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Cloning and expression of 32 kDa ferritin from galleria mellonella

机译:梅花gall中32 kDa铁蛋白的克隆与表达

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We have sequenced a cDNA clone encoding 32-kDa ferritin subunit in the Wax Moth, Galleria mellonella. The 32-kDa ferritin subunit cDNA was obtained from PCR using identical primer designed from highly conserved regions of insect ferritins. RACE PCR was used to obtain the complete protein coding sequence. The 32-kDa ferritin subunit encoded a 232 amino acid polypeptide, containing a 19 leader peptide. The iron-responsive element (IRE) sequence with a predicted stem-loop structure was present in the 5'-untranslated region of the wax moth 32-kDa ferritin subunit mRNA. The 32-kDa sequence alignment had 78 and 69% identity with Manduca sexta and Calpodes ethlius (G), respectively. The G. mellonella ferritin subunits showed minimal identity with each other (19%). The glycosylation site (Asn-X-Ser/Thr) was found in the 32-kDa subunit but not in the 26-kDa subunit. Northern blot analysis showed that the mRNA expression of the 32-kDa ferritin was detected in the fat body and midgut. The fat body expression increased after 6 h and the mRNA in midgut dramatically increased about 3-fold the expression level at 12 h after ion feeding. Western blot revealed that a protein level of the 32-kDa subunit is abundant in midgut after 12 and 24 h iron feeding.
机译:我们已在蜡蛾,Galleria mellonella中测序了一个编码32-kDa铁蛋白亚基的cDNA克隆。通过使用从昆虫铁蛋白的高度保守区域设计的相同引物,通过PCR获得32kDa铁蛋白亚基cDNA。使用RACE PCR获得完整的蛋白质编码序列。 32 kDa铁蛋白亚基编码一个232个氨基酸的多肽,其中包含19个前导肽。具有预测的茎环结构的铁响应元件(IRE)序列存在于蜡蛾32-kDa铁蛋白亚基mRNA的5'-非翻译区。 32-kDa序列比对分别与六种Manduca sexta和Calpodes ethlius(G)具有78%和69%的同一性。 G. mellonella铁蛋白亚基彼此之间显示出最小的同一性(19%)。在32 kDa亚基中发现了糖基化位点(Asn-X-Ser / Thr),但在26 kDa亚基中未发现。 Northern印迹分析显示在脂肪体和中肠中检测到32kDa铁蛋白的mRNA表达。喂食离子后12 h,脂肪体表达增加,而中肠的mRNA表达水平显着增加约3倍。 Western印迹显示,喂入铁12和24小时后,中肠中32-kDa亚基的蛋白质水平很高。

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