Spectrophotometric Determination of Iron

Quantitative spectrophotometric analysis will be

employed to determine the concentration of iron in an
unknown solution.

A calibration curve for absorbance data for a series of

iron standards will be obtained. A linear equation
expressing the Beer-Lambert law will be used to
determine the concentration of iron in an unknown
sample.
Beer-Lambert Law: the fraction of incident light absorbed, A, is a function of
the thickness and the concentration of absorbing molecules in the light’s path.

A=εbC
ε = the molar absorptivity constant
b = optical path length, often 1 cm
C = the concentration in moles/liter

P 
A  log 0 
Inside a spectrophotometer P
Preparation of Standards: Mix and let stand.

•Add appropriate amounts of standard iron solution to volumetric flasks using

good burette techniques.

•Add hydroxylamine to reduce Fe3+ to Fe2+

2 Fe 3  2 NH 2OH  2 OH 1  2 Fe 2  N 2  4 H 2O

•Add sodium acetate salt, pH = 8

Add o-phenanthroline, AKA phen, bidentate ligand

Fe2   3 phen  Fe(phen)32

 Absorbance Spectrum

phen
Tris (1,10-phenanthroline)iron(II)
Red-orange complex
λmax = 508 nm
 Using the Genesys 20 Spectrophotometer

1.Allow the instrument to warm up for 30 minutes before using it.

2.Press A/T/C to select absorbance as the mode shown on the display.

3.Press nm▲or nm▼ to select the proper wavelength.

4.Insert you blank into the cell holder and close the sample door.

5.Press 0 ABS/100%T to set the black to 0 A.

6.Remove your blank, using the same curette, insert your sample into the cell
holder. The sample measurement appears on the LCD display.
 Curette Preparation Reminders:

Prepare a blank by filling an empty curette ¾ full with De-Ionized Water.

Seal the curette with a lid.

Remember:
 All curettes should be wiped clean and dry on the outside with a tissue.
 Handle curettes only by the top edge of the ribbed sides.
 All solutions should be free of bubbles.
 Always position the curette so the light path (indicated by the arrow)
passes through the clear walls.
Data Analysis

•Calculate the molarity of iron in the standard solutions, M1V1=M2V2

•Construct a Calibration Curve (Absorbance vs. Concentration).

(Directions for Excel 2007 available.)

Use the equation of the best fit line for your calibration curve to calculate
the amount of iron in your unknown.