ASTM E2471-2005(2011)e1 Standard Test Method for Using Seeded-Agar for the Screening Assessment of Antimicrobial Activity In Carpets《用籽粒琼脂进行地毯中抗菌剂活性的筛选评估的标准试验方法》.pdf
《ASTM E2471-2005(2011)e1 Standard Test Method for Using Seeded-Agar for the Screening Assessment of Antimicrobial Activity In Carpets《用籽粒琼脂进行地毯中抗菌剂活性的筛选评估的标准试验方法》.pdf》由会员分享,可在线阅读,更多相关《ASTM E2471-2005(2011)e1 Standard Test Method for Using Seeded-Agar for the Screening Assessment of Antimicrobial Activity In Carpets《用籽粒琼脂进行地毯中抗菌剂活性的筛选评估的标准试验方法》.pdf(3页珍藏版)》请在麦多课文档分享上搜索。
1、Designation: E2471 05 (Reapproved 2011)1Standard Test Method forUsing Seeded-Agar for the Screening Assessment ofAntimicrobial Activity In Carpets1This standard is issued under the fixed designation E2471; the number immediately following the designation indicates the year oforiginal adoption or, in
2、 the case of revision, the year of last revision. A number in parentheses indicates the year of last reapproval. Asuperscript epsilon () indicates an editorial change since the last revision or reapproval.1NOTEEditorial changes were made throughout in April 2011.INTRODUCTIONTodays modern commercial
3、carpets (especially modular carpet tile) often incorporate antimicrobialagents either in or on the face fibers or incorporated into the primary backing (attachment point ofcarpet fiber to the backing structure). The American Association of Textile Chemists and Colorists(AATCC) Method 174 permits bot
4、h qualitative and quantitative antibacterial assessment andantifungal assessment (qualitative only) of antimicrobial treatments in or on carpet. However, themethod is not suited for rapid screening of antimicrobials low in water solubility or that have slowdiffusion rates when incorporated into the
5、carpets primary backing layer. The test method describedhere provides a rapid screen of antimicrobial activity in or on carpets and allows for the simultaneousassessment of multiple components of the carpet (not just the fibers).1. Scope1.1 This test method is designed to evaluate (qualitatively)the
6、 presence of antimicrobial activity in or on carpets. Use thistest method to qualitatively evaluate both antibacterial andantifungal activity.1.2 Use half strength (nutrient and agar) tryptic soy agar asthe inoculum vehicle for bacteria and half strength potatodextrose agar as the inoculum vehicle f
7、or mold conidia. Use ofhalf strength agars may reduce undue neutralization of anantimicrobial due to excessive organic load.1.3 This test method simultaneously evaluates (both visualand stereo-microscopic) antimicrobial activity both at the fiberlayer and at the primary backing layer of carpet.1.4 U
8、se this test method to assess the durability of theantimicrobial treatments on new carpets, and on those repeat-edly shampooed or exposed to in-use conditions.1.5 Knowledge of microbiological techniques is requiredfor the practice of this test method.1.6 This standard does not purport to address all
9、 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.2. Referenced Documents2.1 American Association of Textile Chemi
10、sts and Colorists(AATCC) Standard:Method 174-2007, Antimicrobial Activity Assessment ofCarpets23. Terminology3.1 Definitions:3.1.1 face fiber, nthe wear layer of the carpet; can becomposed of nylon, polypropylene, wool, or other natural orsynthetic polymers. Typically, face fiber is tufted into a wo
11、venor non-woven scrim and then coated with latex to bond the facefiber securely to the backing; this latex coated scrim forms theprimary backing.3.1.2 inoculum vehicle, ncarrier solution used to transportbacterial cells or mold conidia to the test substrate.3.1.3 primary backing, nthe uppermost laye
12、r of carpetbacking where carpet fiber bundles are physically attached atthe base to the backing structure. This layer is typicallyconstructed of synthetic latex (ethylene vinyl acetate, styrenebutadiene, or a thermo-polymer; that is, ethylene vinyl acetatehot-melt adhesive).3.1.4 seeded agar, na thi
13、n layer of molten (liquid) micro-biological agar containing either bacterial cells or mold conidia(spores) used to challenge a test substrate.1This test method is under the jurisdiction of ASTM Committee E35 onPesticides, Antimicrobials, and Alternative Control Methods and is the directresponsibilit
14、y of Subcommittee E35.15 on Antimicrobial Agents.Current edition approved March 1, 2011. Published April 2011. Originallyapproved in 2005 as E2471 05. DOI: 10.1520/E2471-05R11E01.2Available from American Association of Textile Chemists and Colorists(AATCC), P.O. Box 12215, Research Triangle Park, NC
15、 27709, http:/www.aatcc.org.1Copyright ASTM International, 100 Barr Harbor Drive, PO Box C700, West Conshohocken, PA 19428-2959, United States.4. Summary of Test Method4.1 Cut carpet samples into small rectangular pieces eithervia a carpet knife or mechanical die and press. Shave half ofthe face fib
16、er on each sample using electric hair clippers andarrange in sterile Petri dishes (typically with the shaven half ofthe sample facing the center of the dish. Cool molten agars (fullor partial complement) to 45 6 2C and inoculate with thechallenge bacteria or mold conidia. Following wrist actionmixin
17、g, immerse samples into the seeded-molten agar, placeinto a Petri dish and pour additional seeded agar into the dishto surround but not cover the test sample. Incubate the Petridish for 24 to 72 h at 30 6 2C. Visually and microscopicallyexamine both at the face fiber and shaven (primary backing)laye
18、r for inhibition of the challenge microorganisms. Reportthe presence of carpet surface inhibition (for low water solubleor slow migrating antimicrobials) or zone of inhibition forwater soluble antimicrobials.35. Significance and Use5.1 This test method provides for rapid screening of anti-microbial
19、treatments located in or on the carpet face fiber orincorporated into the backing structure of the carpet (or both).5.2 This test method simulates actual use conditions thatmay occur on carpets (for example, food and beverage spills,soiling from foot traffic, prolonged moisture exposure).5.3 This te
20、st method provides a means to screen for activityand durability of an antimicrobial treatment under conditionsof organic loading.5.4 This test method provides for the simultaneous assess-ment of multiple carpet components for antimicrobial activity.5.5 Carpets may be cleaned prior to testing with th
21、is testmethod in order to assess the durability of the antimicrobialeffect.6. Apparatus6.1 Stereomicroscope,10to703 objectives.6.2 Erlenmeyer Flasks, 250 mL.6.3 Sterile Petri Dishes, 150 mm.6.4 Incubators, set at required temperatures (30 6 2C and37 6 2C).6.5 Autoclave.6.6 Water Bath, capable of mai
22、ntaining water at 45 6 2C.6.7 Test Tubes, 16 by 100 mm.6.8 Hot Plate with Stirrer.6.9 Spectrophotometer.6.10 Sterile Cuvettes.6.11 Test Carpet.6.12 Electric Hair Clippers (Oster Golden A5 or equivalent#30 Blade).6.13 Canned Air (compressed air for surface dusting).6.14 Sterile Petri Dishes, 100 mm.6
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