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生成与荧光蛋白的染色体定位转录融合体用于丁香假单胞菌的单细胞基因表达分析

Generating Chromosome-Located Transcriptional Fusions to Fluorescent Proteins for Single-Cell Gene Expression Analysis in Pseudomonas syringae.

作者信息

Rufián José S, López-Márquez Diego, López-Pagán Nieves, Grant Murray, Ruiz-Albert Javier, Beuzón Carmen R

机构信息

Dpto. Biología Celular, Genética y Fisiología, Instituto de Hortofruticultura Subtropical y Mediterránea, Universidad de Málaga-Consejo Superior de Investigaciones Científicas (IHSM-UMA-CSIC), Málaga, Spain.

School of Life Sciences, University of Warwick, Conventry, UK.

出版信息

Methods Mol Biol. 2018;1734:183-199. doi: 10.1007/978-1-4939-7604-1_15.

Abstract

The last decade has seen significant effort directed toward the role of phenotypic heterogeneity in bacterial adaptation. Phenotypic heterogeneity usually refers to phenotypic diversity that takes place through nongenetic means, independently of environmental induced variation. Recent findings are changing how microbiologists analyze bacterial behavior, with a shift from traditional assays averaging large populations to single-cell analysis focusing on bacterial individual behavior. Fluorescence-based methods are often used to analyze single-cell gene expression by flow cytometry, fluorescence microscopy and/or microfluidics. Moreover, fluorescence reporters can also be used to establish where and when are the genes of interest expressed. In this chapter, we use the model bacterial plant pathogen Pseudomonas syringae to illustrate a method to generate chromosome-located transcriptional gene fusions to fluorescent reporter genes, without affecting the function of the gene of interest.

摘要

在过去十年中,人们为研究表型异质性在细菌适应性中的作用付出了巨大努力。表型异质性通常是指通过非遗传方式发生的表型多样性,与环境诱导的变异无关。最近的研究结果正在改变微生物学家分析细菌行为的方式,从传统的对大量群体进行平均分析的方法转向专注于细菌个体行为的单细胞分析。基于荧光的方法通常用于通过流式细胞术、荧光显微镜和/或微流控技术分析单细胞基因表达。此外,荧光报告基因还可用于确定感兴趣的基因在何处以及何时表达。在本章中,我们使用模式细菌植物病原菌丁香假单胞菌来说明一种生成与荧光报告基因的染色体定位转录基因融合体的方法,同时不影响感兴趣基因的功能。

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