ASTM E1053-1997(2002) Standard Test Method for Efficacy of Virucidal Agents Intended for Inanimate Environmental Surfaces《对无生物环境表面杀病毒剂预期效力的试验方法》.pdf
《ASTM E1053-1997(2002) Standard Test Method for Efficacy of Virucidal Agents Intended for Inanimate Environmental Surfaces《对无生物环境表面杀病毒剂预期效力的试验方法》.pdf》由会员分享,可在线阅读,更多相关《ASTM E1053-1997(2002) Standard Test Method for Efficacy of Virucidal Agents Intended for Inanimate Environmental Surfaces《对无生物环境表面杀病毒剂预期效力的试验方法》.pdf(3页珍藏版)》请在麦多课文档分享上搜索。
1、Designation: E 1053 97 (Reapproved 2002)Standard Test Method forEfficacy of Virucidal Agents Intended for InanimateEnvironmental Surfaces1This standard is issued under the fixed designation E 1053; the number immediately following the designation indicates the year oforiginal adoption or, in the cas
2、e of revision, the year of last revision. A number in parentheses indicates the year of last reapproval. Asuperscript epsilon (e) indicates an editorial change since the last revision or reapproval.1. Scope1.1 This laboratory test method is used to evaluate thevirucidal efficacy of liquid, aerosol,
3、or trigger spray antimicro-bial solutions on inanimate nonporous environmental surfaces.This test method may be employed with most viruses and isdesigned for cell culture host systems.1.2 This test method should be performed only by thosetrained in microbiological or virological techniques.1.3 This
4、standard does not purport to address all of thesafety concerns, if any, associated with its use. It is theresponsibility of the user of this standard to establish appro-priate safety and health practices and determine the applica-bility of regulatory limitations prior to use. The user shouldconsult
5、a reference for the laboratory safety recommenda-tions.21.4 It is the responsibility of the investigator to determinewhether Good Laboratory Practice regulations (GLPs) arerequired and to follow them where appropriate (40 CFR, Part160 for EPA submissions and 21 CFR, Part 58 for FDAsubmissions). Refe
6、r to the appropriate regulatory agency forperformance standards of virucidal efficacy.2. Referenced Documents2.1 ASTM Standards:3E 1052 Test Method for Efficacy of Virucidal AgentsAgainst Viruses in SuspensionsE 1153 Test Method for Efficacy of Sanitizers Recom-mended for Inanimate Non-Food Contact
7、SurfacesE 1482 Test Method for Neutralization of Virucidal Agentsin Virucidal Efficacy Evaluations2.2 Federal Standards:Title 40, Code of Federal Regulations (CFR), Environmen-tal Protection Agency, Subchapter E, Pesticide Programs;Part 160, Good Laboratory Practice Standards4Title 21, Code of Feder
8、al Regulations (CFR), Food andDrug Administration, Part 58, Laboratory Practice forNonclinical Laboratory Studies43. Summary of Test Method3.1 The virus suspension is dried on an inanimate, nonpo-rous surface. The antimicrobial is added over the dried film asa use dilution solution or sprayed from a
9、n aerosol can or triggerspray container following the recommended directions. Afterexposure at the appropriate temperature (usually 22 6 2C) forthe recommended time, the virus-antimicrobial mixture isassayed in a host system appropriate for the test virus. Thevirus titer of an untreated surface is d
10、etermined by the medianinfective dose (ID50) method of virus titration. Cytotoxicity tothe host system of the antimicrobial at the tested concentrationis determined by an LD50method. The virus-antimicrobialmixture is assayed in numerous units of the host system at adilution just beyond the cytotoxic
11、ity range of the antimicrobial.The extent of virus inactivation by the antimicrobial is deter-mined. Results are recorded as log10-virus inactivated.3.2 This test method is designed to be performed by atrained virologist who is responsible for choosing the appro-priate host system for the test virus
12、 and applying the techniquesnecessary for propagation and maintenance of host and testvirus. For a reference text, refer to Schmidt and Emmons.54. Significance and Use4.1 This test method may be used to determine the effec-tiveness of liquid and aerosol antimicrobial products againstdesignated proto
13、type viruses.4.2 The effective antimicrobial concentration should bedetermined utilizing cell cultures as the host system for specificviruses.4.3 This test method is applicable for testing of liquid andpressurized antimicrobial products against viruses on inani-mate nonporous environmental surfaces.
14、1This test method is under the jurisdiction of ASTM Committee E35 onPesticides and is the direct responsibility of Subcommittee E35.15 onAntimicrobialAgents.Current edition approved April 10, 1997. Published June 1997. Originallypublished as E 1053 85. Last previous edition E 1053 91.2CDC-NIH, Biosa
15、fety in Microbiological and Biomedical Laboratories, 3rd ed.,U.S. Department of Health and Human Services, Washington, DC, May 1993.3For referenced ASTM standards, visit the ASTM website, www.astm.org, orcontact ASTM Customer Service at serviceastm.org. For Annual Book of ASTMStandards volume inform
16、ation, refer to the standards Document Summary page onthe ASTM website.4Available from U.S. Government Printing Office, Superintendent of Docu-ments, Washington, DC 20402.5Diagnostic Procedures for Viral and Rickettsial Infections, N. J. Schmidt and R.W. Emmons, eds., 6th ed., American Public Health
17、 Association, Washington, DC,1989.1Copyright ASTM International, 100 Barr Harbor Drive, PO Box C700, West Conshohocken, PA 19428-2959, United States.5. Materials and Reagents5.1 Cell Culture Technique:55.1.1 Cell Culture System, appropriate for test virus.5.1.2 Growth Media/Maintenance Media, Medium
18、 199, Ea-gles minimal essential medium (EMEM) or equivalent,supplemented with appropriate concentration of serum (inac-tivated and mycoplasma-free), antibiotics, and other growthfactors as needed.65.1.3 Diluent, the media listed in 5.1.2, phosphate bufferedsaline, trypticase soy broth supplemented w
19、ith serum or othersimilar buffered solutions.5.1.4 Plastic Cell Culture Ware.75.1.5 Incubator, capable of maintaining 37 6 1C or othertemperature appropriate for replication of the specific testvirus.5.1.6 Refrigerator,46 2C.5.1.7 Test Tubes, screw-capped.5.1.8 Pipettes, serological, 10, 1, and 0.5
20、mL.5.1.9 Microtitration Kit.85.1.10 Petri Plates, glass, 60-mm diameter, 1 cm deep.5.2 Additional or equivalent materials and reagents specificto the host recovery system may be necessary. The trainedmicrobiologist or virologist is responsible to choose accord-ingly as needed.6. Test Viruses6.1 To d
21、etermine virucidal efficacy, a prototype strain froma particular virus family must be tested. Because new strains ofviruses are being discovered continuously and methods ofisolation and growth are being improved, the following proto-types and the cell cultures in which to grow and test them aresugge
22、sted. Other strains within a family may be substituted astesting prototypes for specific marketing claims.6.2 To demonstrate the range of antiviral activity of anantimicrobial, the formulation should be tested against virusesrepresenting a range of resistances to germicides. A possiblegroup of virus
23、es includes a poliovirus (representative of thoseviruses most resistant to chemical germicides), a herpes virus(representative of those most easily inactivated), and an aden-ovirus (representative of intermediate resistance to germi-cides). The following is a list of suggested virus strains thattypi
24、cally are assayed, as well as cell cultures that support theirgrowth.6.3 Typical test virus strains and cell cultures.6.3.1 Poliovirus, Type 1, Chat strain, ATCC VR-192.Cell line options: Monkey Kidney Cells (VERO): HumanEpidermoid.Carcinoma, Larynx (HEp-2):African Green Monkey Kid-ney (CV-1).6.3.2
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