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使用生物相容性大分子封端剂制备的球形银纳米粒子的抗菌活性:诱导细菌延滞期大大延长的证据。

Antimicrobial activity of spherical silver nanoparticles prepared using a biocompatible macromolecular capping agent: evidence for induction of a greatly prolonged bacterial lag phase.

机构信息

Molecular Characterization of Foodborne Pathogens Research Unit, Eastern Regional Research Center, Agricultural Research Service, U, S, Department of Agriculture, 600 East Mermaid Lane, Wyndmoor, PA 19038 USA.

出版信息

J Nanobiotechnology. 2010 Dec 21;8:34. doi: 10.1186/1477-3155-8-34.

Abstract

BACKGROUND

We have evaluated the antimicrobial properties of Ag-based nanoparticles (Nps) using two solid phase bioassays and found that 10-20 μL of 0.3-3 μM keratin-stabilized Nps (depending on the starting bacterial concentration = CI) completely inhibited the growth of an equivalent volume of ca. 103 to 104 colony forming units per mL (CFU mL-1) Staphylococcus aureus, Salmonella Typhimurium, or Escherichia coli O157:H7 on solid surfaces. Even after one week at 37°C on solid media, no growth was observed. At lower Np concentrations (= [Np]s), visible colonies were observed but they eventually ceased growing.

RESULTS

To further study the physiology of this growth inhibition, we repeated these experiments in liquid phase by observing microbial growth via optical density at 590 nm (OD) at 37°C in the presence of a [Np] = 0 to 10-6 M. To extract various growth parameters we fit all OD[t] data to a common sigmoidal function which provides measures of the beginning and final OD values, a first-order rate constant (k), as well as the time to calculated 1/2-maximal OD (tm) which is a function of CI, k, as well as the microbiological lag time (T).Performing such experiments using a 96-well microtitre plate reader, we found that growth always occurred in solution but tm varied between 7 (controls; CI = 8 × 103 CFU mL-1) and > 20 hrs using either the citrate-([Np] ~ 3 × 10-7 M) or keratin-based ([Np] ~ 10-6 M) Nps and observed that {∂tm/∂ [Np]}citrate ~ 5 × 107 and {∂tm/∂ [Np]}keratin ~ 107 hr·L mol-1. We also found that there was little effect of Nps on S. aureus growth rates which varied only between k = 1.0 and 1.2 hr-1 (1.1 ± 0.075 hr-1). To test the idea that the Nps were changing the initial concentration (CI) of bacteria (i.e., cell death), we performed probabilistic calculations assuming that the perturbations in tm were due to CI alone. We found that such large perturbations in tm could only come about at a CI where the probability of any growth at all was small. This result indicates that much of the Np-induced change in tm was due to a greatly increased T (e.g., from ca. 1 to 15-20 hrs). For the solid phase assays we hypothesize that the bacteria eventually became non-culturable since they were inhibited from undergoing further cell division (T > many days).

CONCLUSION

We propose that the difference between the solid and liquid system relates to the obvious difference in the exposure, or residence, time of the Nps with respect to the bacterial cell membrane inasmuch as when small, Np-inhibited colonies were selected and streaked on fresh (i.e., no Nps present) media, growth proceeded normally: e.g., a small, growth-inhibited colony resulted in a plateful of typical S. aureus colonies when streaked on fresh, solid media.

摘要

背景

我们使用两种固相生物测定法评估了基于银的纳米粒子(Nps)的抗菌性能,发现 10-20μL 的 0.3-3μM 角蛋白稳定的 Nps(取决于起始细菌浓度=CI)完全抑制了相当于体积的约 103 至 104 个菌落形成单位每毫升(CFU mL-1)金黄色葡萄球菌、肠炎沙门氏菌或大肠杆菌 O157:H7 在固体表面上的生长。即使在 37°C 的固体培养基上放置一周,也观察不到任何生长。在较低的 Np 浓度(= [Np]s)下,观察到可见的菌落,但它们最终停止生长。

结果

为了进一步研究这种生长抑制的生理学,我们通过在 37°C 下在存在[Np]=0 至 10-6 M 的情况下通过 590nm 处的光密度(OD)观察微生物生长,在液相中重复了这些实验。为了提取各种生长参数,我们将所有 OD[t]数据拟合到一个常见的 S 形函数中,该函数提供了起始和最终 OD 值、一级速率常数(k)以及计算出的 1/2-最大 OD(tm)的措施,这是 CI、k 以及微生物滞后时间(T)的函数。使用 96 孔微量滴定板读数器进行此类实验,我们发现生长总是在溶液中发生,但 tm 变化范围为 7(对照;CI=8×103 CFU mL-1)至>20 小时,使用柠檬酸([Np]3×10-7 M)或角蛋白基([Np]10-6 M)Nps,观察到{∂tm/∂[Np]}柠檬酸5×107 和 {∂tm/∂[Np]}角蛋白107 hr·L mol-1。我们还发现 Nps 对金黄色葡萄球菌生长速率几乎没有影响,其变化仅在 k=1.0 和 1.2hr-1 之间(1.1±0.075hr-1)。为了测试 Nps 改变细菌初始浓度(CI)的想法(即细胞死亡),我们进行了概率计算,假设 tm 的扰动仅归因于 CI 。我们发现,tm 的如此大的扰动只能在 CI 下发生,在该 CI 下,任何生长的可能性都很小。这一结果表明,tm 中的大部分 Np 诱导变化是由于 T 大大增加(例如,从约 1 到 15-20 小时)。对于固相测定,我们假设细菌最终变得不可培养,因为它们被抑制进一步细胞分裂(T>数天)。

结论

我们提出,固相和液相系统之间的差异与 Nps 相对于细菌细胞膜的暴露或停留时间明显不同,因为当选择小的、受 Np 抑制的菌落并在新鲜(即无 Nps 存在)培养基上划线时,生长正常进行:例如,当在新鲜的固体培养基上划线时,一个小的、受生长抑制的菌落导致了大量典型的金黄色葡萄球菌菌落。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8b82/3224545/05929ac94ec0/1477-3155-8-34-1.jpg

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