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Article Type:

Perspective

Article History:

Received: 13 Mar. 2015

Revised: 11 June 2015

Accepted: 01 July 2015

ePublished: 26 July 2015

Keywords:

Thiobarbitoric acid reactive

substances

Oxidative stress

Biomarker

Abstract

Despite very wide variations of malondialdehyde (MDA) concentrations in biological samples, it is still used as a biomarker of oxidative stress in clinical investigations. In the current perspective study, we aimed to summarize a number of critical analytical points for determination of MDA. Technical problems and controversial findings in healthy people and some psychiatric disorders reveal that the reliability of MDA as a biomarker of oxidative stress needs to be re-evaluated by experts.

Malondialdehyde (MDA) is the most frequently used biomarker of oxidative stress in many health problems such as cancer, psychiatry chronic obstructive pulmonary disease, asthma, or cardiovascular diseases. This perspective study aimed to collect some evidence for low reliability of the MDA as a biomarker of oxidative stress. Our main hypothesis is that MDA assay is not able to provide valid analytical data for biological samples due to its high reactivity and possibility of various cross-reactions with co-existing biochemicals. Thiobarbitoric acid (TBA) assay is the most commonly used method for determination of the MDA in biological fluids.1 The assay is based on a condensation reaction of two molecules of TBA with one molecule of MDA, in which the reaction rate depends on temperature, pH and concentration of TBA. The reaction is carried out in acidic solution and temperature of ~ 100°C within one hour time course and most of MDA is produced during reaction process from decomposition of products of lipid peroxidation.2 The rapidity ease of use and cost of TBA assay made it the most common method in spite of some consideration and limitations of the method. These mainly are:

* Non-specificity of TBA reactivity on MDA3,4 and production of MDA from reactions other than lipid peroxidation.5 Concerning these characteristics of TBA assay and cross-reaction of other aldehydes produced from lipid peroxidation, most of researchers used total values of TBA reactive substances (TBARs) as a biomarker of oxidative stress instead of MDA values,

* Effects of procedural modifications on MDA-TBA adduct development,3

* Low stability of MDA in biological samples due to its high tendency for reacting with proteins, amino acids etc.6 and rapid enzymatic degradation,7

* Poor reproducibility of analytical results,4&9

* Low recovery test results.10

Variations of TBARs in biological samples of a number of psychiatric patients were investigated and compared with the values of healthy controls (for details see Table l).9,1136

In a more recent article, de Sousa et al19 compared plasma TBARs and some other markers in healthy individuals and patients with bipolar disorder (BD) before and after lithium therapy. Plasma samples were collected during two years, stored at -80°C and TBARs were measured using a spectrophotometric analysis. The reported TBARs for healthy controls was 62.74 ± 37.58 nmol/mL, those of BD patients before and after lithium therapy were 60.77 ± 45.14 and 37.88 ± 35.85 nmol/mL, respectively, and a significant decrease was observed from baseline to endpoint TBARs (p=0.023) in patients with lithium therapy.19 Decreased TBAR levels after lithium therapy (3.6 ± 0.3 vs. 5.1 ± 1.1 nmol/mL) has been confirmed by Machedo-Vieira et al,28 whereas no significant difference (6.33 ± 1.16 vs. 6.63 ± 1.15 nmol/mL) was observed in another investigation.17 Further, no change in TBAR levels in healthy people receiving lithium was observed by the same group of de Sousa.25 There are also other controversies on TBARs of healthy people (e.g., for plasma ranging from 0.6714 to 62.7410 nmol/mL) among various reports (Figs. 1 and 2). In both Figs. 1 and 2, one datum with very high deviation was excluded, however, significant variations were observed for healthy people, which is obviously questionable finding. One might consider analytical methods as a source of these discrepancies. When we considered a given analytical technique, namely, Wills method,11 discrepancies were still present varying from 0.67 ± 0.01 nmol/mL24 to 6.18 ± 0.58 nmol/mL.25 We would like to point out some considerations on TBARs measurements and to discuss their validity from a bioanalytical point of view. A number of reasons could be considered as possible causes of these observations including variations in sample preparation, storage, pre-treatment, and analysis which are briefly reviewed in this perspective. Full details could be found in a recent review article.37

There are some concerns in serum preparation, since TBARs are increased during coagulation process.38 In plasma preparation, one should consider the effects of EDTA on TBAR values. A significant increase in TBARs for plasma samples (1.39 ± 0.26 nmol/mL) treated with EDTA was reported when compared with the corresponding serum (1.07 ± 0.27 nmol/mL) and heparinized plasma (1.11 ±0.18 nmol/mL) samples.31

Storage of serum/plasma samples at -20°C without addition of antioxidants increased TBAR levels by a factor of two after 3-7 days and the addition of EDTA ± glutathione increased the stability of TBARs up to 35 days.31

Most of TBARs are produced during the heating of acidic solutions.2,39 Some authors claimed preventive effects of addition of butylated hydroxyl toluene40 and some others denied such effect.41 It has been shown that different acids and their concentrations could affect the results of TBAR assay.41

Measurement of TBARs using spectroscopic methods is simple, low cost, convenient, and widely used in clinical studies. Modifications were made on analytical conditions, therefore various values could be produced which make the comparison of reported values very difficult and even impossible. As mentioned above, poor selectivity of spectroscopic method is another disadvantage and the methods based on separation of analytes may overcome this limitation. However, some of these methods resulted in poor recovery, reproducibility, and repeatability values.42 As clearly noted by Wade and van Rij,43 most of problems associated with TBA assay were ignored by many researchers. Despite of these points, MDA is still used as an oxidative stress biomarker.44,45

Concerning above mentioned points on TBAR levels in healthy individuals and patients, controversial findings on TBARs in psychological disorders, official definitions of a biomarker,46 poor reproducibility, low repeatability, non-specificity, low stability of the standard solutions of TBA assay, and lack of full validation data of TBARs measurements in biological fluids, the reliability of TBARs as a biomarker of oxidative stress in the psychological disorders is questionable. As a conclusion, a number of bioanalytical points are summarized and the discussions on other viewpoints are open. We believe that MDA as an oxidative stress biomarker needs to be re-evaluated by an expert panel.

Acknowledgements

This communication is a part of PhD by research project of M. Khoubnasabjafari. Authors would like to thank the reviewers' comments on this submission and Tabriz University of Medical Sciences for partial financial support.

Ethical issues

There is none to be declared.

Competing interests

We have no conflicting interests with regard to the present submission.

Sidebar

Perspective Highlights

What is current knowledge?

V MDA is used as a biomarker of oxidative stress in various diseases despite its wide variations even in healthy people.

What is new here?

V According to the collected evidence, most of the technical problems on MDA measurement are unresolved and need further investigation, and the biomarker role of MDA should be re-evaluated by experts.

References

References

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AuthorAffiliation

Maryam Khoubnasabjafari1, Khalil Ansarin1, Abolghasem Jouyban2*

1 Tuberculosis and Lung Disease Research Center, Tabriz University of Medical Sciences, Tabriz, Iran

2 Drug Applied Research Center and Faculty of Pharmacy, Tabriz University of Medical Sciences, Tabriz, Iran

Corresponding author: Abolghasem Jouyban, Email: [email protected]

© 2015 The Author(s). This work is published by Bioimpacts as an open access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.Org/licenses/by-nc/4.0/). Non-commercial uses of the work are permitted, provided the original work is properly cited.

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Copyright Tabriz University of Medical Sciences 2015

Abstract

A significant increase in TBARs for plasma samples (1.39 ± 0.26 nmol/mL) treated with EDTA was reported when compared with the corresponding serum (1.07 ± 0.27 nmol/mL) and heparinized plasma (1.11 ±0.18 nmol/mL) samples.31 Storage of serum/plasma samples at -20°C without addition of antioxidants increased TBAR levels by a factor of two after 3-7 days and the addition of EDTA ± glutathione increased the stability of TBARs up to 35 days.31 Most of TBARs are produced during the heating of acidic solutions.2,39 Some authors claimed preventive effects of addition of butylated hydroxyl toluene40 and some others denied such effect.41 It has been shown that different acids and their concentrations could affect the results of TBAR assay.41 Measurement of TBARs using spectroscopic methods is simple, low cost, convenient, and widely used in clinical studies.

Details

Title
Reliability of malondialdehyde as a biomarker of oxidative stress in psychological disorders
Author
Khoubnasabjafari, Maryam; Ansarin, Khalil; Jouyban, Abolghasem
Pages
123-127
Section
Perspective
Publication year
2015
Publication date
2015
Publisher
Tabriz University of Medical Sciences
ISSN
22285652
e-ISSN
22285660
Source type
Scholarly Journal
Language of publication
English
ProQuest document ID
1746918864
Copyright
Copyright Tabriz University of Medical Sciences 2015