A spectrophotometric method for estimating hemin in biological systems | Health & Environmental Research Online (HERO)

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Citation
Tags

HERO ID

5015352

Reference Type

Journal Article

Title

A spectrophotometric method for estimating hemin in biological systems

Author(s)

Lombardo, ME; Araujo, LS; Ciccarelli, AB; Batlle, A

Year

2005

Is Peer Reviewed?

Yes

Journal

Analytical Biochemistry
ISSN: 0003-2697
EISSN: 1096-0309

Volume

341

Issue

Page Numbers

199-203

Language

English

PMID

15907864

DOI

10.1016/j.ab.2004.11.002

Abstract

Hemin chlorides exhibit two absorption maxima in the Soret region, one at about 360-380 nm (S' band) and the other between 400 and 430 nm (S band). We present here a simple and fast spectrophotometric assay to determine concentration of hemin between 1.15 and 9.20 microM employing the Soret region (S' band) as a reference. In this method the hemin is quantitatively extracted from biological materials by acidified chloroform. By recording the absorbance of the chloroform extract at its maximum peak at 388, 450, and 330 nm and applying the correction formula A(c)=2A388-(A450+A330), a very good linear correlation between the A(c) and the concentration of hemin is attained. The method can be used to estimate hemin in the presence of protein (0.06-5.00 mg/ml) and porphyrin (0.19-2.97 microM). Compared with the pyridine hemochromogen method, the assay reported here is highly reproducible, with 15- to 30-fold more sensitivity, and it allows the quantification of four times lower hemin concentrations.