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Capture of a catabolic plasmid that encodes only 24-dichlorophenoxyacetic acid:alpha-ketoglutaric acid dioxygenase (TfdA) by genetic complementation.

机译：通过遗传互补捕获仅编码24-二氯苯氧基乙酸：α-酮戊二酸双加氧酶（TfdA）的分解代谢质粒。

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摘要

The modular pathway for the metabolism of 2,4-dichlorophenoxyacetic acid (2,4-D) encoded on plasmid pJP4 of Alcaligenes eutrophus JMP134 appears to be an example in which two genes, tfdA and tfdB, have been recruited during the evolution of a catabolic pathway. The products of these genes act to convert 2,4-D to a chloro-substituted catechol that can be further metabolized by enzymes of a modified ortho-cleavage pathway encoded by tfdCDEF. Given that modified ortho-cleavage pathways are comparatively common and widely distributed among bacteria, we sought to determine if microbial populations in soil carry tfdA on plasmid vectors that lack tfdCDEF or tfdB. To capture such plasmids from soil populations, we used a recipient strain of A. eutrophus that was rifampin resistant and carried a derivative of plasmid pJP4 (called pBH501aE) in which the tfdA had been deleted. Upon mating with mixed bacterial populations from soil treated with 2,4-D, transconjugants that were resistant to rifampin yet able to grow on 2,4-D were obtained. Among the transconjugants obtained were clones that contained a ca. 75-kb plasmid, pEMT8. Bacterial hosts that carried this plasmid in addition to pBH501aE metabolized 2,4-D, whereas strains with only pEMT8 did not. Southern hybridization showed that pEMT8 encoded a gene with a low level of similarity to the tfdA gene from plasmid pJP4. Using oligonucleotide primers based on known tfdA sequences, we amplified a 330-bp fragment of the gene and determined that it was 77% similar to the tfdA gene of plasmid pJP4 and 94% similar to tfdA from Burkholderia sp. strain RASC. Plasmid pEMT8 lacked genes that exhibited significant levels of homology to tfdB and tfdCDEF. Moreover, cell extracts from A. eutrophus(pEMT8) cultures did not exhibit TfdB, TfdC, TfdD, and TfdE activities, whereas cell extracts from A. eutrophus(pEMT8)(pBH501aE) cultures did. These data suggest that pEMT8 encodes only tfdA and that this gene can effectively complement the tfdA deletion mutation of pBH501aE.

机译：真人拟南芥JMP134质粒pJP4上编码的2,4-二氯苯氧基乙酸（2,4-D）代谢的模块化途径似乎是一个例子，其中在拟南芥进化过程中募集了两个基因tfdA和tfdB。分解代谢途径。这些基因的产物将2，4-D转化为氯取代的邻苯二酚，后者可以被tfdCDEF编码的修饰的邻位裂解途径的酶进一步代谢。鉴于修饰的邻位裂解途径相对普遍并且在细菌中广泛分布，我们试图确定土壤中的微生物种群是否在缺乏tfdCDEF或tfdB的质粒载体上携带tfdA。为了从土壤种群中捕获此类质粒，我们使用了对利福平具有抗性且含有tpdA缺失的质粒pJP4衍生物（称为pBH501aE）的嗜碱曲霉的受体菌株。与来自用2,4-D处理过的土壤中的混合细菌种群交配后，获得了对利福平具有抗性但能够在2,4-D上生长的转缀合剂。在所获得的转缀合剂中是含有约10％的克隆。 75 kb质粒，pEMT8。除pBH501aE外，携带该质粒的细菌宿主代谢了2,4-D，而仅带有pEMT8的菌株则没有。 Southern杂交表明，pEMT8编码的基因与质粒pJP4的tfdA基因的相似性较低。使用基于已知tfdA序列的寡核苷酸引物，我们扩增了该基因的330 bp片段，并确定与质粒pJP4的tfdA基因有77％的相似性，与Burkholderia sp。的tfdA有94％的相似性。 RASC菌株。质粒pEMT8缺乏与tfdB和tfdCDEF表现出显着水平同源性的基因。此外，从嗜碱曲霉（pEMT8）培养物的细胞提取物不表现出TfdB，TfdC，TfdD和TfdE活性，而从嗜碱曲霉（pEMT8）（pBH501aE）培养物的细胞提取物却表现出TfdB，TfdC，TfdD和TfdE活性。这些数据表明pEMT8仅编码tfdA，并且该基因可以有效地补充pBH501aE的tfdA缺失突变。

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期刊名称 Applied and Environmental Microbiology
作者
E M Top; O V Maltseva; L J Forney;
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年(卷),期 1996(62),7
年度 1996
页码 2470–2476
总页数 7
原文格式 PDF
正文语种
中图分类应用微生物学;微生物学;
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专利

1. Capture of a catabolic plasmid that encodes only 2,4-dichlorophenoxyacetic acid:alpha-ketoglutaric acid dioxygenase (TfdA) by genetic complementation. [J] . E M Top, O V Maltseva, L J Forney Applied and Environmental Microbiology . 1996,第7期

机译：通过遗传互补捕获仅编码2,4-二氯苯氧基乙酸：α-酮戊二酸双加氧酶（TfdA）的分解代谢质粒。
2. Enhanced degradation of phenoxyacetic acid in soil by horizontal transfer of the tfdA gene encoding a 2,4-dichlorophenoxyacetic acid dioxygenase [J] . de Lipthay JR., Sorensen SJ., Barkay T. FEMS Microbiology Ecology . 2001,第1期

机译：通过水平转移编码2,4-二氯苯氧乙酸双加氧酶的tfdA基因，可增强土壤中苯氧乙酸的降解
3. Utilization of phenoxyacetic acid, by strains using either the ortho or meta cleavage of catechol during phenol degradation, after conjugal transfer of tfdA, the gene encoding a 2,4-dichlorophenoxyacetic acid/2-oxoglutarate dioxygenase [J] . J. Radonti de Lipthay, T. Barkay, J. Vekova, Applied Microbiology and Biotechnology . 1999,第2期

机译：在结合转移tfdA后，利用苯酚降解过程中邻苯二酚的邻位或间位裂解菌株对苯氧乙酸的利用，该基因编码2,4-二氯苯氧乙酸/ 2-氧戊二酸双加氧酶
4. POLY(D,L-LACTIC ACID) ENHANCES IMMUNE RESPONSES TO LIPOSOMAL DNA ENCODED ANTIGEN: MULTICOMPONENT PLASMID DNA DELIVERY SYSTEMS [C] . V. Bramwell, J. Eyles, S. Somavarapu, International symposium on controlled release of bioactive materials;Consumer diversified products conference . 2001

机译：聚（D，L-乳酸）增强了对脂质体DNA编码抗原的免疫反应：多组分质粒DNA递送系统
5. Synthesis of unnatural amino acids for genetic encoding by the pyrrolysyltRNA/ RNA synthetase system [D] . Knight, William Arthur 2015

机译：焦磷酸RNA / RNA合成酶系统合成非天然氨基酸用于遗传编码
6. Root Nodule Bradyrhizobium spp. Harbor tfdAα and cadA Homologous with Genes Encoding 24-Dichlorophenoxyacetic Acid-Degrading Proteins [O] . Kazuhito Itoh, Yoshiko Tashiro, Kazuko Uobe, 2004

机译：根瘤状根瘤菌属。港口tfdAα和cadA与编码24-二氯苯氧基乙酸降解蛋白的基因同源
7. Abundance of Novel and Diverse tfdA-Like Genes, Encoding Putative Phenoxyalkanoic Acid Herbicide-Degrading Dioxygenases, in Soil▿ † [O] . Zaprasis, Adrienne, Liu, Ya-Jun, Liu, Shuang-Jiang, 2009

机译：土壤中大量新颖的tfdA样基因，编码假定的苯氧基链烷酸除草剂降解双加氧酶▿†
8. Cloning and Characterization of tfdS, the Repressor-Activator Gene of tfdB, fromthe 2,4-Dichlorophenoxyacetic Acid Catabolic Plasmid pJP4 [R] . Kaphammer, B., Olsen, R. H. 1990

机译：2,4-二氯苯氧乙酸分解代谢质粒pJp4的tfdB阻遏活化基因tfds的克隆与鉴定

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