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寄生黄蜂双斑侧沟茧蜂中一种新型畸胎细胞特异性羧酸酯酶的分子克隆与分析

Molecular cloning and analysis of a novel teratocyte-specific carboxylesterase from the parasitic wasp, Dinocampus coccinellae.

作者信息

Gopalapillai Ravikumar, Kadono-Okuda Keiko, Okuda Takashi

机构信息

National Institute of Agrobiological Sciences, Owashi 1-2, Tsukuba, Ibaraki 305 8634, Japan.

出版信息

Insect Biochem Mol Biol. 2005 Oct;35(10):1171-80. doi: 10.1016/j.ibmb.2005.05.010.

DOI:10.1016/j.ibmb.2005.05.010
PMID:16102422
Abstract

Teratocytes derived from the embryonic membrane (serosa) of parasitoids are released into the host hemocoel when the parasitoid eggs hatch, where they perform several functions during the post-embryonic stage. A full-length cDNA encoding a putative carboxylesterase was isolated from the teratocytes of Dinocampus coccinellae and was designated as teratocyte-specific carboxylesterase (TSC). It contained an open reading frame of 2571 bp coding for a protein of 857 amino acids with a calculated molecular mass of 89 kDa. The deduced amino acid sequence had many structural features that are highly conserved among serine hydrolases including Ser, Glu and His as a catalytic triad, carboxylesterase type-B (FGGNPNSVTLLGYSAG)/ lipase-serine (VTLLGYSAGA) active sites, and six N-glycosylation sites. Interestingly, the mRNA encoding the TSC gene was expressed exclusively in teratocytes but not in the parasitoid larva or in the non-parasitized host. Most notably, the TSC protein was distinguished by an insertion of 294 amino acids towards the N-terminal region and was flanked by carboxylesterase domains. Furthermore, sequence alignment and homology search revealed these additional amino acids to be unique to TSC and the insertion contributed significantly to its molecular mass resulting in a larger protein than other esterases. In addition to sequence analysis, the possible role of TSC in relation to the host (Coccinella septempunctata) and parasitoid (D. coccinellae) system is discussed.

摘要

当寄生蜂卵孵化时,源自寄生蜂胚胎膜(浆膜)的畸形细胞会释放到宿主血腔中,在胚胎后期阶段它们发挥多种功能。从食蚜蝇茧蜂的畸形细胞中分离出一个编码假定羧酸酯酶的全长cDNA,并将其命名为畸形细胞特异性羧酸酯酶(TSC)。它包含一个2571 bp的开放阅读框,编码一个857个氨基酸的蛋白质,计算分子量为89 kDa。推导的氨基酸序列具有许多在丝氨酸水解酶中高度保守的结构特征,包括作为催化三联体的Ser、Glu和His、羧酸酯酶B型(FGGNPNSVTLLGYSAG)/脂肪酶丝氨酸(VTLLGYSAGA)活性位点以及六个N-糖基化位点。有趣的是,编码TSC基因的mRNA仅在畸形细胞中表达,而在寄生蜂幼虫或未被寄生的宿主中不表达。最值得注意的是,TSC蛋白的特点是在N端区域插入了294个氨基酸,并两侧是羧酸酯酶结构域。此外,序列比对和同源性搜索显示这些额外的氨基酸是TSC特有的,并且该插入对其分子量有显著贡献,导致其比其他酯酶更大。除了序列分析外,还讨论了TSC在宿主(七星瓢虫)和寄生蜂(食蚜蝇茧蜂)系统中的可能作用。

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