ASTM E169-04(2014)

NOTICE: This standard has either been superseded and replaced by a new version or withdrawn.
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Designation: E169 − 04(Reapproved 2014)
Standard Practices for
General Techniques of Ultraviolet-Visible Quantitative
Analysis
This standard is issued under the fixed designation E169; the number immediately following the designation indicates the year of
original adoption or, in the case of revision, the year of last revision.Anumber in parentheses indicates the year of last reapproval.A
superscript epsilon (´) indicates an editorial change since the last revision or reapproval.
1. Scope law are defined in Terminology E131. Beer’s law (Note 1)
holds at a single wavelength and when applied to a single
1.1 These practices are intended to provide general infor-
component sample it may be expressed in the following form
mation on the techniques most often used in ultraviolet and
(see Section 10):
visible quantitative analysis. The purpose is to render unnec-
essary the repetition of these descriptions of techniques in A 5 abc (1)
individual methods for quantitative analysis.
Whenappliedtoamixtureof nnon-interactingcomponents,
1.2 The values stated in SI units are to be regarded as
it may be expressed as follows:
standard. No other units of measurement are included in this
A 5 a bc 1a bc 1….1a bc (2)
1 1 2 2 n n
standard.
1.3 This standard does not purport to address all of the
NOTE 1—Detailed discussion of the origin and validity of Beer’s law
safety concerns, if any, associated with its use. It is the
maybefoundinthebooksandarticleslistedinthebibliographyattheend
responsibility of the user of this standard to establish appro-
of these practices.
priate safety and health practices and determine the applica-
3.2 This practice describes the application of Beer’s law in
bility of regulatory limitations prior to use.
typical spectrophotometric analytical applications. It also de-
2. Referenced Documents scribes operating parameters that must be considered when
2 using these techniques.
2.1 ASTM Standards:
E131Terminology Relating to Molecular Spectroscopy
4. Significance and Use
E168Practices for General Techniques of Infrared Quanti-
3 4.1 These practices are a source of general information on
tative Analysis (Withdrawn 2015)
the techniques of ultraviolet and visible quantitative analyses.
E275PracticeforDescribingandMeasuringPerformanceof
Theyprovidetheuserwithbackgroundinformationthatshould
Ultraviolet and Visible Spectrophotometers
help ensure the reliability of spectrophotometric measure-
E925Practice for Monitoring the Calibration of Ultraviolet-
ments.
Visible Spectrophotometers whose Spectral Bandwidth
does not Exceed 2 nm 4.2 These practices are not intended as a substitute for a
E958Practice for Estimation of the Spectral Bandwidth of thorough understanding of any particular analytical method. It
is the responsibility of the users to familiarize themselves with
Ultraviolet-Visible Spectrophotometers
the critical details of a method and the proper operation of the
3. Summary of Practice
available instrumentation.
3.1 Quantitative ultraviolet and visible analyses are based
5. Sample Preparation
upontheabsorptionlaw,knownasBeer’slaw.Theunitsofthis
5.1 Accurately weigh the specified amount of the sample
(solid or liquid). Dissolve in the appropriate solvent and dilute
These practices are under the jurisdiction of ASTM Committee E13 on
tothespecifiedvolumeinvolumetricglasswareoftherequired
Molecular Spectroscopy and Separation Science and are the direct responsibility of
Subcommittee E13.01 on Ultra-Violet, Visible, and Luminescence Spectroscopy.
accuracy, ensuring that all appropriate temperature range
Current edition approved Aug. 1, 2014. Published August 2014. Originally
tolerancesaremaintained.Ifneeded,adilutionshouldbemade
approvedin1960.Lastpreviouseditionapprovedin2009asE169–04(2009).DOI:
with a calibrated pipet and volumetric flask, using adequate
10.1520/E0169-04R14.
volumes for accuracy. With the availability of moderin wide
For referenced ASTM standards, visit the ASTM website, www.astm.org, or
contact ASTM Customer Service at service@astm.org. For Annual Book of ASTM
range electronic balances, (capable of reading kg quantities to
Standards volume information, refer to the standard’s Document Summary page on
four or five decimal places), gravimetric dilution should be
the ASTM website.
3 considered as a more accurate alternative to volumetric, if
The last approved version of this historical standard is referenced on
www.astm.org. available. Fill the absorption cell with the solution, and fill the
Copyright © ASTM International, 100 Barr Harbor Drive, PO Box C700, West Conshohocken, PA 19428-2959. United States
E169 − 04 (2014)
comparisonorblankcellwiththepuresolvent,atleast2×to3× being used. Procedures for checking precision and accuracy of
(if sufficient sample or solvent is available), before measuring. these scales are presented in Practices E275 and E925.
6. Cell and Base-Line Checks 8. Resolution and Bandwidth
8.1 If the analytical method specifies a resolution or a
6.1 Clean and match the cells. Suggested cleaning proce-
dures are presented in Practice E275. spectral slit width, set the resolution of the instrument to the
specified value. If the instrument has only a mechanical
6.2 Establish the base line of a recording double-beam
bandwidth indicator, use the information provided in the
spectrophotometer by scanning over the appropriate wave-
manufacturer’s literature to calculate the bandwidth that cor-
length region with pure solvent in both cells. Determine
responds to the specified resolution.
apparent absorbance of the sample cell at each wavelength of
interest. These absorbances are cell corrections that are sub-
NOTE 2—The accuracy of resolution and mechanical bandwidth indi-
cators can be determined using the procedure given in Practice E958.
tracted from the absorbance of the sample solution at the
corresponding wavelengths.
8.2 If the analytical method does not state a required
resolution or a bandwidth value but includes an illustrative
6.3 Forsinglebeaminstruments,eitherusethesamecellfor
spectrum, set the resolution or bandwidth of the instrument to
pure solvent and sample measurements, use matched cells, or
obtain comparable data. As a rule of thumb, the resolution
apply appropriate cell corrections.
should be less than one-eighth of the bandwidth; thus for a
6.4 On most software-controlled instruments, the cell cor-
peak of bandwidth 40 nm, the resolution should not exceed 5
rections or the blank cell absorbance is stored in memory and
nm.
automatically incorporated into the sample absorbance mea-
8.3 If the method neither specifies resolution or bandwidth
surement.
nor provides an illustrative spectrum, use the smallest resolu-
6.5 An accurate determination of cell path length in the
tion or bandwidth that yields an acceptable signal-to-noise
1-cm range is not practical in most laboratories, and common
ratio. Record this value for future reference.
practiceistopurchasecellsofknownpathlength.Moderncell
NOTE 3—Changes in the day-to-day values of resolution or bandwidth
manufacturing techniques employed by a number of leading
obtained with a given gain, or changes in signal-to-noise ratio at a given
manufacturers can guarantee the path length of a 1-cm cell to
resolution, are indicative of present or potential problems. Increased
60.01 mm or better.
resolution or a lowering of the S/N ratio may result from a lower output
of the light source, deterioration of optical components, deposits on the
7. Analytical Wavelengths and Photometry
windows of the cell compartment or on the inside wall of the reference
cell, an absorbing impurity in the solvent, or a faulty electronic compo-
7.1 Analytical wavelengths are those wavelengths at which
nent.
absorbance readings are taken for use in calculations. These
may include readings taken for purposes of background cor-
9. Solvents and Solvent Effects
rections. To minimize the effect of wavelength error, the
9.1 The ultraviolet absorption spectrum of a compound will
analytical wavelengths are frequently chosen at absorption
varyindifferentsolventsdependingonthechemicalstructures
maxima, but this is not always necessary. If the wavelength
involved. Non-polar solvents have the least effect on the
accuracy of the spectrophotometer is such that the calculated
absorption spectrum. Non-polar molecules in most instances
uncertainty in the absorbance measurement is within accept-
are not affected in polar solvents. However, polar molecules in
ablelimitsattheextremesofthiswavelengthuncertainyrange,
polar solvents may show marked differences in their spectra.
then single point measurements on a slope can be used. For
Any interaction between solute and solvents leads to a broad-
example, the use of isoabsorptive or isosbestic points is
ening and change in structural resolution of the absorption
frequently useful.
bands. Ionic forms may be created in acidic or basic solutions.
7.2 Record the absorbance readings at the specified analyti-
In addition, there are possible chemical reactions between
cal wavelengths, operating the instrument in accordance with
solute and solvent, and also photochemical reactions arising
the recommendations of the manufacturer or Practice E275.
from either room illumination or the short wavelengths in the
beam of the spectrophotometer. It is important that the solvent
7.3 Absorbance values should be used only if they fall
used be specified in recording spectral data. (The change in
within the acceptably accurate range of the particular spectro-
spectrabetweenacidicandbasicconditionsmaysometimesbe
photometerandmethodemployed.Iftheabsorbanceistoolow,
employed in multicomponent analysis.)
either use a longer absorption cell or prepare a new solution of
higher concentration. If the absorbance is too high, use a
9.2 Reference solvent data is shown in Table 1.Availability
shorter cell or make a quantitative dilution. If different cells
of a particular solvent may be restricted by international
are used, a new base-line must be obtained.
agreement, and the users’ attention is directed to 1.3 of these
practices. The short wavelength limit is approximate, and
7.4 Theprecisionandbiasofthewavelengthandphotomet-
referstothewavelengthatwhicha1-cmlightpathlengthgives
ric scales of the instrument must be adequate for the method
an absorbance of unity.
9.3 Water,and0.1Msolutionsofhydrochloricacid,sulfuric
The errors associated with cell path lengths are significantly less than those
acid, and sodium hydroxide also are commonly used as
generatedbyvolumetricdilution,andthereforewherepossible,differentpathlength
cells should be used in preference to volumetric procedures. solvents. Buffered solutions, involving non-absorbing
E169 − 04 (2014)
A
TABLE 1 Solvents
Note that c and C , have the dimensions of grams per litre.
s
Solvent Cutoff, nm
Ifdilutionismade, C isnottheconcentrationinthecellatthe
s
Pyridine 305
timetheabsorbanceisdetermined;theconcentrationinthecell
Tetrachloroethylene 290
is C /f.
s
Benzene 280
N,N-Dimethylformamide 270
10.3 ChemicalCalibration—Theabsorptivityoftheabsorb-
Carbon tetrachloride 265
ing material, the concentration of which it is desired to
Methyl formate 260
Chloroform 245
determine, is obtained by examination of a series of quantita-
Dichloromethane 235
tive dilutions of a neat sample of this material. However, if no
Ethyl ether 220
such neat sample is available, the best available material is
Acetonitrile 215
Isopropyl alcohol 210
used, or a value of the absorptivity is taken from the literature.
Ethyl alcohol 210
Take care to specify this, by reporting values as “percentage
Methyl alcohol 210
against calibration material” or by noting that the accuracy of
Cyclohexane <210
Isooctane <210
the analysis is dependent upon a published value of the
A
Procedures for special purification of solvents for further improvement in the
absorptivity or molar absorptivity. (Areference must be cited.)
wavelength limit are given in Refs (1, 2). Solvents of high purity for use in
10.3.1 Some sample materials are highly fluorescent which
absorption spectroscopy also are available commercially.
cansignificantlyreducethemeasuredabsorbance.Theeffectof
samplefluorescencemayvarydependinguponthespectropho-
tometerandwavelengthchosen.Samplefluorescencemaybea
materials, are frequently used; both the composition of the
particular problem when using published absorptivity values.
buffer and the measured pH should be specified. Mixtures of
10.4 Types of Analyses (see Fig. 1):
0.1 M di-hydrogen sodium phosphate and 0.1 M hydrogen
di-sodium phosphate are useful in the 4.5 to 8.9 pH range. A 10.4.1 One Component, No Background Correction:
table of non-absorbing buffers has been presented by Abbott
C 5 Af/~abC ! (7)
s
(3).
10.4.2 One Component, Simple Background Correction:
10. Calculations
A 2 A 3f
~ !
1 2
C 5 (8)
10.1 Quantitative analysis by ultraviolet spectrophotometry
a bC
1 s
depends upon Beer’s law. The terms and symbols used are
where the subscripts refer to analytical wavelengths. The
those defined in Terminology E131. According to Beer’s law:
term A is the absorbance at the wavelength used for making a
A 5 abc 5 ~ε/M! 3bc (3)
simple subtractive correction. It is usually selected from
where: examination of the spectral curve of the reference material at a
wavelengthlongerthanthatofA ,preferablywherea ismuch
A = absorbance, 1 2
less than a .
a = absorptivity,
b = cell length, cm, 10.4.3 One Component, with Slope-Type Background Cor-
c = concentration, g/L,
rection:
ε = molar absorptivity, and
A 2 A 1S λ 2 λ f
@ ~ !#
1 2 2 1
M = molecular weight.
C 5 (9)
a bC
1 s
10.1.1 Inpractice,adistinctionmustbemadebetweenc,the
where:
concentration of the absorbing material in the cell at the time
S = slopebetweenwavelengths1and2forthebackground.
ofobservation,andtheconcentrationoftheabsorbingmaterial
in the sample as received. This is here designated as a mass
10.4.3.1 The background absorption is usually not linear
fraction C (g/g). The solution to be examined has a concentra-
between the analytical wavelength and the wavelength at
tion of sample in solution, C , which is in units of grams per
s
which a simple subtractive background correction may be
litre.
obtained. When it is possible to determine the slope between
c 5 A/ab (4) wavelengths 1 and 2 by observation of the samples that do not
contain the absorbing material that is to be determined, this
C 5 c/C 5 A/~abC ! (5)
s s
may be used as a correction for the background absorption.
10.2 If one or more dilutions are then made, the quantity
10.4.4 One Component, With Linear Background Correc-
calledthedilutionfactormustbeincluded.Dilutionfactor,f,is
tion:
the ratio of the final volume to the initial volume. If more than
10.4.4.1 The
...