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家蚕胚胎发育过程中蜕皮激素20-羟化酶的分子克隆及该酶的表达模式

Molecular cloning of ecdysone 20-hydroxylase and expression pattern of the enzyme during embryonic development of silkworm Bombyx mori.

作者信息

Maeda Sayaka, Nakashima Asuka, Yamada Ryouichi, Hara Noriyuki, Fujimoto Yoshinori, Ito Yoichi, Sonobe Haruyuki

机构信息

Department of Biology, Konan University, Kobe 658-8501, Japan.

出版信息

Comp Biochem Physiol B Biochem Mol Biol. 2008 Mar;149(3):507-16. doi: 10.1016/j.cbpb.2007.11.015. Epub 2007 Dec 14.

Abstract

In various insects, 20-hydroxyecdysone (20E) is indispensable for embryonic development. In eggs of the silkworm Bombyx mori, 20E has been demonstrated to be produced by two metabolic pathways: de novo synthesis from cholesterol and dephosphorylation of ovary-derived physiologically inactive ecdysteroid phosphates. In the former, ecdysone 20-hydroxylase (E20OHase) has been suggested to be a key enzyme. In the latter, it has been demonstrated that the dephosphorylation of ecdysteroid phosphates is catalyzed by a specific enzyme, ecdysteroid-phosphate phosphatase (EPPase). In this study, a cDNA encoding E20OHase was cloned from 3-day-old nondiapause eggs of B. mori and sequenced using PCR techniques. The protein exhibited the signature sequences characteristic of P450 enzymes, and mediated the conversion of ecdysone to 20E using the baculovirus expression system. Semi-quantitative analysis revealed that the E20OHase mRNA is expressed predominantly during gastrulation and organogenesis in nondiapause eggs, but is scarcely detected in diapause eggs whose development is arrested at the late gastrula stage. The developmental changes in the expression patterns of E20OHase and EPPase suggest that both enzyme activities are regulated at the transcription level, and both enzymes contribute cooperatively to 20E formation during embryonic development.

摘要

在多种昆虫中,20-羟基蜕皮酮(20E)对胚胎发育至关重要。在家蚕卵中,已证明20E通过两种代谢途径产生:由胆固醇从头合成以及卵巢来源的生理无活性蜕皮甾类磷酸盐的去磷酸化。在前一种途径中,蜕皮酮20-羟化酶(E20OHase)被认为是关键酶。在后一种途径中,已证明蜕皮甾类磷酸盐的去磷酸化由一种特定的酶——蜕皮甾类磷酸盐磷酸酶(EPPase)催化。在本研究中,从3日龄家蚕非滞育卵中克隆了编码E20OHase的cDNA,并使用PCR技术进行测序。该蛋白表现出P450酶特有的特征序列,并利用杆状病毒表达系统介导蜕皮酮向20E的转化。半定量分析表明,E20OHase mRNA主要在非滞育卵的原肠胚形成和器官发生过程中表达,但在发育停滞于原肠胚晚期的滞育卵中几乎检测不到。E20OHase和EPPase表达模式的发育变化表明,这两种酶的活性均在转录水平受到调控,且在胚胎发育过程中这两种酶协同作用于20E的形成。

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