Use of a modified Bacteroides-Prevotella shuttle vector to transfer a reconstructed beta-1,4-D-endoglucanase gene into Bacteroides uniformis and Prevotella ruminicola B(1)4.

R G Gardner; J B Russell; D B Wilson; G R Wang; N B Shoemaker

首页> 外文期刊>Applied and Environmental Microbiology >Use of a modified Bacteroides-Prevotella shuttle vector to transfer a reconstructed beta-1,4-D-endoglucanase gene into Bacteroides uniformis and Prevotella ruminicola B(1)4.

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Use of a modified Bacteroides-Prevotella shuttle vector to transfer a reconstructed beta-1,4-D-endoglucanase gene into Bacteroides uniformis and Prevotella ruminicola B(1)4.

机译：使用修饰的拟杆菌-小球藻穿梭载体将重构的β-1,4-D-内葡聚糖酶基因转移到统一拟杆菌和小球藻B（1）4中。

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A carboxymethyl cellulase (CMCase) gene from Prevotella ruminicola B(1)4 was reconstructed by adding a cellulose binding domain from a Thermomonospora fusca cellulase and was conjugally transferred from Escherichia coli to Bacteroides uniformis 0061 by using a chloramphenicol and tetracycline resistance shuttle vector (pTC-COW). pTC-COW was specifically constructed to facilitate conjugal transfer of vectors from B. uniformis donors to P. ruminicola recipients. B. uniformis transconjugants containing CMCase constructs cloned into pTC-COW expressed Cmr, but they did not produce the reconstructed CMCase until a xylanase promoter from P. ruminicola 23 was added upstream of the CMCase (pTC-XRCMC). The xylanase promoter allowed the B. uniformis transconjugants to produce large amounts of the reconstructed CMCase, which was present on the outside surface of the cells. Although the reconstructed CMCase alone did not allow B. uniformis to grow on acid-swollen cellulose, rapid growth was observed when two exocellulases were added to the culture supernatant. Under these conditions, the reconstructed CMCase permitted faster growth than the wild-type CMCase. The frequency of transfer of pTC-XRCMC from B. uniformis to P. ruminicola B(1)4 was increased 100-fold when strictly anaerobic conditions, nitrocelluose filters (cell immobilization), and more stringent selections were employed. Although the P. ruminicola B(1)4 (pTC-XRCMC) transconjugates expressed Tcr and had DNA that hybridized with a probe to the shuttle vector, these transconjugants did not produce detectable levels of the reconstructed CMCase even when xylan was the carbon source. On the basis of these results, it appears that not all of the promoters recognized by B. uniformis and P. ruminicola 23 are functional in P. ruminicola B(1)4. However, the results with B. uniformis suggest that the introduction of a P. ruminicola B(1)4 promoter should allow expression of the reconstructed CMCase in P. ruminicola B(1)4.

机译：通过添加来自单孢单胞菌纤维素酶的纤维素结合域来重建小球藻丙酸杆菌B（1）4的羧甲基纤维素酶（CMCase）基因，并使用氯霉素和四环素抗性穿梭载体（pTC）将其从大肠杆菌中共轭转移至统一细菌0061。 -牛）。 pTC-COW是专门构建的，以利于将载体从统一芽孢杆菌供体向瘤胃假单胞菌接受者的结合转移。含有克隆到pTC-COW中的CMCase构建体的统一芽孢杆菌转导结合体表达了Cmr，但是直到在CMCase上游添加了来自Ruminicola 23的木聚糖酶启动子（pTC-XRCMC），它们才产生重组的CMCase。木聚糖酶启动子允许统一芽孢杆菌转导结合物产生大量的重建的CMCase，其存在于细胞的外表面。尽管仅重建的CMCase不允许统一芽孢杆菌在酸溶胀的纤维素上生长，但在培养上清液中添加了两种外切纤维素酶时，观察到快速生长。在这些条件下，重建的CMCase比野生型CMCase具有更快的生长速度。当严格厌氧条件，硝酸纤维素滤膜（细胞固定化）和更严格的选择条件下使用时，pTC-XRCMC从统一芽孢杆菌向芸苔假单胞菌B（1）4转移的频率增加了100倍。尽管ruminicola B（1）4（pTC-XRCMC）反式共轭物表达Tcr并具有与穿梭载体探针杂交的DNA，但即使木聚糖是碳源，这些反式结合物也无法产生可检测水平的重组CMCase。根据这些结果，似乎并非所有由B.uniformis和P.ruminicola 23识别的启动子都在P. ruminicola B（1）4中起作用。但是，与统一芽孢杆菌的结果表明，引入了一个新的ruminicola B（1）4启动子应该允许在ruminicola B（1）4中表达重建的CMCase。

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《Applied and Environmental Microbiology》 |1996年第1期|共7页
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R G Gardner; J B Russell; D B Wilson; G R Wang; N B Shoemaker;
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1. Construction of Prevotella ruminicola-Escherichia coli Shuttle Vector pRAM45 and Transformation of P. ruminicola Strains by Electroporation [J] . Koretsugu Ogata, Roustam I. Aminov, Kiyoshi Tajima, Journal of Bioscience and Bioengineering . 1999,第3期

机译：金黄色葡萄球菌大肠杆菌穿梭载体pRAM45的构建及电穿孔法转化金黄色葡萄球菌
2. Construction of Prevotella ruminicola-Escherichia coli Shuttle Vector pRAM45 and Transformation of P. ruminicola Strains by Electroporation [J] . Koretsugu Ogata, Roustam I. Aminov, Kiyoshi Tajima, Journal of Bioscience and Bioengineering . 1999,第3期

机译：金黄色葡萄球菌大肠杆菌穿梭载体pRAM45的构建及电穿孔法转化金黄色葡萄球菌
3. A PCR Assay To Discriminate Human and Ruminant Feces on the Basis of Host Differences in Bacteroides-Prevotella Genes Encoding 16S rRNA [J] . Anne E. Bernhard, Katharine G. Field Applied and Environmental Microbiology . 2000,第10期

机译：基于宿主差异的编码16S rRNA的拟杆菌属基因的PCR鉴定人粪和反刍粪便
4. Self-assembly of PEI Modified Biodegradable Complex Micelles as Gene Transfer Vector for Proliferation of ECs [C] . Juan Lv, Jing Yang, Xuefang Hao, European conference on biomaterials . 2014

机译：PEI修饰的可降解复合胶束的自组装作为EC增殖的基因转移载体
5. Use of a modified Bacteroides-Prevotella shuttle vector to transfer a reconstructed beta-14-D-endoglucanase gene into Bacteroides uniformis and Prevotella ruminicola B(1)4. [O] . R G Gardner, J B Russell, D B Wilson, 1996

机译：使用修饰的拟杆菌-小球藻穿梭载体将重构的β-14-D-内葡聚糖酶基因转移到统一拟杆菌和小球藻B（1）4中。
6. Use of a modified Bacteroides-Prevotella shuttle vector to transfer a reconstructed beta-1,4-D-endoglucanase gene into Bacteroides uniformis and Prevotella ruminicola B(1)4 [O] . R G Gardner, J B Russell, D B Wilson, 1996

机译：使用修饰的Bacteroides-Pvototella梭子载体向量将重建的β-1,4-D-内切葡聚糖酶基因转移到Brageodes均匀和FRVotella Ruminicola B（1）4中

Use of a modified Bacteroides-Prevotella shuttle vector to transfer a reconstructed beta-1,4-D-endoglucanase gene into Bacteroides uniformis and Prevotella ruminicola B(1)4.

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