Urinary Iodine-Method A

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IODINE DEFICIENCY DISORDERS

annex

Method for measuring urinary iodine


using ammonium persulfate (Method A)

Principle
Urine is digested with ammonium persulfate. Iodide is the catalyst in the
reduction of ceric ammonium sulfate (yellow) to cerous form (colourless), and
is detected by rate of colour disappearance (Sandell-Kolthoff reaction).

Equipment
Heating block (vented fume hood not necessary), colorimeter, thermometer,
test tubes (13 x 100 mm), reagent flasks and bottles, pipettes, balance scales.

Reagents
1.
2.
3.
4.
5.
6.
7.

Ammonium persulfate (analytical grade)


As2O3
NaCl
H2SO4
Ce(NH4)4(SO4)4.2H2O
Deionized H2O
KIO3

Solutions
1.0 M Ammonium persulfate: Dissolve 114.1 g H2N2O8S2 in H2O; make up
to 500 ml with H2O. Store away from light. Stable for at least one month.
5 N H2SO4: Slowly add 139 ml concentrated (36 N) H2SO4 to about 700 ml
deionized water (careful - this generates heat!). When cool, adjust with
deionized water to a final volume of 1 litre.
Arsenious acid solution: In a 2000 ml Erlenmeyer flask, place 20 g As2O3
and 50 g NaCl, then slowly add 400 ml 5 N H2SO4. Add water to about 1 litre,
heat gently to dissolve, cool to room temperature, dilute with water to 2 litres,
filter, store in a dark bottle away from light at room temperature. The solution
is stable for months.

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IODINE DEFICIENCY DISORDERS

Ceric ammonium sulfate solution: Dissolve 48 g ceric ammonium sulfate


in 1 litre 3.5 N H2SO4. (The 3.5 N H2SO4 is made by slowly adding 97 ml
concentrated (36 N) H2SO4 to about 800 ml deionized water (careful - this
generates heat!), and when cool, adjusting with deionized water to a final
volume of 1 litre). Store in a dark bottle away from light at room temperature.
The solution is stable for months.
Standard iodine solution, 1 g iodine/ml (7.9 mol/l): Dissolve 0.168 mg
KIO3 in deionized water to a final volume of 100 ml (1.68 mg KIO3 contains
1.0 mg iodine; KIO 3 is preferred over KI because it is more stable,
but KI has been used by some laboratories without apparent problems).
It may be more convenient to make a more concentrated solution, e.g., 10 or
100 mg iodine/ml, then dilute to 1 g/ml. Store in a dark bottle. The solution is
stable for months. Useful standards are 20, 50, 100, 150, 200, and 300 g/l.

Procedure
1. Mix urine to suspend sediment.
2. Pipette 250 l of each urine sample into a 13 x 100 mm test tube. Pipette
each iodine standard into a test tube, and then add H2O as needed to make a
final volume of 250 l. Duplicate iodine standards and a set of internal urine
standards should be included in each assay.
3. Add 1 ml 1.0 M ammonium persulfate to each tube.
4. Heat all tubes for 60 minutes at 100oC.
5. Cool tubes to room temperature.
6. Add 2.5 ml arsenious acid solution. Mix by inversion or vortex. Let stand
for 15 minutes.
7. Add 300 l of ceric ammonium sulfate solution to each tube (quickly mixing)
at 15-30 second intervals between successive tubes. A stopwatch should be
used for this. With practice, a 15 second interval is convenient.
8. Allow to sit at room temperature. Exactly 30 minutes after addition of ceric
ammonium sulfate to the first tube, read its absorbance at 420 nm.
Read successive tubes at the same interval as when adding the ceric
ammonium sulfate.

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IODINE DEFICIENCY DISORDERS

Calculation of results
Construct a standard curve on graph paper by plotting iodine concentration of
each standard on the abscissa against its optical density at 405 g/l (OD405)
on the ordinate.

Notes
1. This is modified from the former method (see reference below), substituting
ammonium persulfate for chloric acid (more toxic) as digestant.
2. Since the digestion procedure has no specific end-point, it is essential to run blanks
and standards with each assay to allow for variations in heating time, etc.
3. The exact temperature, heating time, and cooling time may vary. However,
within each assay, the interval between the time of addition of ceric
ammonium sulfate and the time of the reading must be the same for all samples,
standards, and blanks.
4. With the longer ceric ammonium sulfate incubation and with 15 second
interval additions of CAS, up to 120 tubes can be read in a single assay.
5. The volumes and proportions of samples and reagents can be varied
to achieve different concentrations or a different curve shape, if conditions
warrant. If different tube sizes are used, corresponding sized holes in the
heating block are also needed.
6. If necessary, this method could probably be applied without a heating block,
using a water, oil, or sand bath, but this is not recommended. It is essential
that all tubes be uniformly heated and that the temperature be constant within
the range described above.
7. Test tubes can be reused if they are carefully washed to eliminate any
iodine contamination.
8. Various steps of this procedure are suitable for automation. For example,
the colorimetric readings can be done in microtiter plates with a scanner, and
the standard curves plotted and read on a simple desk computer.

Reference
ICCIDD, UNICEF, WHO. Dunn JT et al. Methods for measuring iodine in
urine. The Netherlands, ICCIDD, 1993.

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