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Interspecies Social Spreading: Interaction between Two Sessile Soil Bacteria Leads to Emergence of Surface Motility.种间社会传播:两种固着土壤细菌之间的相互作用导致表面能动性的出现。
mSphere. 2019 Jan 30;4(1):e00696-18. doi: 10.1128/mSphere.00696-18.
2
Chromatic Bacteria - A Broad Host-Range Plasmid and Chromosomal Insertion Toolbox for Fluorescent Protein Expression in Bacteria.嗜色细菌——一种用于在细菌中表达荧光蛋白的广泛宿主范围的质粒和染色体插入工具箱。
Front Microbiol. 2018 Dec 12;9:3052. doi: 10.3389/fmicb.2018.03052. eCollection 2018.
3
Phyllosphere microbiology: at the interface between microbial individuals and the plant host.叶片微生物学:在微生物个体与植物宿主之间的界面。
New Phytol. 2018 Jun;218(4):1327-1333. doi: 10.1111/nph.15054. Epub 2018 Mar 5.
4
Complete genome sequence of P3B5, a candidate for microbial phyllo-remediation of hydrocarbon-contaminated sites.P3B5的全基因组序列,一种用于微生物修复烃污染场地的候选菌株。
Stand Genomic Sci. 2016 Sep 26;11:75. doi: 10.1186/s40793-016-0190-6. eCollection 2016.
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Symplasmata are a clonal, conditional, and reversible type of bacterial multicellularity.共生体是一种克隆的、条件的和可逆的细菌多细胞类型。
Sci Rep. 2016 Aug 18;6:31914. doi: 10.1038/srep31914.
6
MiniTn7-transposon delivery vectors for inducible or constitutive fluorescent protein expression in Enterobacteriaceae.用于肠杆菌科中诱导型或组成型荧光蛋白表达的MiniTn7转座子递送载体。
FEMS Microbiol Lett. 2016 Aug;363(16). doi: 10.1093/femsle/fnw178. Epub 2016 Jul 20.
7
A set of versatile brick vectors and promoters for the assembly, expression, and integration of synthetic operons in Methylobacterium extorquens AM1 and other alphaproteobacteria.一组通用的砖型载体和启动子,用于在嗜甲基甲基杆菌AM1和其他α-变形菌中组装、表达和整合合成操纵子。
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Crucial factor for increasing the conjugation frequency in Streptomyces netropsis SD-07 and other strains.提高嗜网链霉菌SD-07及其他菌株中接合频率的关键因素。
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9
Draft Genome Sequence of the Phyllosphere Model Bacterium Pantoea agglomerans 299R.叶际模式细菌成团泛菌299R的基因组序列草图
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10
Quantification of lateral heterogeneity in carbohydrate permeability of isolated plant leaf cuticles.定量分析离体植物叶片角质层中碳水化合物渗透性的横向异质性。
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通过接合作用将“彩色细菌”荧光蛋白标签递送至变形菌门细菌

Delivering "Chromatic Bacteria" Fluorescent Protein Tags to Proteobacteria Using Conjugation.

作者信息

Schlechter Rudolf O, Remus-Emsermann Mitja Np

机构信息

School of Biological Sciences and Biomolecular Interaction Centre, University of Canterbury, Christchurch, New Zealand.

出版信息

Bio Protoc. 2019 Apr 5;9(7):e3199. doi: 10.21769/BioProtoc.3199.

DOI:10.21769/BioProtoc.3199
PMID:33654996
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC7854147/
Abstract

Recently, we published a large and versatile set of plasmids, the chromatic bacteria toolbox, to deliver eight different fluorescent protein genes and four combinations of antibiotic resistance genes to Gram-negative bacteria. Fluorescent tags are important tools for single-cell microbiology, synthetic community studies, biofilm, and host-microbe interaction studies. Using conjugation helper strain S17-1 as a donor, we show how plasmid conjugation can be used to deliver broad host range plasmids, Tn transposons delivery plasmids, and Tn transposon delivery plasmids into species belonging to the Proteobacteria. To that end, donor and recipient bacteria are grown under standard growth conditions before they are mixed and incubated under non-selective conditions. Then, transconjugants or exconjugant recipients are selected on selective media. Mutant colonies are screened using a combination of tools to ensure that the desired plasmids or transposons are present and that the colonies are not containing any surviving donors. Through conjugation, a wide range of Gram-negative bacteria can be modified without prior, often time-consuming, establishment of competent cell and electroporation procedures that need to be adjusted for every individual strain. The here presented protocol is not exclusive for the delivery of Chromatic bacteria plasmids and transposons, but can also be used to deliver other mobilizable plasmids to bacterial recipients.

摘要

最近,我们发表了一组庞大且通用的质粒,即嗜色菌工具箱,用于将八个不同的荧光蛋白基因和四种抗生素抗性基因组合导入革兰氏阴性菌。荧光标签是单细胞微生物学、合成群落研究、生物膜以及宿主-微生物相互作用研究的重要工具。以接合辅助菌株S17-1作为供体,我们展示了如何利用质粒接合将广泛宿主范围的质粒、转座子Tn递送质粒以及转座子Tn递送质粒导入变形菌门的物种。为此,供体菌和受体菌在标准生长条件下培养,然后混合并在非选择性条件下孵育。接着,在选择性培养基上筛选接合子或接合后受体。使用多种工具组合筛选突变菌落,以确保存在所需的质粒或转座子,并且菌落中不含有任何存活的供体菌细胞。通过接合,可以对多种革兰氏阴性菌进行改造,而无需事先建立通常耗时的感受态细胞制备和电穿孔程序,这些程序还需要针对每个单独的菌株进行调整。这里介绍的方案并非仅适用于嗜色菌质粒和转座子的递送,也可用于将其他可移动质粒递送至细菌受体。