Estimation of the Postmortem Duration of Mouse Tissue by Electron Spin Resonance Spectroscopy

Author:

Ito Shinobu12,Mori Tomohisa3,Kanazawa Hideko2,Sawaguchi Toshiko4

Affiliation:

1. I.T.O. Provitamin Research Center, 1-6-7-3F Nakamachi, Musashino, Tokyo, Japan

2. Faculty of Pharmacy, Keio University, 1-5-30 Shibakoen, Minato-ku, Tokyo 105-8512, Japan

3. Department of Pharmacology and Experimental Neuroscience, College of Medicine, University of Nebraska at Omaha, Omaha, NE 68182, USA

4. Department of Occupational Therapy, Faculty of Regional Health Therapy, Teikyo Heisei University, 4-1 Uruido-minami, Ichihara, Chiba, Japan

Abstract

Electron spin resonance (ESR) method is a simple method for detecting various free radicals simultaneously and directly. However, ESR spin trap method is unsuited to analyze weak ESR signals in organs because of water-induced dielectric loss (WIDL). To minimize WIDL occurring in biotissues and to improve detection sensitivity to free radicals in tissues, ESR cuvette was modified and used with 5,5-dimethtyl-1-pyrroline N-oxide (DMPO). The tissue samples were mouse brain, hart, lung, liver, kidney, pancreas, muscle, skin, and whole blood, where various ESR spin adduct signals including DMPO-ascorbyl radical (AsA), DMPO-superoxide anion radical (OOH), and DMPO-hydrogen radical (H) signal were detected. Postmortem changes in DMPO-AsAand DMPO-OOH were observed in various tissues of mouse. The signal peak of spin adduct was monitored until the 205th day postmortem. DMPO-AsAin liver (y=113.840.7 log (day),R1=-0.779,R2=0.6,P<.001) was found to linearly decrease with the logarithm of postmortem duration days. Therefore, DMPO-AsAsignal may be suitable for detecting an oxidation stress tracer from tissue in comparison with other spin adduct signal on ESR spin trap method.

Publisher

Hindawi Limited

Subject

Pharmacology,Toxicology

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