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大肠杆菌 K-12(pEGFPluxABCDEamp):一种用于实时分析抗菌剂对细菌的杀伤作用和人补体活性的工具。

Escherichia coli K-12 (pEGFPluxABCDEamp): a tool for analysis of bacterial killing by antibacterial agents and human complement activities on a real-time basis.

机构信息

Department of Biochemistry and Food Chemistry, The University of Turku, Turku, Finland.

出版信息

Luminescence. 2013 Sep-Oct;28(5):771-9. doi: 10.1002/bio.2435. Epub 2012 Nov 6.

DOI:10.1002/bio.2435
PMID:23129448
Abstract

Photorhabdus luminescens luxCDABE genes were integrated into E. coli K-12 using a high copy number plasmid containing modified luxABCDE genes under the control of the powerful Lac promoter. This strain emitted 10 times higher bioluminescence (BL) than P. luminescens. BL production under different growth conditions was studied. In both bacterial strains, the increase in BL signal correlated with the increase in optical density (OD) in a rich growth medium. However, at the logarithmic growth phase, the BL signal was roughly constant. By contrast, in minimal growth media, there was no substantial growth and the BL/cell was approximately five times higher than in the rich medium. The dynamic measurement range of BL was 10(2) -10(7) colony-forming units (CFU) in E. coli and 10(3) -10(7)  CFU in P. luminescens. Because the decrease in the BL signal correlated with the decrease in CFU and OD, i.e. the number of bacterial cells killed, it proved to be very suitable for assessing the antibacterial effects of different antimicrobial agents. Unlike with plate counting, the kinetics of killing can be monitored on a real-time basis using BL measurements. Complement activities in different samples can be estimated using only one serum dilution. The transformed E. coli strain appeared to be superior to P. luminescens in these applications because E. coli was complement sensitive, the detection limit of E. coli was one order lower and the BL-producing system of P. luminescens appeared to be quite unstable.

摘要

发光杆菌 luxCDABE 基因被整合到大肠杆菌 K-12 中,使用含有改良 luxABCDE 基因的高拷贝数质粒,这些基因受强大的 Lac 启动子控制。该菌株的生物发光(BL)比发光杆菌高出 10 倍。研究了不同生长条件下的 BL 产生情况。在两种细菌菌株中,BL 信号的增加与富营养生长培养基中光密度(OD)的增加成正比。然而,在对数生长期,BL 信号大致保持不变。相比之下,在最小生长培养基中,没有实质性的生长,BL/细胞大约是富培养基中的 5 倍。BL 的动态测量范围在大肠杆菌中为 10(2) -10(7) 个菌落形成单位(CFU),在发光杆菌中为 10(3) -10(7) 个 CFU。由于 BL 信号的下降与 CFU 和 OD 的下降相关,即细菌细胞的死亡数量,因此它被证明非常适合评估不同抗菌剂的抗菌效果。与平板计数不同,使用 BL 测量可以实时监测杀伤动力学。仅使用一个血清稀释度就可以估计不同样品中的补体活性。在这些应用中,转化的大肠杆菌菌株似乎优于发光杆菌,因为大肠杆菌对补体敏感,大肠杆菌的检测限低一个数量级,发光杆菌的 BL 产生系统似乎相当不稳定。

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