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By Christopher Burgess
Pharmaceutical Technology
Most analytical procedures rely on the accurate preparation of reference standard solutions. It is common practice to prepare
such solutions volumetrically using standard glassware. Usually a stock solution is prepared followed by a dilution or series of
dilutions to arrive at a working concentration of the reference standard. This column looks at the effects of choice of dilution
schemes on the accuracy of the prepared reference standard.
A previous column looked at the basics of measurement uncertainty and related it to the direct preparation of a standard solution
were discussed (1). This column will review the preparation of standard solutions by simple and serial dilution using standard
pipettes and flasks. Only the uncertainties in the volumetric glassware, however, will be considered to answer the question: “Is
my dilution accurate enough?” It will be assumed that all the other factors (e.g., operator variability when pipetting or making
up to the mark, temperature, and solvent effects) are constant.
Further, it will be assumed that standard Grade A glassware are being used (2). Accuracy in the context of this column is the
International Organization for Standardization (ISO) definition. In ISO, accuracy combines the concepts of unbiasedness
(termed trueness) and precision (3).
Suppose an analytical procedure states that a standard solution of 1 mg per liter is required by dilution of a 50 mg/L stock
solution. The question arises “What is the ‘best way’ to perform this dilution volumetrically?” The ‘best way’ would be to have
minimal dilution error (i.e., smallest measurement uncertainty commensurate with the analytical need). This column will only
consider some whole number dilutions, but the principles apply to any dilution or dilution sequence.
Equation 1
Hence, for a sequence 20 to 1000 followed by 25 to 500, C would be 1/1000 or a dilution of 1000:1.
Consider the number of combinations of standard glassware to make a single dilution. Assume that in the laboratory, there are
pipettes from 1 mL to 25 mL and volumetric flasks from 5 mL to 1000 mL. Table II illustrates single step whole number
dilution ratios from 5 to 1000. The dilution ratio here is 1/C of Equation 2.
Equation 2
Based on error propagation theory (7), the combination of relative errors for any pipette (Pi)/flask (Fi)dilution combination
sequence of n steps can be calculated from Equation 3 and the results are shown in Table III.
Equation 3
Table III : Combined relative uncertainties for a single dilution, uc, for
combinations of pipettes and flasks in mL.
In this example of preparing a 1 mg per liter dilution from a 50 mg/L stock solution in a single step, five combinations can be
selected from Table II; 1 to 50, 2 to 100, 5 to 250, 10 to 500, and 20 to 1000. Do they all have the same accuracy? To answer
this question, look up the appropriate combined relative uncertainties in Table II.
For all the combinations in Table II, Table III gives the combined uncertainties as a %.
From Table III, the bigger the pipette and the bigger the flask is, the lower the combined relative standard uncertainty. Larger
amounts of both solvent and solute, however, are needed to achieve a factor of 5 gain from a single dilution.
Returning to the 50-fold dilution, this effect is illustrated (Table IV) as the 20 to 1000 dilution produces a lower uncertainty by a
factor of four compared with the 1 to 50 dilution. This comes at a cost of solvent and solute. So what is ‘best for you’? The 1
to 50 dilution may be perfectly acceptable.
Table IV: 50-fold dilution examples and the relative contributions compared with
the 1- to 50-dilution step.
Suppose, however, the laboratory wanted to achieve this 1:50 dilution with minimum solvent and solute usage by preparing a
stock solution in a 10-mL flask and serially diluting it 1 to 5 and then 1 to 10. The resulting standard uncertainty from volumetric
sources would be seen in Equation 4.
Equation 4
The numerical values are taken from the ux/x values in Tables I and III. Note that this value is slightly different from the value
in Table IV. This is because there is a small contribution from the original 10-mL flask.
Ignoring the uncertainty contribution associated with weighing 0.5 mg of a reference standard, the volumetric uncertainty due to
the serial dilution is 0.40%, which is 1.6 times larger than a simple 1 to 50 dilution. Bearing in mind that at a coverage factor, k,
of 2 (95.45% Confidence), the volumetric uncertainty alone would approach 1%. In this instance, a complete error budget
calculation would probably show that the overall uncertainty at a coverage factor of 2 might be too large from this sequence to be
employed in practice for an assay standard.
Quite often a 1000-fold dilution is needed. Table V shows three examples. In the first one, it is a simple one-step 1 to 1000
dilution resulting in a reasonably accurate result. However, it requires a lot of solvent. A three-stage serial dilution process is
attractive to reduce solvent usage. The smallest serial dilution process is three 1.00 to 10.0 dilution steps. This dilution sequence
results in about twice the measurement uncertainty. However, three 5.00 to 50.0 dilution steps or three 10.00 to 100.0 dilution
steps could also be used to achieve the same dilution. The three 5.00 to 50.0 dilution steps shows not only an improvement of
about half the measurement uncertainty of the 1000-fold dilution, it also saves approximately 75% of the solvent. There is no
advantage in using three 10.00 to 100.0 dilution steps over three 5.00 to 50.0 dilution and it uses twice as much solvent.
Table V: Dilution sequences for 1000:1 and % relative error with solvent usage.
Conclusion
As analytical procedures rely on the accurate preparation of reference standard solutions, it is important to know what the
probable effect of analytical operations will be on the overall measurement uncertainty of the analytical result. Whereas
volumetric dilution errors are small, they are not insignificant. The structure of dilution sequences can play a significant role in
contributing to an uncertainty budget. Examples in this column have demonstrated both the method of estimation and extent of
uncertainty contributions.
References
1. C. Burgess, Pharm. Techn., 37(9) 62-64, 73 (2013).
2. ISO 648:2008 Laboratory glassware. Single-volume pipettes. ISO 1042:2000 Laboratory Glassware - One-mark volumetric
flasks
3. S L R Ellison and A Williams (Eds). Eurachem/CITAC guide: Quantifying Uncertainty in Analytical Measurement, 3rd
Edition, (2012) ISBN 978-0-948926-30-3.
4. R. B. Lam and T. L. Isenhour, Anal. Chem., 52(7), 1158 -1161 (1980).
5. Y Hayashi and R Matsuda, Analytical Sciences, 10(6) 881-888 (Japan Society for Analytical Chemistry, 1994).
6. D. A. Skoog, D.M. West, F J Holler, Fundamentals of Analytical Chemistry, 7th edition, 798-808 (Saunders College
Publishing, 1996).
7. A.A. Clifford, Multivariate Error Analysis, Applied Science Publishers (Wiley, New York, 1973).
Article Details
Pharmaceutical Technology
Vol. 39, Issue 1
Pages: 62–64
Citation: When referring to this article, please cite as C. Burgess, “How Accurate are Your Dilutions?,” Pharmaceutical
Technology39(1) 2015.