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埃及伊蚊几丁质合成酶cDNA的克隆与特性分析

Cloning and characterization of a chitin synthase cDNA from the mosquito Aedes aegypti.

作者信息

Ibrahim G H, Smartt C T, Kiley L M, Christensen B M

机构信息

Department of Animal Health and Biomedical Sciences, 1656 Linden Drive, University of Wisconsin-Madison, WI 53706, USA.

出版信息

Insect Biochem Mol Biol. 2000 Dec;30(12):1213-22. doi: 10.1016/s0965-1748(00)00100-4.

DOI:10.1016/s0965-1748(00)00100-4
PMID:11044667
Abstract

Characterization of the enzymes involved in the chitin biosynthetic pathway in mosquitoes is critical due to the importance of chitin in the formation of the peritrophic matrix [PM] and its potential impact on vector competence. Chitin is the homopolymer of the amino sugar N-acetyl-D glucosamine [GlcNAc]. The final step of incorporation of GlcNAc into the chitin polymer is catalyzed by the enzyme chitin synthase [CS]. CS is a membrane bound enzyme, but the mechanism of its action in the biosynthesis of the PM is not understood. We have isolated and sequenced a CS-encoding cDNA clone from the mosquito Aedes aegypti, compared its sequence with CS from other organisms and studied its RNA expression. The cDNA is 3.5 kb in length with an open reading frame of 2.6 kb that encodes a protein of 865 amino acids with a predicted molecular mass of 99.5 kDa. The putative translation product shares 90% similarity to two CS proteins from Caenorhabditis elegans and 50% similarity to Saccharomyces cerevisiae in the catalytic domain of CS enzymes. Data suggest that CS is a single copy gene. RT-PCR analysis shows CS message in whole non-blood-fed females, whole blood-fed females, non-blood-fed midguts and in midguts dissected at different time points post-blood-feeding. In situ hybridization studies of midgut samples revealed that CS mRNA increases following a bloodmeal and is localized to the periphery of the epithelial cells facing the midgut lumen.

摘要

由于几丁质在围食膜[PM]形成中的重要性及其对媒介能力的潜在影响,对蚊子几丁质生物合成途径中相关酶的特性进行表征至关重要。几丁质是氨基糖N-乙酰-D-葡萄糖胺[GlcNAc]的同聚物。GlcNAc掺入几丁质聚合物的最后一步由几丁质合酶[CS]催化。CS是一种膜结合酶,但其在PM生物合成中的作用机制尚不清楚。我们从埃及伊蚊中分离并测序了一个编码CS的cDNA克隆,将其序列与其他生物的CS进行比较,并研究了其RNA表达。该cDNA长度为3.5 kb,开放阅读框为2.6 kb,编码一个865个氨基酸的蛋白质,预测分子量为99.5 kDa。推定的翻译产物在CS酶的催化结构域中与秀丽隐杆线虫的两种CS蛋白有90%的相似性,与酿酒酵母有50%的相似性。数据表明CS是一个单拷贝基因。RT-PCR分析显示,在未吸血的雌蚊整体、吸血的雌蚊整体、未吸血的中肠以及吸血后不同时间点解剖的中肠中均有CS信息。中肠样本的原位杂交研究表明,CS mRNA在吸血后增加,并定位于面向中肠腔的上皮细胞周边。

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