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首页> 外文期刊>Molecular biology reports >Expression of EGFP-spider dragline silk fusion protein in BmN cells and larvae of silkworm showed the solubility is primary limit for dragline proteins yield.
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Expression of EGFP-spider dragline silk fusion protein in BmN cells and larvae of silkworm showed the solubility is primary limit for dragline proteins yield.

机译:EGFP-spider牵引线丝融合蛋白在BmN细胞和家蚕幼虫中的表达表明其溶解度是牵引线蛋白产量的主要限制。

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摘要

Spider dragline silk is a unique fibrous protein with combination of tensile strength and elasticity, but the isolation of large amount of silk from spiders is not feasible. In this paper, we used a newly established Bac-to-Bac/BmNPV Baculovirus expression system to express the recombinant spider (Nephila clavata) dragline silk protein (MaSp1) fused EGFP in BmN cells and larvae of silkworm. A 70 kDa fusion protein was visualized after rBacmid/BmNPV/drag infection by SDS-PAGE and immunoblotting analysis. Fusion protein expressed in the BmN cells probably occupied five percent of the cell total protein; In a silkworm larva, approximately 6 mg fusion proteins were expressed. Solubility analysis of the expressed spider dragline silk protein indicated that 60% fusion protein is insoluble. EGFP fluorescence showed that fusion protein is tend to form aggregate by self assemblage. The results indicated the solubility is the primary limit for spider dragline proteins yield. It also suggested that directly produce fibrous spider silk in the secreting-silk organs of the transgenic silkworm larvae might be a better method.
机译:蜘蛛拉铲丝是具有抗张强度和弹性的独特纤维蛋白,但是从蜘蛛中分离大量丝是不可行的。在本文中,我们使用新建立的Bac-to-Bac / BmNPV杆状病毒表达系统在BmN细胞和家蚕幼虫中表达融合了EGFP的重组蜘蛛(Nephila clavata)拉索丝蛋白(MaSp1)。在rBacmid / BmNPV / drag感染后,通过SDS-PAGE和免疫印迹分析可以看到70 kDa的融合蛋白。在BmN细胞中表达的融合蛋白可能占据了细胞总蛋白的5%。在家蚕幼虫中,表达了约6 mg融合蛋白。表达的蜘蛛牵引丝蛋白的溶解度分析表明60%的融合蛋白不溶。 EGFP荧光显示融合蛋白倾向于通过自组装形成聚集体。结果表明溶解度是蜘蛛拉丝蛋白产量的主要限制。这也表明在转基因蚕幼虫分泌丝器官中直接产生纤维状蜘蛛丝可能是一种更好的方法。

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