Analyse von Protein-Protein-Wechselwirkungen und der <i>in vivo</i> Phosphorylierung des Sarkomerproteins Myomesin / Analysis of Protein-Protein Interactions and in vivo Phosphorylation of the Sarcomeric Protein Myomesin

Himmel, Mirko

January 2004

Für ein tiefergehendes Verständnis von Entwicklung und Funktion der quergestreiften Muskulatur ist eine Betrachtung der am Aufbau der Myofibrillen, den kontraktilen Organellen, beteiligten Proteine essentiell.<br> Die vorliegende Arbeit beschäftigt sich mit Myomesin, einem Protein der sarkomeren M-Bande. Zunächst wurde die cDNA des humanen Myomesins vollständig kloniert, sequenziert und nachfolgend die komplette Größe der aminoterminalen Kopfdomäne bestimmt. Es konnte gezeigt werden, daß Myomesin in vitro mit den Domänen 1 und 12 an Myosin bindet. Die muskelspezifische Isoform der Kreatinkinase bindet an die Domänen 7 und 8.<br> Stimulations- und Inhibitionsexperimente belegen, daß Myomesin an Serin 618 in vivo durch die Proteinkinase A phosphoryliert wird und daß diese Phosphorylierung durch Aktivierung beta2-adrenerger Rezeptoren stimulierbar ist. In Muskelgewebeproben von Patienten, die an der Hypertrophen Kardiomyopathie, einer genetisch bedingten Herzmuskelkrankheit, erkrankt sind, konnte mit einem neu hergestellten phosphorylierungsabhängigen Antikörper eine Verminderung der Menge phosphorylierten Myomesins nachgewiesen werden. Mögliche Ursachen werden diskutiert.<br> Myomesin bildet Dimere, wie durch hefegenetische und biochemische Experimente gezeigt werden konnte. Die Dimerisierung von Myomesin könnte eine zentrale Rolle für den Einbau der Myosinfilamente in die naszierende Myofibrille haben. Anhand der gewonnenen Daten wurde ein verbessertes Modell der zentralen M-Bande erstellt. / A deep understanding of the development and function of the sarcomeric muscle depends on the careful study of proteins involved in the assembly of myofibrills, the contractile organelles in cross-striated muscle.<br> This thesis deals with the sarcomeric M-band protein myomesin. First, the complete cDNA of human myomesin was cloned, sequenced, and subsequently the size of the aminoterminal head domain of myomesin was determined. Myomesin binds to myosin in vitro via domains 1 and 12. Musclespecific creatine kinase is binding to the domains 7 and 8 of myomesin.<br> Stimulation and inhibition experiments revealed, that serin 618 in human myomesin is phosphorylated in vivo by protein kinase A and that this phosphorylation can be stimulated by activation of beta2-adrenergic receptors. In muscle tissue of patients showing symptoms of the hypertrophic cardiomyopathy, a cardiac disease caused by genetic defects, the amount of phosphorylated myomesin was lowered as detected by a phosphospecific antibody which was established new.<br> Myomesin dimerizes as shown by yeast two hybrid and biochemical experiments. Myomesin dimerization could be a central point in myofibrillogenesis, when myosin filaments were incorporated in nascent myofibrills. Taking all the data together, an improved model of the central M-band was developed.

Proteine

Myofibrille

Sarkomer

Phosphorylierung

M-Bandenmodell

PKA

M-band model

PKA

Life sciences

Myofibrillens finstruktur i tvärstrimmig skelettmuskulatur

Edman, Anne-Christine

January 1988

The detailed structure of the myofibrillar material in fibres from different muscles has been studied. Specimens have been obtained from human muscles and from different muscles frequently examined in experimental studies. Both light- and electron microscopical techniques have been used. Of central importance has been the method, which makes it possible to prepare ultrathin sections of frozen tissue, i.e. cryo-ult- ramicrotomy. A number of techniques for image analysis have been applied in order to obtain objektive data from the micrographs. In Paper I the present knowledge about muscle fibre structure, cryo-- sectioning and image analysis is summarized and relevant methodological problems are discussed. Paper II describes the detailed structure of the C-zone of the A-band and shows, above all, that structures occur with different repeats along the long axis of the myofibril. Paper III describes the subcellular organization of different fibres in a homogeneous (based on enzyme histochemical mATPase) population, and shows that different structural characteristies can vary independently of each other. Paper IV describes the structural diversity of the myofibrillar M-band, and paper V the diversity of the myofilament fine structure in different fibres. The results show that there is a most sophisticated, and previosly unrealized, structural specialization both within the myofibrils and between myofibrils from different fibres and muscles, even if the fibres are of the same fibre type. The findings suggest that generally used models, showing the structural organization within myofibrils and myofilaments, are oversimplifications. The fibre population is more heterogeneously built up than the common systems for fibre type classification makes one to belive. / <p>Diss. (sammanfattning) Umeå : Umeå universitet, 1988, härtill 5 uppsatser.</p> / digitalisering@umu

Muscle

muscle fibre

fibre type

myofilament

A-band

M-band

cryo-ultramicrotomy

electron microscopy

image analysis

A unified approach to orthogonally multiplexed communication using wavelet bases and digital filter banks

Jones, William Wayne

January 1994

No description available.

orthogonally multiplexed communication

wavelet bases

digital filter banks

QAM symbols

M-band wavelets