Yoshiga T, Okano K, Mita K, Shimada T, Matsumoto S
Laboratory of Molecular Entomology and Baculovirology, RIKEN, Hirosawa 2-1, Wako, Saitama, Japan.
Gene. 2000 Apr 4;246(1-2):339-45. doi: 10.1016/s0378-1119(00)00047-0.
We have isolated two acyl-CoA desaturase clones from a pheromone gland cDNA library by using the EST (expressed sequence tag) database of Bombyx mori. The putative acyl-CoA desaturases encoded by the clones desat 1 (2029bp) and desat 2 (2341bp) have 98% identity, and both proteins show 61% identities to Trichoplusia ni acyl-CoA Delta(11) desaturase. The deduced amino acid sequences conserve well the histidine clusters that are catalytically essential for acyl-CoA desaturase activity. Northern blot and RT-PCR analyses revealed that both transcripts of desat 1 and desat 2 were expressed predominantly in the pheromone gland. Both transcripts detected 3days before adult eclosion dramatically increased a day before adult eclosion, keeping the mRNA levels high even after eclosion. These results, combined with the fact that Delta(11) and Delta(10, 12) desaturation of palmitate is a key step to synthesize pheromone in B. mori, suggest that the desaturases encoded by desat 1 and desat 2 are involved in either or both of the desaturation steps in the pheromone biosynthetic pathway of B. mori. The mRNA levels of desat 1 and desat 2 were not affected by decapitation or injection of the pheromone biosynthesis activating neuropeptide (PBAN) into the adult female moth, suggesting that the transcription of desat 1 and desat 2 is not regulated by PBAN. In addition to the clones in the pheromone gland, eight other clones encoding the same Delta(9) desaturase homolog were found in an embryonic cDNA library by searching from the EST database of B. mori. The deduced amino acid sequence from one of the clones (desat 3) shows 79% identity to T. ni Delta(9) desaturase but only 52% identity to the desaturases in the pheromone gland of B. mori. Northern blot analysis showed that the mRNA corresponding to the desat 3 was detected in the ovary and fat body, but not in the pheromone gland. Abundance of the Delta(9) desaturase clones (eight out of the 762 randomly sequenced clones) in the library prepared from diapause-destined embryos (40h after oviposition) suggests that the Delta(9) desaturase encoded by desat 3 plays an important role in embryonic development in B. mori.
我们利用家蚕的EST(表达序列标签)数据库,从性信息素腺cDNA文库中分离出了两个酰基辅酶A去饱和酶克隆。由克隆desat 1(2029bp)和desat 2(2341bp)编码的推定酰基辅酶A去饱和酶具有98%的同一性,并且这两种蛋白质与粉纹夜蛾酰基辅酶A Δ(11)去饱和酶均显示61%的同一性。推导的氨基酸序列很好地保留了对酰基辅酶A去饱和酶活性起催化关键作用的组氨酸簇。Northern印迹和RT-PCR分析表明,desat 1和desat 2的转录本均主要在性信息素腺中表达。在成虫羽化前3天检测到的这两种转录本在成虫羽化前一天急剧增加,甚至在羽化后仍保持较高的mRNA水平。这些结果,再结合棕榈酸的Δ(11)和Δ(10, 12)去饱和是家蚕性信息素合成的关键步骤这一事实,表明desat 1和desat 2编码的去饱和酶参与了家蚕性信息素生物合成途径中的一个或两个去饱和步骤。desat 1和desat 2的mRNA水平不受断头或向成年雌蛾注射性信息素生物合成激活神经肽(PBAN)的影响,这表明desat 1和desat 2的转录不受PBAN调控。除了性信息素腺中的克隆外,通过在家蚕的EST数据库中搜索,在胚胎cDNA文库中还发现了另外八个编码相同Δ(9)去饱和酶同源物的克隆。其中一个克隆(desat 3)推导的氨基酸序列与粉纹夜蛾Δ(9)去饱和酶显示79%的同一性,但与家蚕性信息素腺中的去饱和酶仅显示52%的同一性。Northern印迹分析表明,在卵巢和脂肪体中检测到了与desat 3相对应的mRNA,但在性信息素腺中未检测到。在滞育胚胎(产卵后40小时)制备的文库中,Δ(9)去饱和酶克隆的丰度(762个随机测序克隆中有8个)表明,desat 3编码的Δ(9)去饱和酶在家蚕胚胎发育中起重要作用。
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