本文旨在明确烟芽夜蛾囊泡病毒3h毒株（HvAV-3h）编码的第161号开放阅读框（3h-161）的序列特征及表达谱，为深入研究其功能奠定基础。【方法】 采用PCR技术克隆3h-161的CDs序列，构建原核表达载体，并制备高效的多克隆抗体；利用RT-PCR技术检测3h-161的转录情况，利用蛋白免疫印迹法检测3H-161的表达情况。【结果】 3h-161编码区长516 bp，共编码172个氨基酸残基，感染甜菜夜蛾Spodoptera exigua 3龄幼虫后12 h开始转录、48 h开始表达；3H-161在囊泡病毒属内的不同毒株（HvAV-3j、HvAV-3i、HvAV-3e、HvAV-3f和HvAV-3g）间高度保守，序列一致性为100%。【结论】 本研究阐明了3h-161的序列特征、获得了3H-161的多克隆抗体，明确了其表达谱，为进一步研究该基因在HvAV-3h感染甜菜夜蛾过程中发挥的作用奠定基础。

[Objectives]  To clarify the sequence characteristics and expression profile of the 3h-161 (open reading frame 161) gene in Heliothis virescens ascovirus 3h (HvAV-3h), thereby laying a foundation for further study of the function of this gene. [Methods]  The CDs sequence of 3h-161 was cloned using PCR technology, a prokaryotic expression plasmid vector constructed and efficient polyclonal antibody prepared. RT-PCR and Western blotting technology was then used to detect the transcription and expression of 3H-161. [Results]  The coding regions of 3h-161 are 516 bp in length, encoding 172 amino acids, respectively. Transcription began at 12 h and expression from 48 h in 3rd instar S. exigua larvae after infection with HvAV-3h. The putative protein sequences of 3h-161 are highly conservative in the Ascovirus and share 100% amino acid sequence identity with HvAV-3j, HvAV-3i, HvAV-3e, HvAV-3f and HvAV-3g. [Conclusion]  The sequence characteristics of 3h-161 were determined, a polyclonal antibody of 3H-161 was obtained, and the expression profile of this gene was clarified, all of which lay a foundation for further study of the function of the 3h-161 gene during the infection of S. exigua by HvAV-3h.