物有害生物科学观测试验站, 福州 350013)
  • 出版日期:2021-02-20 发布日期:2021-03-11

Effects of RNAi-mediated suppression of Br-Z2/3 gene on the expression of downstream apoptotic genes and pupation in the diamondback moth, Plutella xylostella (Lepidoptera: Plutellidae)

HU Xiao-Han1, TIAN Su-Fen1, LI Ya-Qing1, LIN Shuo2,3, CHEN Yi-Xin2,3, WEI Hui2,3, GU Xiao-Jun1,2,*, HUANG Jing-Fei1,2,*, WANG Xi-Ying1, LI Zhi-Hua1   

  1. (1. College of Plant Protection, Fujian Agriculture and Forestry University, Fuzhou 350002, China; 2. Fujian Key Laboratory for Monitoring and Integrated Management of Crop Pests, Fujian Academy of Agricultural Sciences, Fuzhou 350003, China; 3. Fuzhou Scientific Observing and Experimental Station of Crop Pests of Ministry of Agriculture and Rural Affairs, Fujian Academy of Agricultural Sciences, Fuzhou 350013, China)
  • Online:2021-02-20 Published:2021-03-11

摘要:  【目的】本研究旨在构建用于小菜蛾Plutella xylostella蛹期特异表达基因Br-Z2/3 dsRNA合成的体外原核表达系统,研究RNAi抑制Br-Z2/3基因对小菜蛾Br-Z2/3和细胞凋亡基因表达及化蛹的影响。【方法】构建小菜蛾L4440-Br-Z2/3重组载体,转化大肠杆菌Escherichia coli HT115感受态细胞,经IPTG诱导大量获得Br-Z2/3 dsRNA,显微注射Br-Z2/3 dsRNA至小菜蛾4龄幼虫进行RNAi;qPCR检测干扰Br-Z2/3基因12和24 h后小菜蛾4龄幼虫Br-Z2/3及其下游细胞凋亡基因reaper, caspase-9和Gadd45g的表达量;观察并统计Br-Z2/3 RNAi后小菜蛾4龄幼虫的化蛹率、平均化蛹时间、蛹畸形率和幼虫死亡率。【结果】成功实现了Br-Z2/3 dsRNA的原核表达。qPCR结果表明,RNAi干扰Br-Z2/3后,小菜蛾4龄幼虫Br-Z2/3基因和相关联的细胞凋亡基因reaper表达量显著下降,但caspase-9和Gadd45g表达量显著上升。注射Br-Z2/3 dsRNA的处理组,化蛹率显著低于对照组,且化蛹高峰期推迟,幼虫死亡率显著高于对照组且畸形蛹率增加。【结论】本研究成功构建了用于小菜蛾Br-Z2/3基因dsRNA合成的体外原核表达系统,利用显微注射法对Br-Z2/3进行RNA干扰,证明Br-Z2/3是调控小菜蛾化蛹的关键基因。

关键词: 小菜蛾; Br-Z2/3, 细胞凋亡基因, dsRNA, RNA干扰, 显微注射, 化蛹

Abstract: 【Aim】 This study aims to establish an in vitro prokaryotic expression system for synthesis of the dsRNA of pupa-specific expression gene Br-Z2/3 from the diamondback moth, Plutella xylostella, and to find out the effects of RNAi-mediated suppression of Br-Z2/3 on the expression of Br-Z2/3 and apoptotic genes and the pupation of the moth. 【Methods】 The L4440-Br-Z2/3 recombinant vector was constructed and transformed into competent cells of Escherichia coli HT115. The dsRNA of Br-Z2/3 was obtained after induction with IPTG, and RNAi was carried out by microinjecting Br-Z2/3 dsRNA into the 4th instar larvae of P. xylostella. At 12 and 24 h after RNAi of Br-Z2/3, the expression levels of Br-Z2/3 and its downstream apoptotic genes, reaper, caspase-9 and Gadd45g, were detected through qPCR. Simultaneously, the pupation rate, average pupation time, rate of deformed pupae and larval mortality of the 4th instar larvae of P. xylostella after RNAi of Br-Z2/3 were observed and recorded. 【Results】 The dsRNA of Br-Z2/3 was successfully expressed in the prokaryotic system. The qPCR results showed that the expression levels of Br-Z2/3 and the related apoptotic gene reaper decreased significantly, but those of caspase-9 and Gadd45g increased significantly after RNAi of Br-Z2/3 in the 4th instar larvae of P. xylostella. Compared with the control group, the dsBr-Z2/3-injected group showed significantly lower pupation rate with delayed pupation peak, and had significantly higher mortality and higher rate of deformed pupae. 【Conclusion】 An in vitro prokaryotic expression system for synthesis of the dsRNA of Br-Z2/3 from P. xylostella was successfully established. RNAi of Br-Z2/3 by microinjection demonstrates that Br-Z2/3 plays a crucial role in the pupation of P. xylostella.

Key words: Plutella xylostellaBr-Z2/3, apoptotic genes, dsRNA, RNA interference, microinjection, pupation