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Assembly of cyanobacterial and higher plant ribulose bisphosphate carboxylase subunits into functional homologous and heterologous enzyme molecules in Escherichia coli

机译:蓝细菌和高级植物核糖二磷酸羧化酶亚基在大肠杆菌中装配成功能性同源和异源酶分子

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摘要

The genes for the large (rbcL) and small (rbcS) subunits of ribulose-1,5 bisphosphate carboxylase-oxygenase (RuBPCase) from the cyanobacterium Synechococcus PCC 6301, and the rbcS gene of wheat, have been expressed in Escherichia coli in order to study homologous and heterologous enzyme assembly. Synechococcus L subunits expressed in E. coli in the absence of S subunits assemble into oligomeric structures without detectable enzyme activity. Co-expression of L and S subunits, achieved after infection with an M13 recombinant phage containing the rbcS gene, restores enzyme activity, thus demonstrating the essential role of S in the formation of an active RuBPCase. The S subunit, however, is neither required for the solubility nor for the assembly of the L subunits into oligomeric forms. The specific activity of the homologous Synechococcus RuBPCase can be modulated by changing the intracellular pool size of S by phage infection. Heterologous assembly between L subunits of Synechococcus and S subunits of wheat can be demonstrated and results in a functional enzyme. The hybrid RuBPCase has approximately 10% of the activity of the homologous Synechococcus enzyme.
机译:为了从大肠杆菌中表达出蓝细菌Synechococcus PCC 6301的核糖-1,5双磷酸羧化酶加氧酶(RuBPCase)的大(rbcL)和小(rbcS)亚基的基因,以及小麦的rbcS基因已在大肠杆菌中表达。研究同源和异源酶组装。在不存在S亚基的情况下,在大肠杆菌中表达的Synocococcus L亚基组装成寡聚结构,没有可检测的酶活性。在用含有rbcS基因的M13重组噬菌体感染后,L和S亚基的共表达恢复了酶的活性,从而证明了S在形成活性RuBPCase中的重要作用。然而,S亚基对于L亚基的溶解度或组装成寡聚体形式都不是必需的。同源Syechococcus RuBPCase的比活可以通过噬菌体感染改变S的胞内池大小来调节。可以证明Synechococcus的L亚基和小麦的S亚基之间的异源装配,并产生功能性酶。杂交RuBPCase具有同源Synechococcus酶的活性的约10%。

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