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首页> 外文期刊>Biotechnology Letters >Production of human basic fibroblast growth factor (FGF-2) in Bifidobacterium breve using a series of novel expression/secretion vectors
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Production of human basic fibroblast growth factor (FGF-2) in Bifidobacterium breve using a series of novel expression/secretion vectors

机译:使用一系列新型表达/分泌载体在短双歧杆菌中生产人碱性成纤维细胞生长因子(FGF-2)

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Four E. coli-Bifidobacterium shuttle vectors were constructed using Bifidobacterium plasmids, pB44 and pB80. The vectors carry two bifidobacterial promoters, a signal peptide-encoding sequence, sec2, of Bifidobacterium breve, and a transcriptional terminator from hup gene of Bifidobacterium longum. Functionality of the constructs were tested using human FGF-2 gene. The expression of FGF-2 was detected by Western blotting in B. breve transformed with three of the vectors. The highest amount of FGF-2 was produced upon transformation with pESH86, which is a pB80-based plasmid carrying FGF-2 under control of a hup promoter (Phup). Similarly, the level of FGF-2 mRNA transcribed from pESH86 was approximately threefold higher, 882 ± 70 AU (arbitrary units), when compared to those transcribed from pB44-based pESH46 (Phup) (289 ± 65 AU) and pESH47 (Pgap) (282 ± 37 AU). These results suggest the vectors have the potential for production of exported fusion proteins in bifidobacteria and the expression levels can be regulated through the employment of different bifidobacterial promoters and/or replicons.
机译:使用双歧杆菌质粒pB44和pB80构建了四个大肠杆​​菌-双歧杆菌穿梭载体。这些载体带有两个双歧杆菌启动子,短双歧杆菌的信号肽编码序列sec2和长双歧杆菌hup基因的转录终止子。使用人FGF-2基因测试构建体的功能。通过Western印迹检测在用三种载体转化的短双歧杆菌中FGF-2的表达。用pESH86转化可产生最高量的FGF-2,pESH86是在hup启动子(Phup)的控制下携带FGF-2的基于pB80的质粒。同样,与基于pB44的pESH46(Phup)(289±65 AU)和pESH47(Pgap)转录的FGF-2 mRNA相比,从pESH86转录的FGF-2 mRNA的水平大约高三倍,为882±70 AU(任意单位)。 (282±37 AU)。这些结果表明载体具有在双歧杆菌中产生输出的融合蛋白的潜力,并且表达水平可以通过使用不同的双歧杆菌启动子和/或复制子来调节。

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