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迷你Tn7转座子在沙门氏菌疫苗株选定染色体位点的多拷贝整合。

Multicopy integration of mini-Tn7 transposons into selected chromosomal sites of a Salmonella vaccine strain.

作者信息

Roos Karen, Werner Esther, Loessner Holger

机构信息

Bacterial Vaccines and Immune Sera, Department of Veterinary Medicine, Paul Ehrlich Institute, Langen, 63225, Germany.

出版信息

Microb Biotechnol. 2015 Jan;8(1):177-87. doi: 10.1111/1751-7915.12187. Epub 2014 Dec 9.

Abstract

Chromosomal integration of expression modules for transgenes is an important aspect for the development of novel Salmonella vectors. Mini-Tn7 transposons have been used for the insertion of one such module into the chromosomal site attTn7, present only once in most Gram-negative bacteria. However, integration of multiple mini-Tn7 copies might be suitable for expression of appropriate amounts of antigen or combination of different modules. Here we demonstrate that integration of a 9.6 kb mini-Tn7 harbouring the luciferase luxCDABE (lux) occurs at the natural attTn7 site and simultaneously other locations of the Salmonella chromosome, which were engineered using λ-Red recombinase to contain one or two additional artificial attTn7 sites (a-attTn7). Multicopy integration even at closely spaced attTn7 sites was unexpected in light of the previously reported distance-dependent Tn7 target immunity. Integration of multiple copies of a mini-Tn7 containing a gfp cassette resulted in increasing green fluorescence of bacteria. Stable consecutive integration of two mini-Tn7 encoding lacZ and lux was achieved by initial transposition of lacZ-mini-Tn7, subsequent chromosomal insertion of a-attTn7 and a second round of transposition with lux-mini-Tn7. Mini-Tn7 thus constitutes a versatile method for multicopy integration of expression cassettes into the chromosome of Salmonella and possibly other bacteria.

摘要

转基因表达模块的染色体整合是新型沙门氏菌载体开发的一个重要方面。Mini-Tn7转座子已被用于将一个这样的模块插入染色体位点attTn7,该位点在大多数革兰氏阴性细菌中仅出现一次。然而,多个Mini-Tn7拷贝的整合可能适合于表达适量的抗原或不同模块的组合。在这里,我们证明了携带荧光素酶luxCDABE(lux)的9.6 kb Mini-Tn7在天然attTn7位点发生整合,同时也在沙门氏菌染色体的其他位置发生整合,这些位置是利用λ-Red重组酶构建的,含有一个或两个额外的人工attTn7位点(a-attTn7)。鉴于先前报道的距离依赖性Tn7靶标免疫,即使在紧密间隔的attTn7位点进行多拷贝整合也是出乎意料的。含有gfp盒的Mini-Tn7多拷贝整合导致细菌绿色荧光增加。通过lacZ-Mini-Tn7的初始转座、随后a-attTn7的染色体插入以及lux-Mini-Tn7的第二轮转座,实现了编码lacZ和lux的两个Mini-Tn7的稳定连续整合。因此,Mini-Tn7构成了一种将表达盒多拷贝整合到沙门氏菌及可能其他细菌染色体中的通用方法。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f403/4321384/8b51e715f3c7/mbt20008-0177-f1.jpg

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