家蚕表皮蛋白CPR55基因受转录因子βFTZ-F1调控

IF 1.1 Q3 BIOLOGY
Md. Saheb Ali , Birendra Mishra , R.F. Rahman , Ahsanul Haque Swapon
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引用次数: 4

摘要

昆虫角质层由多种蛋白质组成,在蜕皮过程中形成,是一个复杂的生物学过程,它取决于激素水平和基因表达的相互作用。在本研究中,我们旨在阐明蜕皮激素依赖的表皮蛋白表达的时间调节机制和家蚕变态的潜在控制。CPR55的表达从W3早期就开始观察到,在化蛹时达到峰值,此时表皮甾体滴度下降。蜕皮激素脉冲诱导CPR55,在转移到无激素培养基后24 h达到表达高峰。在含环己亚胺的20E脉冲处理和在V4翅盘中添加20E后均未观察到CPR55的转录本。我们使用基因枪系统分析了CPR55基因的上游区域,该系统仅鉴定了一个βFTZ-F1结合位点,该位点对于通过外源性激素脉冲激活荧光素酶报告基因的顺式作用元件很重要。在589-bp启动子片段的背景下,该元件的定点诱变大大降低了报告基因的活性。通过电泳迁移位移试验鉴定了与βFTZ-F1位点结合的核蛋白,表明CPR55的表达受βFTZ-F1通过脱皮激素脉冲调控。结果证实,转录因子BmβFTZ-F1与角质层蛋白编码基因CPR55启动子中的顺式调控元件结合,调控其在家蚕变态过程中的表达。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
The silkworm Bombyx mori cuticular protein CPR55 gene is regulated by the transcription factor βFTZ-F1

The insect cuticle is composed of various proteins and formed during the moult under a complex biological process that depends on the cross talk between hormone levels and gene expression. In the present study, we aimed to clarify the ecdysone-dependent temporal regulation mechanisms of cuticular proteins expression and the underlying control of Bombyx mori metamorphosis. The expression of CPR55 was observed from the W3 early stage and peaked at pupation when the ecdysteroid titre declined. CPR55 was induced by the ecdysone pulse, and their expression peaked at 24 h after transfer to a hormone free medium. Transcripts of CPR55 were neither observed after the 20E pulse treatment in the presence of cycloheximide nor after the addition of 20E in V4 wing discs. We analysed the upstream region of the CPR55 gene using a transient reporter assay with a gene gun system which identified only one βFTZ-F1 binding site important for cis-acting elements for the transcription activation of the luciferase reporter gene by an ecdysone pulse. Site-directed mutagenesis of this element in the context of the 589-bp promoter fragment drastically decreased the reporter activity. The nuclear protein bound to βFTZ-F1 sites was identified by an electrophoretic mobility shift assay suggesting that CPR55 expression was regulated by βFTZ-F1 through the ecdysone pulse. The results confirmed that transcription factor, BmβFTZ-F1, binds to the cis-regulatory elements in the promoter of the gene coding for cuticle protein, CPR55, and regulates its expression during B. mori metamorphosis.

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