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Poly[G] improved protein productivity of cell-free translation byinhibiting mRNase in wheat germ extract

机译:Poly [G]通过抑制小麦胚芽提取物中的mRNA酶提高无细胞翻译的蛋白质生产率

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摘要

Degradation of template mRNA lowers the efficiency of cell-free translation. Although cell-free translation system using wheat germ extract (WGE) is usually supplemented with placental RNase inhibitor (PRI) to stabilize mRNA, the decay rate of mRNA, however, was still fairly rapid. For elucidating cause of mRNA degradation in wheat germ cell-free translation system, the authors applied activity staining in SDS-PAGE gel to investigate ribonuclease activities in WGE. RNases or nucleases of molecular mass of about 65, 42, and 37 kDa were detected in WGE, and named WGa, WGb and WGc, respectively. WGb and WGc were nucleases that degraded both RNA and DNA, and WGa was an RNase. Polyguanylic acid (5'), poly[G], which was known to have affinity with RNases, strongly inhibited RNase activity in WGE. Addition of poly[G] to wheat germ cell-free translation system resulted in 7-fold increase in protein productivity. Luciferase mRNA that was added in the cell-free translation system as a template was not degraded in 90 min in the presence of poly[G] while it was degraded by 80% in 30 min in the absence of poly[G]. The authors concluded that poly[G] improved the protein productivity of wheat germ cell-free translation system by inhibiting RNase activity that degrades template RNA.
机译:模板mRNA的降解会降低无细胞翻译的效率。尽管通常使用小麦胚芽提取物(WGE)的无细胞翻译系统补充胎盘RNase抑制剂(PRI)来稳定mRNA,但是mRNA的衰减速度仍然相当快。为了阐明小麦无细胞翻译系统中mRNA降解的原因,作者在SDS-PAGE凝胶中应用了活性染色来研究WGE中的核糖核酸酶活性。在WGE中检测到分子量分别约为65、42和37 kDa的RNase或核酸酶,分别命名为WGa,WGb和WGc。 WGb和WGc是降解RNA和DNA的核酸酶,而WGa是RNase。聚鸟苷酸(5'),聚[G],已知与RNase具有亲和力,强烈抑制WGE中的RNase活性。将poly [G]添加到无小麦生殖细胞的翻译系统中导致蛋白质生产率提高了7倍。加入无细胞翻译系统中的荧光素酶mRNA作为模板在poly [G]存在下在90分钟内未降解,而在没有poly [G]的情况下在30分钟内降解了80%。作者的结论是,poly [G]通过抑制降解模板RNA的RNase活性,提高了小麦无细胞翻译系统的蛋白质生产率。

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