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Preservation of rat skeletal muscle energy metabolism by illumination.

Artikel i vetenskaplig tidskrift
Författare Ann Lindgård
Jonas Lundberg
Olivier Rakotonirainy
Anna Elander
Bassam Soussi
Publicerad i Life sciences
Volym 72
Nummer/häfte 23
Sidor 2649-58
ISSN 0024-3205
Publiceringsår 2003
Publicerad vid Institutionen för de kirurgiska disciplinerna, Avdelningen för plastikkirurgi
Institutionen för de kirurgiska disciplinerna, Avdelningen för kirurgi
Sidor 2649-58
Språk en
Länkar www.ncbi.nlm.nih.gov/entrez/query.f...
Ämnesord Adenosine Triphosphate, analysis, Animals, Citrates, pharmacology, Energy Metabolism, Female, Glucose-6-Phosphate, analysis, Hindlimb, Inosine Monophosphate, analysis, Light, Lighting, Magnetic Resonance Spectroscopy, Muscle, Skeletal, metabolism, Phosphates, analysis, Phosphocreatine, analysis, Phosphorus Isotopes, diagnostic use, Rats, Rats, Sprague-Dawley, Singlet Oxygen, Solutions, pharmacology, Tissue Preservation, methods
Ämneskategorier Plastikkirurgi

Sammanfattning

Skeletal muscle viability is crucially dependent on the tissue levels of its high energy phosphates. In this study we investigated the effect of the preservation medium Perfadex and illumination with Singlet Oxygen Energy (SOE). Singlet oxygen can be produced photochemically by energy transfer from an excited photosensitizer. The energy emitted from singlet oxygen upon relaxation to its triplet state is captured as photons at 634 nm and is here referred to as SOE. Rat hind limb rectus femoris muscles were preserved for five hours at 22 degrees C in Perfadex, saline, SOE illuminated Perfadex or SOE illuminated saline. Extracts of the muscles were analysed by 31P NMR. Data were analysed using two-way analysis of variance and are given as mean values micromol/g dry weight) +/- SEM. The ATP concentration was higher (p = 0.006) in saline groups (4.52) compared with Perfadex groups (2.82). There was no statistically significant difference in PCr between the saline groups (1.25) and Perfadex groups (0.82). However, there were higher (p = 0.003) ATP in the SOE illuminated groups (4.61) compared with the non-illuminated groups (2.73). The PCr was also higher (p < 0.0001) in the SOE illuminated groups (1.89) compared with the non-illuminated groups (0.18). In conclusion, Perfadex in this experimental model was incapable of preserving the high energy phosphates in skeletal muscle during 5 hours of ischemia. Illumination with SOE at 634 nm improved the preservation potential, in terms of a positive effect on the energy status of the muscle cell.

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