Electrophoretic and computer analysis of skeletal muscle used for cardiac assistance

O'Brien, Geraldine A.; Cumming, D. V. E.; Pattison, C W; Corbett, Joseph M.; Dünn, Michael J.; Yacoub, Magdi H.

doi:10.1002/elps.1150120716

Cited by 5 publications

(1 citation statement)

References 22 publications

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“…The minigel format was the major factor in reducing processing time. Although other investigators have endeavored to improve protein separation by employing gels as large as 21 cm, the resolution obtained with the 8 X 7 cm gels employed in this study was very satisfactory [8]. Commercially available silver stains provided excellent results in 1 h. The practicality of this technique is underscored by the ability of a single operator to process multiple gels within a single day This rapid high-resolution 2-D PAGE technique for human sperm proteins may be useful for a variety of applications.…”

Section: Discussionmentioning

confidence: 70%

Rapid high resolution two‐dimensional electrophoresis of human sperm proteins

et al. 1992

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An improved protocol has been developed for two-dimensional gel analysis of human sperm proteins through the application of recent technical advances. Advantages of this protocol consist of increased resolving power, reduced processing time, enhanced reproducibility of staining patterns, and applicability to small quantities of protein. Technical improvements include determination of optimal protein loading (20 micrograms/gel), development of a reliable tube gel casting system, and application of minigel technology. In this study over 500 proteins were resolved with molecular weights ranging from 12,000 to 105,000 and isoelectric points from 5.0 to 8.5. This is a three-fold improvement in resolution over earlier results. A single operator was able to generate two-dimensional gels of multiple samples in less than one day. This rapid high resolution technique should facilitate further investigation of human sperm proteins under normal and pathologic conditions.

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Section: Discussionmentioning

confidence: 70%

Rapid high resolution two‐dimensional electrophoresis of human sperm proteins

et al. 1992

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A human myocardial two‐dimensional electrophoresis database: Protein characterisation by microsequencing and immunoblotting

et al. 1992

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This communication briefly describes how a human heart two-dimensional electrophoresis (2-DE) protein database is being established in our laboratory. The database contains more than 1500 polypeptides and approximately fifty proteins from 2-DE gels of human myocardial tissue have been characterised. Information about the proteins has been compiled including molecular weight (M(r)), isoelectric point (pI), sample spot (SSP) number, protein name, partial sequence, and antibody reacting with the protein. The first stage of this project involves the investigation of protein with pIs in the range pH 4-7. Future studies will employ immobilised pH gradient (IPG) gels as the first dimension of the 2-DE to examine basic proteins. The ultimate goal of this project is to establish a global picture of human heart protein expression in both normal and disease conditions.

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Electrophoretic analysis of electrically trained skeletal muscle

et al. 1992

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Sheep latissimus dorsi muscle was electrically trained, thereby inducing fast-to-slow fibre-type transformation. Using a combination of one- and two-dimensional gel electrophoresis techniques with computer analysis, we have analysed altered expression of contractile protein isoforms at protein and mRNA level over a time course of electrical training extending to 5 months. Myosin heavy chain and regulatory myosin light chain analysis showed predominant expression of their slow isoforms (86% and 92%, respectively) after 3 months of training. At the same time point, however, tropomyosin analysis revealed that the slow isoform of the alpha-subunit accounted for 64% of the total alpha expression. Troponin T isoform switching proceeded more slowly over the same time course than tropomyosin and the thick filament proteins studied. Troponin T analysis revealed 5 fast and 2 slow isoforms in the sheep, of which the second slow isoform only became clearly visible after 5 months' training. At this time point the two slow isoforms were more predominant than their fast counterparts. This suggests that a wide heterogeneity of fast and slow isoform combinations are possible in the thin filament of skeletal muscle.

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Electrophoretic and computer analysis of skeletal muscle used for cardiac assistance

Cited by 5 publications

References 22 publications

Rapid high resolution two‐dimensional electrophoresis of human sperm proteins

Rapid high resolution two‐dimensional electrophoresis of human sperm proteins

A human myocardial two‐dimensional electrophoresis database: Protein characterisation by microsequencing and immunoblotting

Electrophoretic analysis of electrically trained skeletal muscle

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