柞蚕Halloween家族基因在长光照解除蛹滞育及发育过程中的表达分析OA
Expression profiling of Halloween family genes in Antheraea pernyi(Lepidoptera:Saturniidae)during pupal diapause termination and development under long photoperiod
[目的]克隆获取柞蚕Antheraea pernyi中参与蜕皮激素合成的Halloween家族基因,并对长光照条件下柞蚕蛹解除滞育过程中Halloween基因的表达模式进行测定,为阐明柞蚕蛹滞育解除过程中蜕皮激素合成的特点奠定基础.[方法]利用RT-PCR从柞蚕中克隆获得5个Halloween家族基因(ApCyp307a1,ApCyp306a1,ApCyp302a1,ApCyp315a1 和 ApCyp314a1),并对其进行生物信息学分析;利用半定量RT-PCR检测柞蚕滞育期和发育期蛹脑、前胸腺、血淋巴、中肠、脂肪体、精巢/卵巢、气管和表皮中上述5个Halloween基因的表达量;利用RT-qPCR检测在室温(19~25℃)和低温(6℃)下储藏的柞蚕蛹在长光照(光周期17L:7D)下前胸腺和脂肪体中上述5个Halloween基因及蜕皮激素受体基因ApEcR和ApUSP的表达量;利用RT-qPCR检测柞蚕4龄幼虫和预蛹中Cyp314a1 RNAi 24 h时脂肪体中Cyp314a1,ApEcR和ApUSP的表达量,观测RNAi对幼虫和预蛹发育的影响.[结果]克隆获得柞蚕5个Halloween家族基因,根据同源序列比对分别命名为ApCyp307a1,ApCyp306a1,ApCyp302a1,ApCyp315a1 和 ApCyp314a1(GenBank 登录号分别为 MW677192,MW677193,MW677194,MW677195 和 MW677196);系统进化树表明,Halloween 基因在进化过程中高度保守.组织半定量PCR结果表明,ApCyp307a1,ApCyp306a1,ApCyp302a1和ApCyp315a1在柞蚕蛹前胸腺中表达量高,且ApCyp302a1和ApCyp315a1在柞蚕蛹发育期含量大幅上升;ApCyp314a1在发育期蛹中肠、脂肪体和精巢/卵巢中均有较高表达.低温保存的柞蚕蛹比室温保存蛹在光周期17L:7D下能更快地羽化;室温储存的柞蚕蛹经光周期17L:7D处理7 d时ApCyp315a1出现表达量高峰,ApCyp306a1,ApCyp302a1和ApUSP在处理21d时表达量升高,ApCyp314a1和ApEcR在临近羽化时(处理35d时)表达量达到高峰.低温保存的柞蚕蛹在光周期17L:7D处理7d时ApCyp307a1在羽化前期表达量较大升高,而ApCyp302a1在光周期17L:7D处理21~35 d时出现高表达量,ApCyp315a1在临近羽化时出现表达量高峰,这与常温滞育蛹解除滞育过程中的表达模式不同;ApCyp314a1在临近羽化时出现表达量高峰,ApEcR和ApUSP与常温组均表现出类似的表达模式.与注射dseGFP的对照组比,ApCyp314a1的RNAi使4龄幼虫和预蛹脂肪体中ApCyp314a1的表达量显著降低,明显抑制柞蚕的幼虫蜕皮和化蛹.[结论]这些结果表明Halloween基因在20-羟基蜕皮酮(20-hydroxyecdysone,20E)合成及柞蚕生长发育中作用显著,长光照解除滞育过程中20E合成相关基因表达量高峰期多在7-21 d,而ApCyp314a1在羽化前期大量表达.低温处理后能够加速柞蚕蛹滞育的解除,除ApCyp306a1呈现多个表达量高峰,其他Halloween基因多在处理中后期表达量升高.
[Aim]To clone and obtain the Halloween family genes involved in ecdysteroid synthesis in the Chinese oak silkworm,Antheraea pernyi,and to characterize their expression patterns during pupal diapause termination under long photoperiod conditions,so as to lay a foundation for elucidating the features of ecdysteroid synthesis throughout diapause termination in A.pernyi pupae.[Methods]Five Halloween family genes(ApCyp307a1,ApCyp306a1,ApCyp302a1,ApCyp315a1 and ApCyp314a1)were cloned from A.pernyi using RT-PCR and subjected to bioinformatic analysis.The expression levels of the above five Halloween genes in the brain,prothoracic gland,hemolymph,midgut,fat body,testis/ovary,trachea and cuticle of pupae of A.pernyi at diapause and developmental stages were examined via semi-quantitative RT-PCR.RT-qPCR was employed to analyze the expression levels of the above five Halloween genes,as well as the ecdysone receptor genes ApEcR and ApUSP,in the prothoracic gland and fat body of A.pernyi pupae stored at both room temperature(19-25 ℃)and low temperature(6 ℃)conditions under a long photoperiod of 17 L:7D.RT-qPCR was used to detect the expression levels of ApCyp314a1,ApEcR and ApUSP in the fat body at 24 h after RNAi of Cyp314a1 in the 4th instar larvae and prepupae of A.pernyi,and the effects of RNAi on the development of larvae and prepupae were further observed and detected.[Results]Five Halloween family genes of A.pernyi were cloned,and designated as ApCyp307a1,ApCyp306a1,ApCyp302a1,ApCyp315a1 and ApCyp314a1(GenBank accession numbers were MW677192,MW677193,MW677194,MW677195 and MW677196,respectively),based on homologous sequence alignment.Phylogenetic tree revealed that Halloween genes are highly conserved throughout evolution.Tissue-specific semi-quantitative PCR results indicated high expression levels of ApCyp307a1,ApCyp306a1,ApCyp302a1 and ApCyp315a1 in the prothoracic gland of A.pernyi pupae,with ApCyp302a1 and ApCyp315a1 showing marked upregulation during developmental stage of A.pernyi pupae.ApCyp314a1 was highly expressed in the midgut,fat body and testis/ovary of A.pernyi pupae at the developmental stage.A.pernyi pupae stored at low temperatures and exposed to the photoperiod of 17 L:7D exhibited accelerated emergence compared to those maintained at room temperature.The expression level of ApCyp315a1 in A.pernyi pupae stored under the photoperiod of 17L:7D at room temperature peaked at 7 d after treatment,those of ApCyp306a1,ApCyp302a1 and ApUSP were increased at 21 d after treatment,whereas those of ApCyp314a1 and ApEcR peaked near eclosion(at 35 d after treatment).After low-temperature storage,the expression level of ApCyp307a1 in A.pernyi pupae was increased substantially during the pre-eclosion phase at 7 d after treatment under the photoperiod of 17L:7D,while ApCyp302a1 was highly expressed at 21-35 d after treatment under the photoperiod of 17L:7D,and the expression level of ApCyp315a1 peaked near eclosion,which showed a different expression pattern from that during the termination of pupae diapause at normal temperatures.The expression level of ApCyp314a1 peaked near eclosion,and ApEcR and ApUSP exhibited the expression profiles similar to those in the normal temperature group.Compared to the control group injected with dseGFP,RNAi of ApCyp314a1 significantly decreased the expression levels of ApCyp314a1 in the fat bodies of the 4th instar larvae and prepupae,and significantly suppressed the larval ecdysis and pupation of A.pernyi.[Conclusion]These results demonstrate that Halloween genes play crucial roles in 20-hydroxyecdysone(20E)synthesis,and growth and development of A.pernyi.During long photoperiod-induced diapause termination,the expression levels of 20E synthesis-related genes increased during 7-21 d,whereas ApCyp314a1 was highly expressed in the pre-eclosion phase.Low-temperature treatment can accelerate diapause termination in A.pernyi pupae.With the exception of ApCyp306a1,which displayed multiple expression level peaks,the other Halloween genes were predominantly upregulated during the middle and late stages of low-temperature treatment.
苏悦;朱梦云;段晓霞;邵鑫颖;汪琪;刘微;朱绪伟;王勇;秦利
沈阳农业大学生物科学技术学院,沈阳 110866沈阳农业大学生物科学技术学院,沈阳 110866沈阳农业大学生物科学技术学院,沈阳 110866沈阳农业大学生物科学技术学院,沈阳 110866沈阳农业大学生物科学技术学院,沈阳 110866沈阳农业大学生物科学技术学院,沈阳 110866||辽宁省昆虫资源专业技术创新中心,沈阳 110866河南省蚕业科学研究院,郑州 450008沈阳农业大学生物科学技术学院,沈阳 110866||辽宁省昆虫资源专业技术创新中心,沈阳 110866沈阳农业大学生物科学技术学院,沈阳 110866||辽宁省昆虫资源专业技术创新中心,沈阳 110866
生物科学
柞蚕蜕皮激素Halloween基因蜕皮激素受体RNAi
Antheraea pernyiecdysoneHalloween geneecdysone receptorRNAi
《昆虫学报》 2026 (3)
351-367,17
国家蚕桑产业技术体系建设专项(CARS-18)辽宁省科技重大专项(2024JH1/11700009)
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