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使用紫外线技术使甲型肝炎病毒、猫杯状病毒和杜兰病毒在福米卡薄板上失活。

Inactivation of hepatitis A virus, feline calicivirus, and Tulane virus on Formica coupons using ultraviolet light technologies.

作者信息

Corson E, Pendyala B, Patras A, D'Souza D H

机构信息

Department of Food Science, 2600 River Drive, University of Tennessee, Knoxville, TN 37996, USA.

Department of Food and Animal Sciences, Tennessee State University, Nashville, Tennessee 37209, USA.

出版信息

Heliyon. 2024 Jan 28;10(3):e25201. doi: 10.1016/j.heliyon.2024.e25201. eCollection 2024 Feb 15.

Abstract

Contaminated fomites can lead to hepatitis A virus (HAV) and human norovirus (HuNoV) disease outbreaks. Improved decontamination methods that are user-friendly, cost-effective, and waterless are being researched for sustainability. Traditional ultraviolet light (UV-C) technologies though effective for surface decontamination have drawbacks, using mercury lamps, that pose user-safety risk and environmental hazards. Therefore, UV-C light emitting diode (LED) systems are being designed for delivering required antiviral doses. The objective of this research was to determine the ability of UV-C LED (279 nm) systems to inactivate HuNoV surrogates, feline calicivirus (FCV-F9) and Tulane virus (TV), and HAV on Formica coupons in comparison to UV-C (254 nm) systems. FCV-F9 (∼6 log PFU/mL), TV (∼7 log PFU/mL), or HAV (∼6 log PFU/mL) at 100 μL were surface-spread on sterile Formica coupons (3 × 3 cm), air-dried, and treated for up to 2.5 min with both systems. Each experiment was replicated thrice. Recovered infectious plaque counts were statistically analyzed using mixed model analysis of variance. FCV-F9, TV, and HAV showed D values of 23.37 ± 0.91 mJ/cm, 16.32 ± 3.6 mJ/cm, and 12.39 ± 0.70 mJ/cm using 279 nm UV-C LED, respectively and D values of 9.97 ± 2.44 mJ/cm, 6.83 ± 1.13 mJ/cm and 12.40 ± 1.15 mJ/cm, respectively with 254 nm UV-C. Higher 279 nm UV-C LED doses were required to cause HuNoV surrogate reduction than 254 nm UV-C, except similar doses with both systems were needed for HAV inactivation on Formica surfaces. It remains critical to measure UV intensity of optical sources and optimize exposure times for desired log reduction on surfaces.

摘要

受污染的污染物可导致甲型肝炎病毒(HAV)和人诺如病毒(HuNoV)疾病爆发。为实现可持续性,正在研究用户友好、经济高效且无水的改进消毒方法。传统的紫外线(UV-C)技术虽然对表面消毒有效,但使用汞灯存在缺点,会带来用户安全风险和环境危害。因此,正在设计UV-C发光二极管(LED)系统以提供所需的抗病毒剂量。本研究的目的是确定与UV-C(254nm)系统相比,UV-C LED(279nm)系统对福米卡样板上的HuNoV替代物猫杯状病毒(FCV-F9)、图兰病毒(TV)和HAV的灭活能力。将100μL的FCV-F9(约6 log PFU/mL)、TV(约7 log PFU/mL)或HAV(约6 log PFU/mL)表面涂抹在无菌福米卡样板(3×3cm)上,风干,然后用这两种系统处理长达2.5分钟。每个实验重复三次。使用混合方差分析对回收的感染性噬斑计数进行统计分析。使用279nm UV-C LED时,FCV-F9、TV和HAV的D值分别为23.37±0.91mJ/cm、16.32±3.6mJ/cm和12.39±0.70mJ/cm,使用254nm UV-C时,D值分别为9.97±2.44mJ/cm、6.83±1.13mJ/cm和12.40±1.15mJ/cm。除了在福米卡表面灭活HAV需要两种系统使用相似剂量外,导致HuNoV替代物减少所需的279nm UV-C LED剂量高于254nm UV-C。测量光源的紫外线强度并优化表面达到所需对数减少所需的暴露时间仍然至关重要。

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