Characterization of Escherichia coli men Mutants Defective in Conversion of o-Succinylbenzoate to 1,4-Dihydroxy-2-Naphthoate

Duncan J. Shaw; John R. Guest; Rangaswamy Meganathan; Ronald Bentley

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Characterization of Escherichia coli men Mutants Defective in Conversion of o-Succinylbenzoate to 1,4-Dihydroxy-2-Naphthoate

机译：将大肠杆菌男性突变体的表征转化为1,4-二羟基-2-萘甲酸盐转化为1,4-二羟基-2-萘酸盐

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Four independent menaquinone (vitamin K₂)-deficient mutants of Escherichia coli, blocked in the conversion of o-succinylbenzoate (OSB) to 1,4-dihydroxy-2-naphthoate (DHNA), were found to represent two distinct classes. Enzymatic complementation was observed when a cell-free extract of one mutant was mixed with extracts of any of the remaining three mutants. The missing enzymes in the two classes were identified by in vitro complementation with preparations of OSB-coenzyme A (CoA) synthetase or DHNA synthase isolated from Mycobacterium phlei. Mutants lacking DHNA synthase (and therefore complementing with M. phlei DHNA synthase) were designated menB, and the mutant lacking OSB-CoA synthetase (and therefore complementing with M. phlei OSB-CoA synthetase) was designated menE. The menB mutants produced only the spirodilactone form of OSB when extracts were incubated with [2,3-14C₂]OSB, ATP, and CoA; the OSB was unchanged on incubation with an extract from the menE mutant under these conditions. Experiments with strains lysogenized by a λ men transducing phage (λG68) and transduction studies with phage P1 indicated that the menB and menE genes form part of a cluster of four genes, controlling the early steps in menaquinone biosynthesis, located at 48.5 min in the E. coli linkage map. Evidence was obtained for the clockwise gene order gyrA....-B-D, where the asterisk denotes the uncertain position of menE relative to menC and menB. The transducing phage (λG68) contained functional menB, menC, and menE genes, but only part of the menD gene, and it was designated λ menC B(D).

机译：四个独立的母蛋白（维生素K _{2 ） - 缺乏大肠杆菌的突变体，在 o - 琥珀基苯甲酸乙酸酯（OSB）转化为1，发现4-二羟基-2-萘甲酸盐（DHNA），代表两个不同的课程。当将一个突变体的细胞提取物与任何剩余的三个突变体的提取物混合时，观察到酶促互补。通过与从分枝杆菌分离的OSB-辅酶A（COA）合成酶或DHNA合成酶的制剂的体外互补来鉴定两类中缺失的酶。缺乏DHNA合成酶的突变体（因此与 m键合。粘合剂 meNb ，缺少OSB-COA合成酶的突变体（因此与 M互补。Phlei OSB-CoA合成酶）被指定为 Mene 。当提取物与[2,3- 14 c _{2 ] OSB，ATP和COA;在这些条件下，OSB与来自 Mene 突变体的提取物的孵育保持不变。用λ晶体化菌株的菌株的实验（λm>转换噬菌体（λg68）和噬菌体p1的转导研究表明 meNb 和 mene 基因形成部分四种基因组，控制梅奈醌生物合成中的早期步骤，位于 E中48.5分钟。 COLI 联系地图。用于顺时针基因命令的证据 Gyra ....-BD，其中星号表示相对于 Menc 的不确定位置和 MENB 。转换噬菌体（λg68）含有功能性 meNb，menc 和 mene 基因，但只有部分 mend 基因，并且它被指定为λ Menc B（d）。}} 展开▼

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《Journal of bacteriology》 |1982年第3期|共6页

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Duncan J. Shaw; John R. Guest; Rangaswamy Meganathan; Ronald Bentley;
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1. Characterization of Escherichia coli men Mutants Defective in Conversion of o-Succinylbenzoate to 1,4-Dihydroxy-2-Naphthoate [J] . Duncan J. Shaw, John R. Guest, Rangaswamy Meganathan, Journal of bacteriology . 1982,第3期

机译：将大肠杆菌男性突变体的表征转化为1,4-二羟基-2-萘甲酸盐转化为1,4-二羟基-2-萘酸盐

2. Characterization of Escherichia coli men Mutants Defective in Conversion of o-Succinylbenzoate to 1,4-Dihydroxy-2-Naphthoate [J] . Duncan J. Shaw, John R. Guest, Rangaswamy Meganathan, Journal of bacteriology . 1982,第3期

机译：将大肠杆菌男性突变体的表征转化为1,4-二羟基-2-萘甲酸盐转化为1,4-二羟基-2-萘酸盐

3. Lipoic acid metabolism in Escherichia coli: isolation of null mutants defective in lipoic acid biosynthesis, molecular cloning and characterization of the E. coli lip locus, and identification of the lipoylated protein of the glycine cleavage system. [J] . T J Vanden Boom, K E Reed, J E Cronan Journal of bacteriology . 1991,第20期

机译：大肠杆菌中的硫辛酸代谢：分离在硫辛酸生物合成中无效的无效突变体，大肠杆菌嘴唇基因座的分子克隆和表征，以及鉴定甘氨酸裂解系统的脂酰化蛋白。

4. The Role of Oxygenation on The Attachment of Escherichia Coli rpoS Mutant Under Aerobic Conditions [C] . Nurul Elfiani Paweli, Prayoga Suryadarma, Indana Mardhiati, International Seminar on Chemistry . 2018

机译：氧合对有氧条件下大肠杆菌RPO突变体的作用

5. The regulation of the dsdCXA locus and the characterization of D-cycloserine resistant mutants in Escherichia coli. [D] . Baisa, Gary Alan. 2011

机译：dsdCXA基因座的调控和大肠杆菌中D-环丝氨酸抗性突变体的表征。

6. Characterization of Escherichia coli men Mutants Defective in Conversion of o-Succinylbenzoate to 14-Dihydroxy-2-Naphthoate [O] . Duncan J. Shaw, John R. Guest, Rangaswamy Meganathan, 1982

机译：大肠杆菌男子突变体表征的邻琥珀酸苯甲酸酯转化为14-二羟基-2-萘甲酸酯

7. Lipoic acid metabolism in Escherichia coli: isolation of null mutants defective in lipoic acid biosynthesis, molecular cloning and characterization of the E. coli lip locus, and identification of the lipoylated protein of the glycine cleavage system. [O] . Vanden Boom, T J, Reed, K E, Cronan, J E 1991

机译：大肠杆菌中的硫辛酸代谢：分离在硫辛酸生物合成中有缺陷的无效突变体，大肠埃希菌嘴唇基因座的分子克隆和表征，以及鉴定甘氨酸裂解系统的脂酰化蛋白。

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机译：基于VTvaf17基因治疗DNA载体的基因治疗DNA载体，其携带选自ANG，ANGPT1，VEGFA，FGF1，HIF1α，HGF，SDF1，KLK4，PDGFC，PROK1，PROK2的靶基因以增加这些靶标的表达水平基因，方法的制备和使用，大肠杆菌菌株SCS110-AF / VTvaf17-ANG或大肠杆菌SCS110-AF / VTvaf17-ANGPT1或大肠杆菌SCS110-AF / VTvaf17-VEGFA或大肠杆菌SCS110-AF / VTvaf17-Fichia-SC110 AF /VTvaf17-HIF1α或大肠杆菌SCS110-AF / VTvaf17-HGF或大肠杆菌SCS110-AF / VTvaf17-SDF1或大肠杆菌SCS110-AF / VTvaf17-KLK4或大肠杆菌SCS110-AF / VTviFi10 S1携带基因治疗DNA载体的大肠杆菌SCS110-AF / VTvaf17-PROK2，其制备方法，工业生产基因治疗DNA载体的方法

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Characterization of Escherichia coli men Mutants Defective in Conversion of o-Succinylbenzoate to 1,4-Dihydroxy-2-Naphthoate

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