生物
转录因子
保幼激素
蜕皮激素受体
抄写(语言学)
RNA干扰
细胞生物学
家蚕
蜕皮激素
20-羟基蜕皮激素
卵黄原蛋白
分子生物学
核糖核酸
遗传学
基因
核受体
激素
内分泌学
哲学
语言学
作者
Zidan Zhu,Chunmei Tong,Binbin Qiu,Hongguang Yang,Jiahui Xu,Sichun Zheng,Qisheng Song,Qili Feng,Huimin Deng
出处
期刊:BMC Biology
[Springer Nature]
日期:2021-02-25
卷期号:19 (1)
被引量:39
标识
DOI:10.1186/s12915-021-00952-2
摘要
Abstract Background Krüppel homolog 1 (Kr-h1) is a critical transcription factor for juvenile hormone (JH) signaling, known to play a key role in regulating metamorphosis and adult reproduction in insects. Kr-h1 can also be induced by molting hormone 20-hydroxyecdysone (20E), however, the underlying mechanism of 20E-induced Kr-h1 expression remains unclear. In the present study, we investigated the molecular mechanism of Kr-h1 induction by 20E in the reproductive system of a model lepidopteran insect, Bombyx mori . Results Developmental and tissue-specific expression analysis revealed that BmKr-h1 was highly expressed in ovaries during the late pupal and adult stages and the expression was induced by 20E. RNA interference (RNAi)-mediated depletion of BmKr-h1 in female pupae severely repressed the transcription of vitellogenin receptor ( VgR ), resulting in the reduction in vitellogenin (Vg) deposition in oocytes. BmKr-h1 specifically bound the Kr-h1 binding site (KBS) between − 2818 and − 2805 nt upstream of BmVgR and enhanced the transcription of BmVgR . A 20E cis -regulatory element (CRE) was identified in the promoter of BmKr-h1 and functionally verified using luciferase reporter assay, EMSA and DNA-ChIP. Using pull-down assays, we identified a novel transcription factor B. mori Kr-h1 regulatory protein (BmKRP) that specifically bound the BmKr-h1 CRE and activated its transcription. CRISPR/Cas9-mediated knockout of BmKRP in female pupae suppressed the transcription of BmKr-h1 and BmVgR , resulting in arrested oogenesis. Conclusion We identified BmKRP as a new transcription factor mediating 20E regulation of B. mori oogenesis. Our data suggests that induction of BmKRP by 20E regulates BmKr-h1 expression, which in turn induces BmVgR expression to facilitate Vg uptake and oogenesis.
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