QUANTITATIVE PCR ANALYSIS REVEALS NOVEL EXPRESSION OF PROTHROMBIN mRNA AND REGULATION OF ITS LEVELS IN DEVELOPING MOUSE MUSCLE

Precise determination of mRNA levels is an essential element in any investigation of complex regulatory systems. Classical methodologies such as Northern hybridization suffer from requirements for significant samples of material and also a degree of non-specificity. Recently, quantitative techniques...

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Bibliographic Details
Published in:Thrombosis research 1997-08, Vol.87 (3), p.303-313
Main Authors: Citron, Bruce A, Smirnova, Irina V, Zoubine, Mikhail N, Festoff, Barry W
Format: Article
Language:English
Subjects:
Animals
Biological and medical sciences
Cells, Cultured
Cloning, Molecular
development
Fundamental and applied biological sciences. Psychology
Gene Expression Regulation, Developmental
Liver - metabolism
Mice
Mice, Inbred BALB C
muscle
Muscle Development
Muscle Proteins - biosynthesis
Muscle Proteins - genetics
Muscle, Skeletal - embryology
Muscle, Skeletal - growth & development
Muscle, Skeletal - metabolism
Organ Specificity
Polymerase Chain Reaction
Prothrombin
Prothrombin - biosynthesis
Prothrombin - genetics
qRT-PCR
RNA, Messenger - analysis
RNA, Messenger - biosynthesis
RNA, Messenger - genetics
Striated muscle. Tendons
Synapses - metabolism
Vertebrates: osteoarticular system, musculoskeletal system
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Summary:Precise determination of mRNA levels is an essential element in any investigation of complex regulatory systems. Classical methodologies such as Northern hybridization suffer from requirements for significant samples of material and also a degree of non-specificity. Recently, quantitative techniques involving PCR amplification have been devised. We have developed and applied such procedures to the determination of prothrombin messages in skeletal muscle cells during development. In addition to its role in the blood coagulation cascade, the serine protease thrombin has been shown to participate in several signaling events in the neuromuscular system. The inactive precursor, prothrombin, primarily produced in the liver, has also been shown to be synthesized and developmentally-regulated in the brain. In skeletal muscle, thrombin is a mediator of activity-dependent polyneuronal synapse elimination (ADPSE) which occurs in early postnatal development. Recent experiments showing that thrombin is released from myotubes in culture under the influence of acetylcholine suggest that locally-synthesized prothrombin may be the source of this Hebbian synaptic interaction. We have determined that prothrombin is expressed in skeletal muscle, as the likely source of thrombin involved in ADPSE, and the current results show the quantitative expression of muscle prothrombin during this time of intense synapse remodeling. Published by Elsevier Science Ltd
ISSN:0049-3848
1879-2472
DOI:10.1016/S0049-3848(97)00132-1