首页> 外文期刊>The Journal of biological chemistry >Chorismate Pyruvate-Lyase and 4-Hydroxy-3-solanesylbenzoate Decarboxylase Are Required for Plastoquinone Biosynthesis in the Cyanobacterium Synechocystis sp. PCC6803
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Chorismate Pyruvate-Lyase and 4-Hydroxy-3-solanesylbenzoate Decarboxylase Are Required for Plastoquinone Biosynthesis in the Cyanobacterium Synechocystis sp. PCC6803

机译:Cyanobacterium indechocystis sp中的塑性醌生物合成需要酸己酯丙酸酯 - 裂解酶和4-羟基-3-甲苯基苯甲酸酯脱羧酶。 PCC6803

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Plastoquinone is a redox active lipid that serves as electron transporter in the bifunctional photosynthetic-respiratory transport chain of cyanobacteria. To examine the role of genes potentially involved in cyanobacterial plastoquinone biosynthesis, we have focused on three Synechocystis sp. PCC 6803 genes likely encoding a chorismate pyruvate-lyase (sll1797) and two 4-hydroxy-3-solanesylbenzoate decarboxylases (slr1099 and sll0936). The functions of the encoded proteins were investigated by complementation experiments with Escherichia coli mutants, by the in vitro enzyme assays with the recombinant proteins, and by the development of Synechocystis sp. single-gene knock-out mutants. Our results demonstrate that sll1797 encodes a chorismate pyruvate-lyase. In the respective knock-out mutant, plastoquinone was hardly detectable, and the mutant required 4-hydroxybenzoate for growth underlining the importance of chorismate pyruvate-lyase to initiate plastoquinone biosynthesis in cyanobacteria. The recombinant Slr1099 protein displayed decarboxylase activity and catalyzed in vitro the decarboxylation of 4-hydroxy-3-prenylbenzoate with different prenyl side chain lengths. In contrast to Slr1099, the recombinant Sll0936 protein did not show decarboxylase activity regardless of the conditions used. Inactivation of the sll0936 gene in Synechocystis sp., however, caused a drastic reduction in the plastoquinone content to levels very similar to those determined in the slr1099 knock-out mutant. This proves that not only slr1099 but also sll0936 is required for plastoquinone synthesis in the cyanobacterium. In summary, our data demonstrate that cyanobacteria produce plastoquinone exclusively via a pathway that is in the first reaction steps almost identical to ubiquinone biosynthesis in E. coli with conversion of chorismate to 4-hydroxybenzoate, which is then prenylated and decarboxylated.
机译:塑料醌是一种氧化还原活性脂质,用作睾丸双官能光合呼吸转移链中的电子转运蛋白。为了检查可能参与蓝藻塑料醌生物合成的基因的作用,我们专注于三个综合症SP。 PCC 6803基因可能编码丙酮酸丙烯酸裂解酶(SLL1797)和两个4-羟基-3-甲苯苯基苯甲酸脱羧酶(SLR1099和SLL0936)。通过用重组蛋白的体外酶测定和通过SengeChocystis Sp的体外酶测定来研究编码蛋白质的功能,并通过与重组蛋白的体外酶测定来研究。单基因敲除突变体。我们的结果表明,SLL1797编码了丙酮酸丙酸盐酶。在各自的敲除突变体中,塑性醌几乎不可检测,并且突变体需要4-羟基苯甲酸酯,以强调酸丙酮酸酶 - 裂解酶的重要性,以在蓝藻中引发塑性醌生物合成。重组SLR1099蛋白质显示脱羧酶活性,并催化在体外用不同戊烯侧链长度的4-羟基-3-苯基苯甲酸酯的脱羧剂。与SLR1099相反,无论使用的条件如何,重组SLL0936蛋白没有显示脱羧酶活性。然而,SNECECHOCYSTIS SP中的SLL0936基因的灭活。然而,使塑性醌含量的急剧降低与SLR1099敲除突变体中确定的那些相似的水平。这证明了不仅是SLR1099,而且还需要SLL0936在蓝藻中的塑性醌合成需要SLL0936。总之,我们的数据表明,Cyanobacteria专门通过在第一反应步骤中的途径产生塑料醌,该途径几乎与大肠杆菌中的泛醌生物合成相同,并转化为4-羟基苯甲酸酯,然后将戊酯和脱羧。

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