稻纵卷叶螟颗粒体病毒的持续感染及检测

doi:10.3864/j.issn.0578-1752.2020.19.012

摘要/Abstract

摘要：

【目的】稻纵卷叶螟颗粒体病毒（Cnaphalocrocis medinalis granulovirus,CnmeGV）是稻纵卷叶螟的专性病原微生物,病毒持续感染对害虫种群控制具有重要作用。研究旨在建立CnmeGV持续感染的检测方法,分析病毒持续感染对害虫种群的控制作用,为病毒杀虫剂的应用提供理论依据。【方法】多重比较分析颗粒体病毒granulin基因序列,选择变异较大区域设计CnmeGV巢式PCR引物并评估探针的灵敏度和可靠性。室内使用玉米苗繁殖稻纵卷叶螟,以10⁶ OB/mL的亚致死浓度口服感染4龄幼虫,并饲养至成虫阶段,统计羽化率。以10%甲醛处理口服感染病毒的昆虫体表,利用探针分析稻纵卷叶螟持续感染种群中幼虫、蛹、蛹蜕及成虫的带毒率。施用10⁶ OB/mL病毒制剂,监测次年稻纵卷叶螟幼虫发病率,并检测田间土壤的带毒率。【结果】建立了CnmeGV的巢式PCR探针,包括外侧引物Cm-gran1和内侧引物Cm-gran2。巢式PCR探针检测最低灵敏度为0.85 fg·μL^-1,是常规PCR的1 000倍。探针具有较高的可靠性,在稻纵卷叶螟的食物源（水稻、玉米）、其他多角体和颗粒体病毒中,均未检测到目标片段。使用10%甲醛处理病毒感染的幼虫体表10、30 min和16 h后,均未检测到病毒目标片段,但处理16 h后,稻纵卷叶螟蛹不能羽化。亚致死浓度的病毒处理稻纵卷叶螟幼虫96 h后,未显症幼虫经体表处理后病毒检出率为100%。待幼虫化蛹及羽化后,蛹、蛹蜕和成虫的病毒检出率分别为87.5%、83.3%和16.7%。经卡方检测,幼虫到化蛹阶段,病毒感染率未有显著变化（χ²=3.2,P=0.234）;而蛹羽化为成虫,病毒检出率显著降低（χ²=32.356,P=0）,表明成虫在变态过程中,大部分病毒随蛹蜕一起被排出体外。进一步待蛹羽化,发现和对照群体93.4%的羽化率相比,病毒感染群体成虫羽化率仅有30.8%。田间调查显示,已使用CnmeGV的田块次年稻纵卷叶螟幼虫病毒显症率为4%,土壤带毒率为58%,病毒可以在土壤中存活并通过水平传播持续感染稻纵卷叶螟种群。【结论】构建的巢式PCR探针具有较高的灵敏度,可用于CnmeGV持续感染的检测。CnmeGV的持续感染可有效控制稻纵卷叶螟的发生,成虫变态在稻纵卷叶螟体内病原物的清除中发挥了重要作用。

关键词: 稻纵卷叶螟, 颗粒体病毒, 持续感染, 潜伏侵染, 分子标记, 水平传播, 昆虫变态

Abstract:

【Objective】Cnaphalocrocis medinalis granulovirus (CnmeGV) is a specific pathogenic microorganism of Cnaphalocrocis medinalis. Persistent infection of baculovirus plays an important role in pest population control. The objective of this study is to construct the detection method of persistent infection with CnmeGV, analyze the control effect of viral persistent infection on pest population, and to provide a theoretical basis for the application of viral pesticides.【Method】The largely diverged regions were selected to design CnmeGV nested PCR primers based on multiple comparisons of granulin gene sequences of granulovirus. The sensitivity and reliability of probes were further evaluated. The maize leaves were used to feed C. medinalis in the laboratory. The 4th instar larvae were singled out, and then fed with maize leaves soaked by CnmeGV with a sublethal concentration of 10⁶ OB/mL. The infected C. medinalis were reared to adult stage, and the emergence rate was counted. After treating the insect body surface with 10% formaldehyde, the carrying CnmeGV rates of larvae, pupae, pupal molts and adults in persistent infection population of C. medinalis were analyzed using these probes. The prevalence rate of larvae and carrying rate of soil in the next year after using CnmeGV were also detected.【Result】The probes of CnmeGV nested PCR were constructed including the outer primer Cm-gran1 and the inner primer Cm-gran2. The sensitivity of nested PCR was 0.85 fg·μL ^-1 genomic DNA, which was 1 000 times higher than that of the conventional PCR. The probes were highly reliable, and no target fragment was detected in the food sources of C. medinalis (rice and maize), other polyhedrosis and granulosis viruses. The target fragments of CnmeGV were not detected in larvae after treated with 10% formaldehyde for 10, 30 min and 16 h, respectively. However, the pupa of C. medinalis could not emerge after 16 h of treatment. The detection rate of CnmeGV was 100% in the larvae of infected population treated with sublethal concentration of CnmeGV for 96 h. After pupation and emergence, the detection rates of pupae, pupal molts and adults were 87.5%, 83.3% and 16.7%, respectively. The detection rate of CnmeGV had no significant change from larva to pupa stage (χ ²=3.2, P=0.234) by Chi-square test. However, the detection rate of CnmeGV decreased significantly (χ ²=32.356, P=0) from pupa to adult stage, indicating that most of the viruses were excreted from the body with pupal molt during metamorphosis. The emergence rate of adult in infected population (30.8%) was significantly lower than that of the control (93.4%). Field tests showed that the prevalence rate of C. medinalis larvae in the field at one year following CnmeGV treatment was 4%, and the rate of soil carrying CnmeGV was 58%, suggesting that CnmeGV could survive in the soil and continue to infect C. medinalis through horizontal transmission.【Conclusion】The sensitivity of constructed nested PCR probes is high and can be used for the detection of CnmeGV persistent infection. Persistent infection of CnmeGV can effectively control the population development of C. medinalis, and adult metamorphosis plays an important role in removing pathogens.

Key words: Cnaphalocrocis medinalis, granulovirus, persistent infection, latent infection, molecular marker, horizontal transmission, insect metamorphosis

韩光杰,刘琴,李传明,祁建杭,徐彬,陆玉荣,徐健. 稻纵卷叶螟颗粒体病毒的持续感染及检测[J]. 中国农业科学, 2020, 53(19): 3988-3995.

HAN GuangJie,LIU Qin,LI ChuanMing,QI JianHang,XU Bin,LU YuRong,XU Jian. The Persistent Infection and Detection of Cnaphalocrocis medinalis Granulovirus in Cnaphalocrocis medinalis[J]. Scientia Agricultura Sinica, 2020, 53(19): 3988-3995.

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引物 Primer	序列 Sequence (5′→3′)	产物大小 Product size (bp)
Cm-gran1	F: TGATGCCGAGTATGAACCG	541
	R: TTCCTCAACCTCTCCCGTAG
Cm-gran2	F: CGCATCACTCTGTTCAAGG	422
	R: ACGAGAGGACGGTAGAAGTAG