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Microbiomes of the dust particles collected from the International Space Station and Spacecraft Assembly Facilities

机译:从国际空间站和航天器装配设施中收集的粉尘颗粒的微生物胶质粒子

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摘要

The International Space Station (ISS) is a unique built environment due to the effects of microgravity, space radiation, elevated carbon dioxide levels, and especially continuous human habitation. Understanding the composition of the ISS microbial community will facilitate further development of safety and maintenance practices. The primary goal of this study was to characterize the viable microbiome of the ISS-built environment. A second objective was to determine if the built environments of Earth-based cleanrooms associated with space exploration are an appropriate model of the ISS environment. Samples collected from the ISS and two cleanrooms at the Jet Propulsion Laboratory (JPL, Pasadena, CA) were analyzed by traditional cultivation, adenosine triphosphate (ATP), and propidium monoazide-quantitative polymerase chain reaction (PMA-qPCR) assays to estimate viable microbial populations. The 16S rRNA gene Illumina iTag sequencing was used to elucidate microbial diversity and explore differences between ISS and cleanroom microbiomes. Statistical analyses showed that members of the phyla Actinobacteria, Firmicutes, and Proteobacteria were dominant in the samples examined but varied in abundance. Actinobacteria were predominant in the ISS samples whereas Proteobacteria, least abundant in the ISS, dominated in the cleanroom samples. The viable bacterial populations seen by PMA treatment were greatly decreased. However, the treatment did not appear to have an effect on the bacterial composition (diversity) associated with each sampling site. The results of this study provide strong evidence that specific human skin-associated microorganisms make a substantial contribution to the ISS microbiome, which is not the case in Earth-based cleanrooms. For example, Corynebacterium and Propionibacterium (Actinobacteria) but not Staphylococcus (Firmicutes) species are dominant on the ISS in terms of viable and total bacterial community composition. The results obtained will facilitate future studies to determine how stable the ISS environment is over time. The present results also demonstrate the value of measuring viable cell diversity and population size at any sampling site. This information can be used to identify sites that can be targeted for more stringent cleaning. Finally, the results will allow comparisons with other built sites and facilitate future improvements on the ISS that will ensure astronaut health.
机译:由于微匍匐,空间辐射,二氧化碳水平,特别是持续的人类居住,国际空间站(ISS)是一种独特的建筑环境。了解ISS微生物群落的组成将有助于进一步发展安全和维护实践。本研究的主要目标是表征可行性环境的可行性微生物组。第二个目标是确定与太空探索相关的地球的洁净室的建筑环境是ISS环境的适当模型。通过传统培养,腺苷三磷酸(ATP)和单氮杂苷 - 定量聚合酶链反应(PMA-QPCR)测定来分析从ISS推进实验室(JPL,帕斯拉迪纳,CA)中的ISS和两种洁净室中的样品进行分析,以估计可行的微生物人口。 16S rRNA基因Illumina Itag测序用于阐明微生物多样性并探讨ISS和洁净室微生物体之间的差异。统计学分析表明,在检测的样品中,Phyla肌动菌,压缩和植物的成员在样品中占优势,但在丰度中变化。肌动菌菌在ISS样本中占主导地位,而噬菌体,在ISS中最少丰富,在洁净室样品中占主导地位。 PMA治疗所见的可行细菌种群大大降低。然而,治疗似乎没有对与每个采样部位相关的细菌组合物(多样性)产生影响。本研究的结果提供了强有力的证据表明,特定人类皮肤相关的微生物对ISS微生物组产生了重大贡献,这并非如此基于地球的洁净室。例如,在可行和总细菌群落组合物方面,棒状杆菌和丙杆菌(抗菌菌)但不是葡萄球菌(Formicsicsoctia)的占主导地位。获得的结果将促进未来的研究,以确定ISS环境随着时间的推移多么稳定。目前的结果还证明了在任何采样部位测量活细胞分集和人口大小的值。此信息可用于识别可以针对更严格清洁的站点。最后,结果将允许与其他建造场所的比较,并促进未来的ISS改进,以确保宇航员健康。

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