ASTM F838-2005(2013) Standard Test Method for Determining Bacterial Retention of Membrane Filters Utilized for Liquid Filtration《测定液体过滤用膜过滤器细菌滞留的标准试验方法》.pdf
《ASTM F838-2005(2013) Standard Test Method for Determining Bacterial Retention of Membrane Filters Utilized for Liquid Filtration《测定液体过滤用膜过滤器细菌滞留的标准试验方法》.pdf》由会员分享,可在线阅读,更多相关《ASTM F838-2005(2013) Standard Test Method for Determining Bacterial Retention of Membrane Filters Utilized for Liquid Filtration《测定液体过滤用膜过滤器细菌滞留的标准试验方法》.pdf(6页珍藏版)》请在麦多课文档分享上搜索。
1、Designation: F838 05 (Reapproved 2013)Standard Test Method forDetermining Bacterial Retention of Membrane FiltersUtilized for Liquid Filtration1This standard is issued under the fixed designation F838; the number immediately following the designation indicates the year of originaladoption or, in the
2、 case of revision, the year of last revision.Anumber in parentheses indicates the year of last reapproval.Asuperscriptepsilon () indicates an editorial change since the last revision or reapproval.1. Scope1.1 This test method determines the bacterial retentioncharacteristics of membrane filters for
3、liquid filtration usingPseudomonas diminuta as the challenge organism. This testmethod may be employed to evaluate any membrane filtersystem used for liquid sterilization.1.2 This standard may involve hazardous materials,operations, and equipment. This standard does not purport toaddress all of the
4、safety concerns, if any, associated with itsuse. It is the responsibility of the user of this standard toestablish appropriate safety and health practices and deter-mine the applicability of regulatory limitations prior to use.2. Referenced Documents2.1 ASTM Standards:2D1193 Specification for Reagen
5、t Water3. Terminology3.1 Definitions:3.1.1 log reduction valuethe logarithm to the base 10 ofthe ratio of the number of microorganisms in the challenge tothe number of organisms in the filtrate.4. Summary of Test Method4.1 After sterilization, the test filter is challenged with asuspension of Pseudo
6、monas diminuta (ATCC 19146)3at aconcentration of 107organisms per cm2of effective filtrationarea (EFA) at a maximum differential pressure across the testfilter of 30 psig (206 kPa) and a flow rate of 0.5 to 1.0 GPM perft2of effective filtration area (2 to410-3LPM per cm2). Theentire filtrate is then
7、 filtered through an analytical membranefiler disc which is subsequently incubated on a solidifiedgrowth medium. Organisms that are not retained by the filterbeing tested will develop into visible colonies on the analysismembrane and can then be enumerated.5. Significance and Use5.1 Since all steril
8、izing filtration processes are performedunder positive pressure, this test method is designed to assessthe retentivity of a sterilizing filter under process conditions.5.1.1 A challenge of 107bacteria per cm2of effectivefiltration area is orders of magnitude higher than one wouldexpect to encounter
9、in a sterilizing filtration process. This levelwas selected in order to provide a high degree of assurance thatthe filter would quantitatively retain large numbers of organ-isms. This concept is important, in view of the requirement toprovide a quantitative assessment in validating a sterilizationpr
10、ocess.5.1.2 The analytical procedure utilized in this test methodprovides a method to assign a numerical value to the filtrationefficiency of the filter being evaluated. This value, coupledwith a knowledge of the number and types of organisms(bioburden) indigenous to the process, may then be utilize
11、d todetermine the probability of obtaining a sterile filtrate.Conversely, the numerical value of the filtration efficiency maybe used when one must meet a specified probability of sterilityassurance to calculate the volume of fluid that may be filteredin order to maintain that level of assurance.6.
12、Apparatus6.1 Assemble the apparatus described below as in Fig. 1:6.1.1 Stainless Steel Pressure Vessel, 12-L capacity (orlarger), fitted witha0to50-psi (0 to 350-kPa) pressure gage.6.1.2 Air Regulator.6.1.3 142-mm Disc Filter Assemblies, two or more, withhose connections.6.1.4 Diaphragm-Protected 0
13、to 50-psi Pressure Gage (0 to350-kPa), for upstream pressure reading. A second equivalentgauge for downstream pressure reading is optional.6.1.5 Manifold, with valves (autoclavable) and hose connec-tions.6.1.6 Autoclavable Tubing, (must be able to withstand apressure of 50 psi (350 kPa).6.1.7 Filter
14、 Housing, with hose connections.1This test method is under the jurisdiction of ASTM Committee E55 onManufacture of Pharmaceutical Products and is the direct responsibility of Subcom-mittee E55.03 on General Pharmaceutical Standards.Current edition approved June 1, 2013. Published June 2013. Original
15、lyapproved in 1983. Last previous edition published in 2005 as F838 05. DOI:10.1520/F0838-05R13.2For referenced ASTM standards, visit the ASTM website, www.astm.org, orcontact ASTM Customer Service at serviceastm.org. For Annual Book of ASTMStandards volume information, refer to the standards Docume
16、nt Summary page onthe ASTM website.3Available from American Type Culture Collection (ATCC), 10801 UniversityBoulevard, Manassas, VA 20110, http:/www.atcc.org.Copyright ASTM International, 100 Barr Harbor Drive, PO Box C700, West Conshohocken, PA 19428-2959. United States16.1.8 Hose Clamps.6.1.9 Incu
17、bator, 30 6 2C.6.1.10 Laminar Flow Bench.6.1.11 Smooth-Tip Forceps.7. Purity of Reagents and Materials7.1 Purity of ReagentsReagent grade chemicals shall beused. Unless otherwise indicated, all reagents shall conform tothe specifications of the American Chemical Society, wheresuch specifications are
18、 available.47.2 Purity of WaterUnless otherwise indicated, referencesto water shall mean reagent water, Type IV as defined inSpecification D1193.7.2.1 Additionally, any water used in this test method mustconform to the requirements for non-bacteriostatic water speci-fied in the current edition of St
19、andard Methods for theExamination of Water and Wastewater.58. Reagents and Materials8.1 Saline Lactose Broth Medium:8.1.1 Lactose BrothDissolve 1.3 g of dehydrated lactosebroth medium in 100 mL of water.8.1.2 Sodium Chloride SolutionDissolve 7.6 g of sodiumchloride (NaCl) in 970 mL of water in a 2-L
20、 flask with anappropriate closure.8.1.3 Add 30 mL of lactose broth (8.1.1) to 970 mL ofsodium chloride solution. Autoclave at 121C for 15 min.8.2 Frozen Cell Paste Method:8.2.1 Growth Medium ADissolve in water and dilute to 1L. Autoclave at 121C for 15 min (pH 6.8 to 7.0).Trypticase Peptone (or Casi
21、tone) 7.5 gYeast Extract 2.5 gSodium Chloride (NaCl) 0.5 gMagnesium Sulfate (MgSO43H2O) 0.35 g8.2.2 Harvesting BufferDissolve 0.790 g of monobasicpotassium phosphate (KH2PO4)and1.0gofK2HPO4in 100mL of glycerol (C3H8O3). Adjust to pH 7.2 with 0.1 Npotassium hydroxide solution. Dilute to 1 L with wate
22、r andsterilize at 121C for 15 min.8.2.3 Potassium Hydroxide Solution (0.1 N)Dissolve 5.61g of potassium hydroxide (KOH) in water and dilute to 1 L ina volumetric flask.8.2.4 Trypticase Soy AgarPrepare according to manufac-turers instructions.8.2.5 Trypticase Soy BrothPrepare according to manufac-tur
23、ers instructions.8.3 Analytical Reagents and Materials:8.3.1 M-Plate Count AgarPrepare according to manufac-turers instructions.8.3.2 Peptone Water (1 g/L)Dissolve the peptone in water.Dispense suitable volumes, for preparing decimal dilutions,into screw-cap containers. Autoclave at 121C for 15 min.
24、8.4 Pseudomonas diminuta (ATCC 19146).8.5 Analytical Membrane Filters, 142-mm diameter, 0.45m pore size, 130 to 160 m thick.8.6 Petri Dishes, 150-mm diameter.9. Methods for Preparation of Bacterial Challenge StockSuspension9.1 GeneralThe following two methods have been usedextensively for the prepar
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