Inactivation of avian influenza virus using common detergents and chemicals

Six disinfectant chemicals were tested individually for effectiveness against low pathogenic avian influenza virus (LPAIV) A/H7N2/Chick/MinhMa/04. The tested agents included acetic acid (C2H4O2), citric acid (C6H8O7), calcium hypochlorite (Ca(ClO)2), sodium hypochlorite (NaOCl), a powdered laundry detergent with peroxygen (bleach), and a commercially available iodine/acid disinfectant. Four of the six chemicals, including acetic acid (5%), citric acid (1% and 3%), calcium hypochlorite (750 ppm), and sodium hypochlorite (750 ppm) effectively inactivated LPAIV on hard and nonporous surfaces. The conventional laundry detergent was tested at multiple concentrations and found to be suitable for inactivating LPAIV on hard and nonporous surfaces at 6 g/L. Only citric acid and commercially available iodine/acid disinfectant were found to be effective at inactivating LPAIV on both porous and nonporous surfaces.     

七类消毒剂对非洲猪瘟病毒荧光定量PCR检测结果的影响

为评价戊二醛、酚、含碘类等常用消毒剂消毒后对非洲猪瘟病毒荧光定量PCR检测结果的影响,基于畜禽栏舍、运载工具、器具消毒及皮肤黏膜消毒目的,按消毒剂说明书推荐选择不同工作浓度,分别与不同滴度的非洲猪瘟病毒培养物于20℃条件下作用30 min后,采用荧光定量PCR方法检测作用后产物。结果显示,与对应的阳性对照组相比,含氯类(二氯异氰尿酸钠)、过硫酸氢钾类、二氧化氯类消毒剂,消毒后对荧光定量PCR检测结果影响最显著,检测Ct值显著上升或检测不到;戊二醛类、含碘类(主要成分聚维酮碘)消毒剂,核酸降解能力相对较弱,检测Ct值稍有上升;酚类、季铵盐类、含碘类(主要成分碘、磷酸、硫酸)类消毒剂,检测Ct值基本无变化。本研究评价了7类常用消毒剂消毒对非洲猪瘟病毒荧光定量PCR检测结果的影响,可为防控实践中科学、客观评价分析消毒效果提供技术参考。     

Effects of chlorine, iodine, and quaternary ammonium compound disinfectants on several exotic disease viruses

The effects of three representative disinfectants, chlorine (sodium hypochlorite), iodine (potassium tetraglicine triiodide), and quaternary ammonium compound (didecyldimethylammonium chloride), on several exotic disease viruses were examined. The viruses used were four enveloped viruses (vesicular stomatitis virus, African swine fever virus, equine viral arteritis virus, and porcine reproductive and respiratory syndrome virus) and two non-enveloped viruses (swine vesicular disease virus (SVDV) and African horse sickness virus (AHSV)). Chlorine was effective against all viruses except SVDV at concentrations of 0.03% to 0.0075%, and a dose response was observed. Iodine was very effective against all viruses at concentrations of 0.015% to 0.0075%, but a dose response was not observed. Quaternary ammonium compound was very effective in low concentration of 0.003% against four enveloped viruses and AHSV, but it was only effective against SVDV with 0.05% NaOH. Electron microscopic observation revealed the probable mechanism of each disinfectant. Chlorine caused complete degeneration of the viral particles and also destroyed the nucleic acid of the viruses. Iodine destroyed mainly the inner components including nucleic acid of the viruses. Quaternary ammonium compound induced detachment of the envelope of the enveloped viruses and formation of micelle in non-enveloped viruses. According to these results, chlorine and iodine disinfectants were quite effective against most of the viruses used at adequately high concentration. The effective concentration of quaternary ammonium compound was the lowest among the disinfectants examined.     

Inactivation of equine infectious anemia virus by chemical disinfectants.

Twelve chemicals and commercial disinfectants were tested for inactivation of equine infectious anemia virus. In the presence of 10% bovine serum, all chemicals inactivated 4 log10 (based on 0.1 ml) of the virus within 5 minutes at 23 C. A reduction of at least 4 log10 was observed when the virus was exposed for 1 minute to substituted phenolic disinfectants (3 commercial preparations and sodium orthophenylphenate), halogen derivatives (iodophor and sodium hypochlorite), chlorhexidine, and 70% ethanol. Sodium hydroxide (5%), 2% formalin, and 2% glutaraldehyde were slower to inactivate the virus, but achieved 4 log10 reduction in titer by 5 minutes' contact time. The susceptibility of the equine infectious anemia virus to chemical disinfectants is similar to that of other enveloped viruses.     

三类常用消毒剂对非洲猪瘟病毒灭活效果的评价

为评价戊二醛类、酚类、含氯类常用消毒剂对非洲猪瘟病毒(ASFV)的灭活效果,参考OIE参考实验室相关操作流程,基于畜禽栏舍、运载工具、器具消毒目的,根据说明书标明的浓度范围选择低、中、高3个工作浓度,与ASFV分别在4℃和20℃条件下作用30 min,10倍连续稀释后接种猪肺泡巨噬细胞,同时加入猪红细胞,培养观察红细胞...     

常见消毒剂对塞内卡病毒杀灭作用的比较研究

为比较常见消毒方法对塞内卡病毒的杀灭作用,开展了不同浓度苯酚溶液、复方甲酚皂消毒液、柠檬酸溶液、NaOH溶液、百毒杀消毒液、新洁尔灭消毒液、84消毒液以及75％酒精和紫外线,与SVA作用10 min、30 min和60 min杀灭效果的研究.结果显示,5.0％的苯酚溶液作用10 min,0.5％以上的NaOH作用10 ...     

Virucidal disinfectants and feline viruses

Thirty-five commonly used commercial disinfectants (disinfectants, antiseptics, sanitizers, and detergents) were evaluated for their virucidal activity against three feline viruses; feline viral rhinotracheitis virus (a herpesvirus), feline calicivirus, and feline panleukopenia virus (a parvovirus). Disinfectants were diluted as recommended by the manufacturer and were reacted with virus for 10 minutes at room temperature. Viruses were separated from disinfectants by gel filtration in special centrifuge tubes, and were assayed for infectivity in feline cell cultures. All 22 products tested were virucidal for feline viral rhinotracheitis virus, 11 of 35 were virucidal for feline calicivirus, but only 3 of 27 tested were effective against feline panleukopenia virus. A 0.175% sodium hypochlorite solution was the most effective and practical broad-spectrum virucidal product used alone or in combination with other disinfectants/detergents.     

复方煤焦油酸溶液对口蹄疫病毒杀灭效果试验

皮下注射经复方煤焦油酸溶液灭活后的O型口蹄疫乳鼠组织毒(LD50=1×10-8.0)感染4日龄乳鼠,通过ELISA试验考察复方煤焦油酸溶液对O型口蹄疫乳鼠组织毒的杀灭效果。结果显示,复方煤焦油酸溶液1∶600倍稀释液在室温条件下作用30 min,能100%杀灭口蹄疫强毒,可用于口蹄疫病毒污染的动物栏舍、运载工具、环境等的消毒,在杀灭病毒、安全性等方面与国外同类产品相当。     

Evaluation of virucidal activity of three commercial disinfectants and formic acid using bovine enterovirus type 1 (ECBO virus), mammalian orthoreovirus type 1 and bovine adenovirus type 1

A modified version of the test method of the Comité Européen de Normalisation (CEN) was developed using formic acid and three commercial disinfectants to evaluate virucidal activity against three non-enveloped viruses, bovine enterovirus type 1 (ECBO virus), mammalian orthoreovirus type 1 and bovine adenovirus type 1 (BAV 1). Determination of the effects of temperature was carried out at 20 and 10 degrees C. All tests with protein load used bovine serum albumin (BSA) and yeast extract. The investigations were performed in suspension tests and in carrier tests using poplar wood virus carriers. The carrier tests showed that ECBO virus could be inactivated at 20 degrees C with 1% formic acid within a 60 min reaction time. For disinfection of ECBO virus at 10 degrees C within 60 min, a 2% concentration of formic acid was necessary. Formic acid was ineffective against reovirus and bovine adenovirus and cannot be recommended as a reference disinfectant. Inactivation of ECBO virus and adenovirus type 1 using a disinfectant containing aldehydes and alcohols could be achieved, but only at room temperature. The disinfection of reovirus type 1 at room temperature with this product was possible without a protein load. This disinfectant exhibited disinfection ability at 10 degrees C at a concentration of more than 2% or with a longer exposure time. A disinfectant containing aldehydes was effective at room temperature but its effect was reduced in the presence of organic matter. Inactivation at 10 degrees C was found only against adenovirus. The fourth disinfectant, which contained peroxiacetic acid, inactivated all test viruses at a concentration of 0.5% within 15 min independent of temperature and protein load.     

Substitution of vaccinia virus Elstree by modified vaccinia virus Ankara to test the virucidal efficacy of chemical disinfectants

After the eradication of variola in 1980, the smallpox vaccination was considered to be no longer required and was subsequently abandoned mainly because of possible adverse effects of vaccinia virus especially in first‐time vaccinees. Despite a growing number of humans without immunity against vaccinia virus, vaccinia virus Lister Elstree (VACV) is still prescribed for testing virucidal efficacy of chemical disinfectants in the guidelines of the German Veterinary Medical Society [Deutsche Veterinärmedizinische Gesellschaft (DVG)], the German Association for the Control of Virus Diseases [Deutsche Vereinigung zur Bekämpfung der Viruskrankheiten (DVV)] and the Robert Koch Institute (RKI). To evaluate a possible substitution of VACV, with the attenuated modified vaccinia virus Ankara (MVA) the virucidal efficacy of four different DVG‐listed commercially available chemical disinfectants representing different groups of chemicals was tested against these two viruses. Quantitative suspension tests and qualitative carrier tests with poplar wood and gauze were performed. Distinction of VACV and MVA was confirmed by cytopathogenic effects, such as differences in plaque morphology. No significant difference in disinfection efficacy between VACV and MVA was observed for any of the disinfectants tested. Implying that vaccinia virus poses a risk after inadvertent inoculation, our results show that MVA, which does not replicate in humans, should replace VACV in the chemical disinfectant testing guidelines.     

Investigations on suitability of different materials for carriers to be used for virucidal testing of chemical disinfectants in the veterinary field

Various materials with rough surfaces were tested to determine their suitability for virus carrier tests designed to evaluate virucidal activity of chemical disinfectants. A non-enveloped RNA virus, bovine enterovirus type 1, strain LCR 4 [entero cytopathogenic bovine orphan virus (ECBO)] and an enveloped RNA virus, paramyxovirus type 1 [Newcastle disease virus (NDV), strain Montana] served as test viruses. Experiments with ECBO virus were carried out in four sets, and those with NDV in three sets. In the first set we used poplar wood, frosted glass slides and Sartorius membrane filters. The second set comprised of poplar wood, frosted glass slides, polyamide filters, and cellulose nitrate filters and, in the third set, glass fibre filters and glass fibre pre-filters were added. The fourth test included poplar wood, frosted glass slides, and polyethersulphone ultra filters. Because of their extremely low levels of virus recovery, glass, polyamide, cellulose nitrate and glass fibre filter, glass fibre pre-filter, and polyethersulphone ultra filters are not suitable for sufficient recovery of ECBO virus. Only poplar wood carriers allowed sufficient recovery rates of ECBO virus. In the first and second set of tests, NDV could be sufficiently recovered from poplar wood, glass slides, and polyamide filter. In the third set, the virus recovery from polyamide filter was very low. Poplar wood carrier is recommended as a reliable carrier for the tests with both viruses, but methods for virus recovery must be improved, e.g. by more vigorous and longer shaking or optimizing the ultrasonic treatment.     

Virucidal efficacy of four new disinfectants

Virucidal efficacy was evaluated for four recently available disinfectants: chlorine dioxide, potassium peroxymonosulfate, a quaternary ammonium compound, and citricidal (grapefruit extract). Sodium hypochlorite (3%) and tap water were used as positive and negative controls respectively. Feline herpesvirus, feline calicivirus, and feline parvovirus were exposed to the manufacturers' recommended dilutions of the evaluated disinfectants. Both chlorine dioxide and potassium peroxymonosulfate completely inactivated the three viruses used in this study. These disinfectants can aid in controlling nosocomial transmission of viruses with less of the deleterious effects of sodium hypochlorite. The quaternary ammonium compound evaluated in this study and citricidal were not effective against feline calicivirus and feline parvovirus.     

Virucidal efficacy of nine commercial disinfectants against porcine circovirus type 2

A number of commercially available disinfectants are commonly used on pig breeding farms and are authorised by the French Agricultural Ministry. However, the efficacy of these disinfectants is unknown with regard to the emergent porcine circovirus type 2 (PCV2). The virucidal efficacy of nine disinfectants was evaluated by testing a suspension of PCV2 isolated in France. The assays were performed at 20 degrees C and the efficacy determined after 30 min contact time between virus and disinfectant. After this time, the mixture was passed through a detoxification column and then diluted to remove compounds toxic to the virus and the porcine kidney cell line. The filtrate was serially diluted and inoculated onto cell culture. The infectivity of PCV2 was determined by an immunoperoxidase monolayer assay. No reduction in PCV2 titre was demonstrated with iodine and phenolic products. Significant PCV2 titre reductions (1.61 log(10)) were noted for the seven other products. For five disinfectants, namely a product composed of potassium monopersulfate, two products comprising a quaternary ammonium with one or three aldehyde(s), sodium hypochlorite, and sodium hydroxide, the concentration that significantly reduced the PCV2 titre was equal or 1.5-4 times lower than the authorised use concentration. Only two disinfectants, one composed of potassium monopersulfate, the other containing peracetic acid with hydrogen peroxide, reduced the PCV2 titre with a product concentration at best equal or two times higher than the authorised use concentration.     

Stability and inactivation of vesicular stomatitis virus,a prototype rhabdovirus

Viruses may remain infectious outside the host cell for considerable time and represent a source of accidental infection if not properly inactivated. In this study, the survival of vesicular stomatitis virus (VSV) in suspension and dried on surfaces was analyzed. In addition, the sensitivity of VSV to disinfectants and physicochemical changes was investigated. VSV showed a notable stability in suspension at 4 °C with virus titers remaining high over several weeks. The presence of serum proteins had a stabilizing effect on virus infectivity, whereas elevated temperatures reduced survival times. VSV dried on polystyrene, glass or stainless steel surfaces remained infectious for at least 6 days at ambient temperature. VSV showed a remarkable resistance to extreme pH in particular in the alkaline range, but could be rapidly inactivated by heating at 55 °C or higher. The virus was highly sensitive to inactivation by commonly used disinfectants such as aldehydes, alcohols, and detergents. The high stability of VSV on surfaces and in suspension may facilitate dissemination of the virus in livestock by contaminated feeding and water troughs, hands, and milking equipment. This knowledge on the sensitivity of VSV to disinfectants will help to set up appropriate hygiene measures.     

Laboratory evaluation of selected disinfectants as virucidal agents against porcine parvovirus, pseudorabies virus, and transmissible gastroenteritis virus

Of a variety of disinfectants evaluated, only sodium hypochlorite and sodium hydroxide inactivated porcine parvovirus (PPV) after a 5-minute incubation period. After the same incubation time, pseudorabies and transmissible gastroenteritis viruses were inactivated by all of the disinfectants tested. When the incubation time was increased to 20 minutes, 2% glutaraldehyde and a double-strength concentration of a commercial formaldehyde preparation also inactivated PPV. Formaldehyde vapor and ultraviolet radiations inactivated PPV also, but relatively long exposure times were required.     

Evaluation of chemical disinfectants for aleutian disease virus of mink

Nine chemicals and commercial disinfectants were tested for inactivation of Aleutian disease virus of mink. In the presence of distilled water, a commercial disinfectant (O-Syl), halogen derivatives (iodophor and sodium hypochlorite), and glutaraldehyde (2.0%) inactivated 4 log10 (based on 0.25 ml) of the virus within 10 minutes at 23 C. Formalin (2.0%) and O-Syl were slower to inactivate the virus, but achieved a 4 log10 reduction in titer by 30 minutes' contact time. In the presence of 10% bovine serum, formalin (1.0%), O-Syl, and sodium hydroxide (0.5%) achieved a 4 log10 reduction within 10 minutes. All agents tested had some virucidal effect.     

Inactivation of canine parvovirus by disinfectants and heat

The resistance of canine parvovirus (CPV) to inactivation by chemical and thermal means was investigated. CPV with and without extraneous protein was tested against 15 commonly used disinfectants at room temperature. The titres of CPV remaining after 5 minutes disinfection time were greater than or equal to those remaining after 30 minutes regardless of the presence or absence of protein. Disinfection of CPV was accomplished more quickly and at lower concentrations of disinfectants when extraneous protein was absent. Halogen compounds, aldehydes and sodium hydroxide were the most acceptable CPV disinfectants. The presence of protein interfered with the two most frequently recommended CPV disinfectants—sodium hypo-chlorite and formaldehyde. The resistance of CPV to inactivation by heat depended on the temperature and the duration of heating. Boiling (100°C) rapidly inactivated CPV. The virus was more resistant to lower temperatures. Detectable infectivity remained after 7 hours at 80°C and 72 hours at 56°C. At both 37°C and room temperature there was no significant change in infectivity titres over 72 hours.     

Virucidal efficacy of acidic electrolyzed water (AEW) against African swine fever virus and avian influenza virus

This study evaluated the virucidal efficacy of acidic electrolyzed water (AEW) against African swine fever virus (ASFV) and avian influenza virus (AIV), according to the Animal and Plant Quarantine Agency (APQA) guidelines for efficacy testing of veterinary disinfectants. AEW (pH 5.0–6.5) was prepared using a commercially available “Electrolyzed Water Generator” with a free chlorine concentration (FCC) of 5–140 ppm, and its efficiency in reducing the titer of ASFV and AIV was tested in a suspension under low- and high-level organic soiling. Under low-level organic soiling conditions, AEW with FCC ≥40 ppm was effective against ASFV; under high-level organic soiling conditions, AEW with FCC ≥80 ppm was effective against ASFV. Under low-level organic soiling conditions, AEW with FCC ≥60 ppm was effective against AIV; under high-level organic soiling conditions, AEW with FCC ≥100 ppm was effective against AIV. The virucidal effect of AEW seemed dependent on the FCC and the presence of organic soiling. Based on these data, we recommend the following minimum FCCs in AEW treatment for routine disinfection in veterinary field under low- and high-level organic soiling conditions: for ASFV, 50 ppm and 100 ppm; and for AIV, 75 ppm and 125 ppm, respectively. In conclusion, the virucidal effects of AEW against ASFV and AIV emphasize its potential utility as a disinfectant, and we suggest considering organic soiling conditions while using AEW for implementing effective control measures for field applications.     

The survival of some air-borne animal viruses in relation to relative humidity

The influence of relative humidity (R.H.) on the survival of the following viruses has been examined; feline herpesvirus (FHV); feline calicivirus (FCV); vesicular exanthema virus (VEV); infectious bovine rhinotracheitis virus (IBRV); parainfluenza 3 virus (PI-3 virus); vesicular stomatitis virus (VSV); equine herpesvirus type 1 (EHV-1), equine arteritis virus (EAV); equine rhinovirus (ERV-1), and African swine fever virus (ASFV). ASFV and PI-3 viruses survived well at all relative humidities when sampled 1 s after formation of an aerosol, but after storage of aerosols for 5 min both viruses were found to be sensitive to high R.H. The other lipid-containing viruses (EAV, VSV, FHV, EHV-1 and IBRV) were unstable when stored as aerosols in moist conditions. The picornavirus ERV-1 was the only virus which survived well at high R.H. but poorly on exposure to dry conditions. The caliciviruses VEV and FCV were sensitive to R.H. in the 30–70% range. When subjected to aeration, all of the lipid-containing viruses which were examined lost infectivity but non-lipid viruses, including bovine adenovirus type 1 (BAdV-1), were stable. The addition of 0.1% peptone reduced losses, probably by protecting against surface inactivation. The significance of these findings in relation to possible control measures for viral respiratory disease is discussed.     

口蹄疫病毒抗原胶体金试纸条的研究

利用单克隆抗体技术制备抗口蹄疫病毒的单克隆抗体,特异性试验表明其只与O、A、Asia 1型3种血清型FMDV抗原结合。进而采用胶体金标记技术,以胶体金标记的抗口蹄疫病毒单克隆抗体、多克隆血清抗体和葡萄球菌A蛋白为主要材料,研制口蹄疫快速检测试纸条。该试纸条检测O、A、Asia 1型3种血清型灭活口蹄疫病毒均为阳性,检测水疱性口炎病毒、猪水疱病病毒、蓝舌病病毒、猪蓝耳病病毒4种灭活抗原及小反刍兽疫病毒疫苗株均为阴性,试验结果与口蹄疫实时荧光定量RT-PCR方法的完全一致,表明其具有良好的特异性。敏感性试验结果是,试纸条的检测极限为1∶160稀释的样品,其敏感性相当于实时荧光定量RT-PCR方法的1/64。由于试纸条具有操作方便、检测快速等优点,因此该试纸条可以用于大量临床样品的快速检测和现场检测。