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本文(ASTM D5578-2004(2015) Standard Test Method for Determination of Ethylene Oxide in Workplace Atmospheres (HBr Derivatization Method)《用于测定工作场所环境中环氧乙烷的标准试验方法 (HBr衍生法)》.pdf)为本站会员(towelfact221)主动上传,麦多课文库仅提供信息存储空间,仅对用户上传内容的表现方式做保护处理,对上载内容本身不做任何修改或编辑。 若此文所含内容侵犯了您的版权或隐私,请立即通知麦多课文库(发送邮件至master@mydoc123.com或直接QQ联系客服),我们立即给予删除!

ASTM D5578-2004(2015) Standard Test Method for Determination of Ethylene Oxide in Workplace Atmospheres (HBr Derivatization Method)《用于测定工作场所环境中环氧乙烷的标准试验方法 (HBr衍生法)》.pdf

1、Designation: D5578 04 (Reapproved 2015)Standard Test Method forDetermination of Ethylene Oxide in Workplace Atmospheres(HBr Derivatization Method)1This standard is issued under the fixed designation D5578; 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.1. Scope1.1 This test method covers a method of collecting andanalyzing samples to determine th

3、e amount of ethylene oxide(ETO) present in workplace atmospheres.1.2 This test method can be used to provide a time-weightedaverage (TWA) over the concentration range from 0.2 to 4 ppm(v).1.3 This test method can be used to determine 15-minexcursions (STEL) ranging from 1 to 25 ppm (v).1.4 The value

4、s stated in SI units are to be regarded as thestandard.1.5 This 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

5、 of regulatory limitations prior to use. See Section 9 forspecific safety hazards.2. Referenced Documents2.1 ASTM Standards:2D1356 Terminology Relating to Sampling and Analysis ofAtmospheresD3686 Practice for Sampling Atmospheres to Collect Or-ganic Compound Vapors (Activated Charcoal Tube Ad-sorpti

6、on Method)D3687 Practice for Analysis of Organic Compound VaporsCollected by the Activated Charcoal Tube AdsorptionMethodE355 Practice for Gas Chromatography Terms and Relation-ships2.2 Other Standard:3Occupational Safety and Health Administration, U.S. De-partment of Labor, Title 29, Code of Federa

7、l Regulations,Part 1910, Subpart Z, Section 1910.10473. Terminology3.1 DefinitionsFor definitions of terms used in this testmethod, refer to Terminology D1356, and Practice E355.4. Summary of Test Method4.1 A known volume of air is pumped through a glass tubepacked with carbon molecular sieve, surfa

8、ce area 400 m2/gimpregnated with hydrogen bromide (HBr) where ETO isadsorbed and converted to 2-bromoethanol.4.2 The tube contains two reactive sections for samplecollection. The backup section collects vapors that passthrough the front section and is used to determine if thecollection capacity of t

9、he front section has been exceeded.4.3 The resultant derivative, 2-bromoethanol, is desorbedwith a mixture of acetonitrile/toluene and analyzed using a gaschromatograph equipped with an electron capture detector.4.4 Desorption efficiency is determined by spiking tubeswith known amounts of 2-bromoeth

10、anol and analyzing with thesame procedure used for air samples.4.5 Quantitation is achieved by comparing peak areas fromsample solutions with areas from standard solutions.5. Significance and Use5.1 Ethylene oxide is a major industrial chemical withproduction volume ranked in the top 25 chemicals pr

11、oduced inthe United States. It is used in the manufacture of a greatvariety of products as well as being a sterilizing agent andfumigant.5.2 This test method provides a means of determiningexposure levels of ETO in the working environment at thepresently recommended exposure guidelines.1This test me

12、thod is under the jurisdiction of ASTM Committee D22 on AirQuality and is the direct responsibility of Subcommittee D22.04 on Workplace AirQuality.Current edition approved Oct. 1, 2015. Published October 2015. Originallyapproved in 1994. Last previous edition approved in 2010 as D5578 04 (2010).DOI:

13、 10.1520/D5578-04R15.2For 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 Document Summary page onthe ASTM website.3Available from U.S. Government Printing

14、 Office, Superintendent ofDocuments, 732 N. Capitol St., NW, Washington, DC 20401-0001, http:/www.access.gpo.gov.Copyright ASTM International, 100 Barr Harbor Drive, PO Box C700, West Conshohocken, PA 19428-2959. United States15.2.1 OSHA Permissible Exposure Limit (PEL) 1 ppm,15-min excursion limit

15、5 ppm (CFR, Part 1910, Subpart Z,Section 1910.1047).35.2.2 ACGIH Threshold Limit Value (TLV) 1 ppm (1.8mg/m3), suspected human carcinogen.46. Interferences6.1 Derivatives and other compounds that have identical ornearly the same GC column retention time as 2-bromoethanolduring the gas chromatographi

16、c analysis will interfere.6.2 Interferences can sometimes be resolved by altering gaschromatographic operating conditions. The identity of sus-pected 2-bromoethanol, or the presence of 2-bromoethanolmasked by a chromatographic interference, or both, can beverified by gas chromatography/mass spectrom

17、etry.7. Apparatus7.1 Carbon Molecular Sieve, surface area 400 m2/g, HBrsampling tube.7.1.1 Preparation of Collection MediumAdd 20 mL ofHBr (24 %) to 70 g of carbon molecular sieve, surface area 400m2/g, in a glass jar. Cap the jar and mix the contents thoroughlyfor 5 min by rotating.Allow to equilib

18、rate and dry overnight orfor 12 h.7.1.2 Tube PreparationInsert a plug of silanized glasswool into a 10-cm by 6-mm outside diameter (4-mm insidediameter) glass tube. Pack the front section of the tube with400 mg of the reactive adsorbent (7.1.1), using gentle tappingor vibration to promote uniform pa

19、cking. Insert another plug ofsilanized wool and pack 200 mg of the adsorbent in the backupsection. Hold the backup section in place by firmly inserting anadditional glass wool plug. The tubes may be flame-sealed orsealed with polyethylene caps. Provide a numerical identifica-tion for each lot of tub

20、es.7.1.3 Tube Holder, capable of preventing breakage andprotecting worker during sampling.7.1.4 High-Density Polyethylene or Polypropylene Caps,tight-fitting, for resealing used tubes.7.2 Pump and Tubing:7.2.1 Sampling Pumps, having stable low flow rates(610 % of set flow rate) within the range from

21、 20 to 100mL/min for up to 8 h.7.2.2 Rubber or Plastic Tubing, 6-mm inside diameter, forconnecting collection tube to pump. All tubing must bedownstream (between tube and pump) of collection tube toprevent contamination or loss of sample.7.3 Vials, glass with PTFE-lined caps, 10 mL, for desorbingsam

22、ples and storing standards.7.4 Pipettes, 5 mL, for adding desorbing solution tosamples.7.5 Syringes, 10, 50, and 100-L syringes, for preparingstandards.7.6 Gas-Tight Syringe, 2 L, with low dead-volume needle.7.7 Gas Chromatograph (GC):7.7.1 Gas Chromatograph, with an electron capture detectorand a s

23、uitable readout device.7.7.2 Chromatographic Column, packed or capillary col-umns in accordance with 7.7.2.1 and 7.7.2.2 have been foundsuitable for this analysis.7.7.2.1 Packed, 3.7 m by 3 mm (12 ft by18 in.), stainlesssteel, packed with 10 % diethylene glycol succinate on diato-maceous earth, flux

24、-calcined, silanized, 80/100 mesh.7.7.2.2 Capillary, 30-m by 0.53-mm inside diameter fusedsilica capillary column with polyethylene glycol phase.8. Reagents8.1 Purity of ReagentsUnless otherwise indicated, it isintended that all reagents conform to the specifications of theCommittee on Analytical Re

25、agents of the American ChemicalSociety where such specifications are available.5Other gradesmay be used, provided it is first ascertained that the reagent isof sufficiently high purity to permit its use without lesseningthe accuracy of the determination.8.2 Acetonitrile, pesticide grade.8.3 2-Bromoe

26、thanol, commercially available at 98 % purityor better.8.4 Desorbing Solution, 1+1 (v/v) mixture of acetonitrileand toluene.8.5 Sodium Carbonate (Na2CO3).8.6 Toluene, pesticide grade.9. Hazards9.1 Minimize exposure to all reagents and solvents byperforming all sample and standard preparations as wel

27、l as tubedesorption in a well-ventilated hood.9.2 Avoid inhalation and skin contact with all reagents andsolvents.9.3 Use suitable protective holders when collecting samplesand handle used tubes carefully to prevent injury.10. Calibration10.1 Sample Pump Calibration:10.1.1 Calibrate the sample pump

28、flow in accordance withPractice D3686, with the ETO sampling tube positionedvertically and in line during calibration of the pump.10.1.2 Calibrate the flow rate of the pump at 20 mL/min forTWAsampling and 100 mL/min for STEL sampling dependingon the duration of the sample and the volume of samplenee

29、ded.10.2 Gas Chromatograph Calibration:4Threshold Limit Values for Chemical Substances and Physical Agents andBiological Exposure Indices, American Conference of Governmental IndustrialHygienists, 6500 Glenway Avenue, Building D-7, Cincinnati, OH 45211-4438.5Reagent Chemicals, American Chemical Soci

30、ety Specifications, AmericanChemical Society, Washington, DC. For Suggestions on the testing of reagents notlisted by the American Chemical Society, see Annual Standards for LaboratoryChemicals, BDH Ltd., Poole, Dorset, U.K., and the United States Pharmacopeiaand National Formulary, U.S. Pharmacopei

31、al Convention, Inc. (USPC), Rockville,MD.D5578 04 (2015)210.2.1 Prepare a 2-bromoethanol stock solution (1 g/L)by adding 57 L of 2-bromoethanol to 100 mL of toluene. Ifrefrigerated, this solution is stable for at least one month.10.2.2 To a series of five 10-mL vials containing 5.0 mL ofdesorbing so

32、lution, add 0.0, 10, 50, 100, and 200 L of stocksolution, thus, providing calibration standards equivalent to0.0, 3.5, 17.4, 34.5, and 67.7 g of ETO per 5 mL of desorbingsolution. These values take into account volume changescaused by the addition of stock solution.10.2.3 The 0.0-g standard describe

33、d in 10.2.2 constitutes areagent blank.10.2.4 Prepare a calibration curve by injecting these stan-dards into the GC following the procedure specified in 11.3.5and 11.3.6. Plot the peak area (or height) versus micrograms ofETO per 5 mL of desorbing solution.10.2.5 To cover a broader ETO concentration

34、 range, prepareadditional standards with the stock and desorbing solutions;however, exercise care by staying within the linear dynamicrange of the electron capture detector.11. Procedure11.1 Sample Collection:11.1.1 Immediately before sampling, break off the ends ofthe sampling tube (if flame sealed

35、) or remove end caps tocreate an opening of at least 2 mm in diameter.11.1.2 Attach a collection tube to a calibrated samplingpump using a section of plastic tubing, with the backup sectionnearest the pump.11.1.3 Place the tube vertically in the tube holder as near tothe breathing zone as possible.1

36、1.1.4 Activate the sampling pump that has been calibratedat the sampling site with the sampling tube in-line for the flowrate desired (20 mL/min for 8 h; or 100 mL/min for 15 min).11.1.5 Record the time, flow rate, barometric pressure, andtemperature when the pump is started.11.1.6 When sampling is

37、completed, check the flow ratebefore deactivating the pump. Immediately record the time,temperature, and barometric pressure again.11.1.7 Disconnect the sample tube and cap the ends withpolyethylene caps. Label the tube with sample identification.11.1.8 Include at least one blank sampling tube with

38、every10 to 15 samples, or for each operation or field survey. Treatthe field blank the same as air samples with the exception thatno air is drawn through the blank tube. The field blank must befrom the same tube lot as the air samples.11.2 Desorption Effciency:11.2.1 Determine the desorption efficie

39、ncy on the same lotof tubes as the air samples.11.2.2 Place 400-mg portions of collection medium (7.1.1)in each of several 10-mL vials.11.2.3 Add appropriate amounts of 2-bromoethanol stocksolution (10.2.1) directly onto the adsorbent prepared in 11.2.2,that correspond to the approximate levels of E

40、TO expected inair samples. Allow the spiked adsorbents to equilibrate over-night (or 12 h) at room temperature.11.2.4 Analyze replicates of each concentration level alongwith 400mg adsorbent tube blanks using the procedureindicated in 11.3.5 11.3.6, inclusively. Calibrate the gaschromatograph using

41、mass of 2-bromoethanol in calibrationstandards (10.2.2) instead of ETO equivalent.11.2.5 Calculate the desorption efficiency (DE) for eachamount of 2-bromoethanol as follows:DE 5Wr2 BWa(1)where:Wr= average mass recovered, g,B = blank, g, andWa= mass added, g.11.3 Analysis:11.3.1 Add 100 mg of Na2CO3

42、and 5.0 mL of desorbingsolution to each of the appropriately labeled vials that indicatethe tube numbers and front or backup section.11.3.2 Score and break tubes just above the front glass woolplug, remove plug, and slowly add front portion of adsorbent tothe appropriate vial. Seal the vial.11.3.3 R

43、emove the glass wool separator and add the backupsection of adsorbent to the proper vial. Make certain adsorbentparticles are not retained on the glass wool plugs and separatorbefore discarding.11.3.4 Desorb for 30 min at room temperature, shaking thevial occasionally during this period.11.3.5 Quant

44、itatively inject 2 L of sample solution into theGC using the solvent flush technique as described in PracticeD3687. Alternatively, samples may be injected using anautomated injection system.11.3.6 Complete the GC analysis following the chromato-graphic conditions described in 11.3.6.1. The approxima

45、teETO retention time and total chromatographic analysis time is4.0 and 8.0 min, respectively.11.3.6.1 Gas Chromatographic Operating ConditionsColumn temperature, 155 C; injection port and detectortemperatures, 240 C; carrier gas (5 % methane/argon) flowrate, 30 mL/min (packed column) or 20 cm/s (cap

46、illarycolumn).11.3.6.2 Determine the peak height or peak area of the2-bromoethanol.12. Calculation12.1 Correct samples for ETO found in the sampling tubeblank (10.2.3).12.2 Determine the amount (g) of ethylene oxide in thefront and backup sections of the sample tube using thecalibration curve genera

47、ted in 10.2.4. If the backup sectioncontains more than 10 % of the amount of ethylene oxidecontained in the front section, report breakthrough and possiblesample loss.612.3 Calculate the concentration of ETO in the air samplesas follows:Ethylene Oxide, ppm by volume 5W 324.47DE 3L 344.05(2)6NIOSH Ma

48、nual of Analytical Methods, Cincinnati, OH 45226.D5578 04 (2015)3where:W = micrograms of ETO in sample (sum of front andbackup section),24.47 = molar volume of an ideal gas, L/mole, at 25 C and101.3 kPa (760 mm Hg),DE = desorption efficiency,L = volume of air sampled, L, and44.05 = molecular weight

49、of ethylene oxide, g/mole.12.4 If a field blank shows contamination, the samplescollected during the survey must be assumed to be contami-nated (see Practice D3687).13. Precision and Bias713.1 PrecisionBased on limited information from onelaboratory, the repeatability standard deviations and the 95 %repeatability limits are approximately 69.3 %, as illustrated inTable 1. The reproducibility of this test method is beingdetermined.13.1.1 The values shown in Table 1 are averages of sixreplicates obtained for each concentration of ETO generated ina 6920L st

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