利用重水诱导的拉曼峰进化监测细菌孢子代谢活性。

Rasmus Öberg, Tobias Dahlberg, Dmitry Malyshev, Magnus Andersson
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引用次数: 1

摘要

孢子内形成细菌与食物变质、食物中毒和医院感染有关。因此,监测孢子代谢活性和验证灭菌的方法引起了人们极大的兴趣。然而,目前追踪代谢活动的方法耗时且资源密集。这项工作研究同位素标记和拉曼显微镜作为一个低成本的快速替代。具体来说,我们监测肠毒性蜡样芽孢杆菌孢子在注入d20的肉汤中萌发和细胞分裂的拉曼光谱。在发芽和细胞分裂过程中,水分被代谢,来自肉汤的氘被纳入蛋白质和脂质,导致在2190 cm-1处出现与C-D键相关的拉曼峰。我们发现在37℃孵育2小时后出现了一个显著的C- d峰。此外,我们发现峰值的出现与观察到的第一次细胞分裂一致,表明萌发期间代谢活动很少。最后,在发酵液中添加30%的重水对孢子的萌发和细胞生长速率没有影响。这显示了实时监测从细菌孢子到分裂细胞的代谢活动的潜力。总之,我们的工作提出了跟踪用d20注入的肉汤孵育的孢子中C-D拉曼峰的演变,作为一种有效的、时间和成本效益的方法来监测孢子种群的生长,同时使我们能够跟踪细菌生长和分裂的时间。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Monitoring bacterial spore metabolic activity using heavy water-induced Raman peak evolution.
Endospore-forming bacteria are associated with food spoilage, food poisoning, and infection in hospitals. Therefore, methods to monitor spore metabolic activity and verify sterilization are of great interest. However, current methods for tracking metabolic activity are time-consuming and resource intensive. This work investigates isotope labeling and Raman microscopy as a low-cost rapid alternative. Specifically, we monitor the Raman spectrum of enterotoxic B. cereus spores undergoing germination and cell division in D2O-infused broth. During germination and cell division, water is metabolized and deuterium from the broth is incorporated into proteins and lipids, resulting in the appearance of a Raman peak related to C-D bonds at 2190 cm-1. We find that a significant C-D peak appears after 2 h of incubation at 37 °C. Further, we found that the peak appearance coincides with the observed first cell division indicating little metabolic activity during germination. Lastly, the germination and cell growth rate of spores were not affected by adding 30% heavy water to the broth. This shows the potential for real-time monitoring of metabolic activity from a bacterial spore to a dividing cell. In conclusion, our work proposes tracking the evolution of the C-D Raman peak in spores incubated with D2O-infused broth as an effective and time-, and cost-efficient method to monitor the outgrowth of a spore population, simultaneously allowing us to track for how long the bacteria have grown and divided.
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