ASTM E169-2004(2009) 3750 Standard Practices for General Techniques of Ultraviolet-Visible Quantitative Analysis《紫外线-可见光定量分析的一般技术规范》.pdf
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1、Designation: E169 04 (Reapproved 2009)Standard Practices forGeneral Techniques of Ultraviolet-VisibleQuantitative Analysis1This standard is issued under the fixed designation E169; the number immediately following the designation indicates the year oforiginal adoption or, in the case of revision, th
2、e 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 These practices are intended to provide general infor-mation on the techniques most often used in ultraviole
3、t andvisible quantitative analysis. The purpose is to render unnec-essary the repetition of these descriptions of techniques inindividual methods for quantitative analysis.1.2 The values stated in SI units are to be regarded asstandard. No other units of measurement are included in thisstandard.1.3
4、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 of regulatory limitations prior to use.2. Referenced Docum
5、ents2.1 ASTM Standards:2E131 Terminology Relating to Molecular SpectroscopyE168 Practices for General Techniques of Infrared Quanti-tative AnalysisE275 Practice for Describing and Measuring Performanceof Ultraviolet and Visible SpectrophotometersE925 Practice for Monitoring the Calibration of Ultrav
6、iolet-Visible Spectrophotometers whose Spectral Bandwidthdoes not Exceed 2 nmE958 Practice for Measuring Practical Spectral Bandwidthof Ultraviolet-Visible Spectrophotometers3. Summary of Practice3.1 Quantitative ultraviolet and visible analyses are basedupon the absorption law, known as Beers law.
7、The units of thislaw are defined in Terminology E131. Beers law (Note 1)holds at a single wavelength and when applied to a singlecomponent sample it may be expressed in the following form(see Section 10):A 5 abc (1)When applied to a mixture of n non-interacting components,it may be expressed as foll
8、ows:A 5 a1bc11 a2bc21 1 anbcn(2)NOTE 1Detailed discussion of the origin and validity of Beers lawmay be found in the books and articles listed in the bibliography at the endof these practices.3.2 This practice describes the application of Beers law intypical spectrophotometric analytical application
9、s. It also de-scribes operating parameters that must be considered whenusing these techniques.4. Significance and Use4.1 These practices are a source of general information onthe techniques of ultraviolet and visible quantitative analyses.They provide the user with background information that should
10、help ensure the reliability of spectrophotometric measure-ments.4.2 These practices are not intended as a substitute for athorough understanding of any particular analytical method. Itis the responsibility of the users to familiarize themselves withthe critical details of a method and the proper ope
11、ration of theavailable instrumentation.5. Sample Preparation5.1 Accurately weigh the specified amount of the sample(solid or liquid). Dissolve in the appropriate solvent and diluteto the specified volume in volumetric glassware of the requiredaccuracy, ensuring that all appropriate temperature range
12、tolerances are maintained. If needed, a dilution should be madewith a calibrated pipet and volumetric flask, using adequatevolumes for accuracy. With the availability of moderin widerange electronic balances, (capable of reading kg quantities tofour or five decimal places), gravimetric dilution shou
13、ld beconsidered as a more accurate alternative to volumetric, if1Precision and Bias These practices are under the jurisdiction of ASTMCommittee E13 on Molecular Spectroscopy and Separation Science and are thedirect responsibility of Subcommittee E13.01 on Ultra-Violet, Visible, and Lumi-nescence Spe
14、ctroscopy.Current edition approved Oct. 1, 2009. Published December 2009. Originallyapproved in 1960. Last previous edition approved in 2004 as E169 04. DOI:10.1520/E0169-04R09.2For referenced ASTM standards, visit the ASTM website, www.astm.org, orcontact ASTM Customer Service at serviceastm.org. F
15、or Annual Book of ASTMStandards volume information, refer to the standards Document Summary page onthe ASTM website.1Copyright ASTM International, 100 Barr Harbor Drive, PO Box C700, West Conshohocken, PA 19428-2959, United States.available. Fill the absorption cell with the solution, and fill theco
16、mparison or blank cell with the pure solvent, at least 23 to33 (if sufficient sample or solvent is available), beforemeasuring.6. Cell and Base-Line Checks6.1 Clean and match the cells. Suggested cleaning proce-dures are presented in Practice E275.6.2 Establish the base line of a recording double-be
17、amspectrophotometer by scanning over the appropriate wave-length region with pure solvent in both cells. Determineapparent absorbance of the sample cell at each wavelength ofinterest. These absorbances are cell corrections that are sub-tracted from the absorbance of the sample solution at thecorresp
18、onding wavelengths.6.3 For single beam instruments, either use the same cell forpure solvent and sample measurements, use matched cells, orapply appropriate cell corrections.6.4 On most software-controlled instruments, the cell cor-rections or the blank cell absorbance is stored in memory andautomat
19、ically incorporated into the sample absorbance mea-surement.6.5 An accurate determination of cell path length in the1-cm range is not practical in most laboratories, and commonpractice is to purchase cells of known path length. Modern cellmanufacturing techniques employed by a number of leadingmanuf
20、acturers can guarantee the path length of a 1-cm cell to60.01 mm or better.7. Analytical Wavelengths and Photometry7.1 Analytical wavelengths are those wavelengths at whichabsorbance readings are taken for use in calculations. Thesemay include readings taken for purposes of background cor-rections.
21、To minimize the effect of wavelength error, theanalytical wavelengths are frequently chosen at absorptionmaxima, but this is not always necessary. If the wavelengthaccuracy of the spectrophotometer is such that the calculateduncertainty in the absorbance measurement is within accept-able limits at t
22、he extremes of this wavelength uncertainy range,then single point measurements on a slope can be used. Forexample, the use of isoabsorptive or isosbestic points isfrequently useful.7.2 Record the absorbance readings at the specified analyti-cal wavelengths, operating the instrument in accordance wit
23、hthe recommendations of the manufacturer or Practice E275.7.3 Absorbance values should be used only if they fallwithin the acceptably accurate range of the particular spectro-photometer and method employed. If the absorbance is too low,either use a longer absorption cell or prepare a new solution of
24、higher concentration. If the absorbance is too high, use ashorter cell or make a quantitative dilution3. If different cellsare used, a new base-line must be obtained.7.4 The precision and bias of the wavelength and photomet-ric scales of the instrument must be adequate for the methodbeing used. Proc
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