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A robust and adaptable high throughput screening method to study host-microbiota interactions in the human intestine

机译:一种强大且适应性强的高通量筛选方法,用于研究人肠中宿主-微生物群的相互作用

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摘要

The intestinal microbiota has many beneficial roles for its host. However, the precise mechanisms developed by the microbiota to influence the host intestinal cell responses are only partially known. The complexity of the ecosystem and our inability to culture most of these micro-organisms have led to the development of molecular approaches such as functional metagenomics, i.e. the heterologous expression of a metagenome in order to identify functions. This elegant strategy coupled to high throughput screening allowed to identify novel enzymes from different ecosystems where culture methods have not yet been adapted to isolate the candidate microorganisms. We have proposed to use this functional metagenomic approach in order to model the microbiota's interaction with the host by combining this heterologous expression with intestinal reporter cell lines. The addition of the cellular component to this functional metagenomic approach introduced a second important source of variability resulting in a novel challenge for high throughput screening. First attempts of high throughput screening with various reporter cell-lines showed a high distribution of the response and consequent difficulties to reproduce the response, impairing an easy and clear identification of confirmed hits. In this study, we developed a robust and reproducible methodology to combine these two biological systems for high throughput application. We optimized experimental setups and completed them by appropriate statistical analysis tools allowing the use this innovative approach in a high throughput manner and on a broad range of reporter assays. We herewith present a methodology allowing a high throughput screening combining two biological systems. Therefore ideal conditions for homogeneity, sensitivity and reproducibility of both metagenomic clones as well as reporter cell lines have been identified and validated. We believe that this innovative method will allow the identification of new bioactive microbial molecules and, subsequently, will promote understanding of host-microbiota interactions.
机译:肠道菌群对其宿主具有许多有益的作用。然而,微生物群开发的影响宿主肠道细胞反应的精确机制仅是部分已知的。生态系统的复杂性以及我们无法培养大多数微生物的能力导致了分子方法的发展,例如功能宏基因组学,即为了鉴定功能而进行的元基因组的异源表达。这种巧妙的策略与高通量筛选相结合,可以从不同的生态系统中鉴定出新的酶,在这些生态系统中,尚未采用合适的培养方法来分离候选微生物。我们已经提议使用这种功能性宏基因组学方法,以通过将这种异源表达与肠道报道细胞系结合起来,来模拟微生物群与宿主的相互作用。在这种功能性宏基因组学方法中增加了细胞成分,这引入了可变性的第二个重要来源,从而为高通量筛选带来了新的挑战。首次尝试使用各种报告基因细胞系进行高通量筛选显示了反应的高分布,并因此难以再现反应,从而影响了对已确认点击的轻松,清晰鉴定。在这项研究中,我们开发了一种健壮且可重现的方法,将这两种生物系统结合起来用于高通量应用。我们优化了实验设置,并通过适当的统计分析工具完成了实验设置,从而可以高通量方式和广泛的报告基因检测方法使用这种创新方法。我们在此提出一种方法,可以将两个生物系统结合起来进行高通量筛选。因此,已经鉴定并验证了宏基因组克隆以及报道细胞系的均质性,敏感性和可再现性的理想条件。我们相信,这种创新方法将有助于鉴定新的生物活性微生物分子,并随后将促进对宿主-微生物群相互作用的了解。

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