Temat: myosin - Katalog OPAC zbiorów

Skocz do pozycji: 1.

Tytuł:: A new method to precipitate myosin v from rat brain soluble fraction
Autorzy:: Melo, Hugo
Coelho, Milton
Powiązania:: https://bibliotekanauki.pl/articles/1041042.pdf
Data publikacji:: 2007
Wydawca:: Polskie Towarzystwo Biochemiczne
Tematy:: myosin V
ATPase
F-actin
Opis:: Myosin can be precipitated from soluble fraction under different assay conditions. This paper describes a new method for precipitating myosin V from rat brain soluble fraction. Brains were homogenized in 50 mM imidazole/HCl buffer, pH 8.0, containing 10 mM EDTA/EGTA, 250 mM sucrose, 1 mM DTT and 1 mM benzamidine, centrifuged at 45000 × g for 40 min and the supernatant was frozen at -20 °C. Forty-eight hours later, the supernatant was thawed, centrifuged at 45000 × g for 40 min and the precipitate was washed in 20 mM imidazole buffer pH 8.0. SDS/PAGE analysis showed four polypeptides in the precipitate: 205, 150, 57 and 43 kDa. The precipitate presented high Mg2+-ATPase activity, which co-purifies with p205. This polypeptide was recognized by a specific myosin V antibody and was proteolised by calpain, generating two stable polypeptides: p130 and p90. The Mg2+-ATPase activity was not stimulated by calcium in both the absence and presence of exogenous calmodulin and the K+/EDTA-ATPase activity represented 25% of the Mg2+-ATPase activity. In this work, myosin V from rat brain was precipitated by freezing the soluble fraction and was co-purificated with a 45 kDa polypeptide.
Źródło:: Acta Biochimica Polonica; 2007, 54, 3; 575-581
0001-527X
Pojawia się w:: Acta Biochimica Polonica
Dostawca treści:: Biblioteka Nauki

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Skocz do pozycji: 2.

Tytuł:: Aktyna i miozyny w jądrze komórkowym
Actins and myosins in the nucleus
Autorzy:: Nowak, Jolanta
Rędowicz, Maria
Powiązania:: https://bibliotekanauki.pl/articles/1033936.pdf
Data publikacji:: 2018
Wydawca:: Polskie Towarzystwo Przyrodników im. Kopernika
Tematy:: actin
gene expression
myosin
nucleus
nucleolus
polymerase
transcription
aktyna
ekspresja genów
miozyna
jądro
jąderko
polimeraza
transkrypcja
Opis:: Aktyna i miozyna to białka kojarzone przede wszystkim z ich kluczową rolą w generacji skurczu mięśni. Natomiast poza izoformami charakterystycznymi dla mięśni są również izoformy aktyny i miozyny, które występują we wszystkich typach komórek i tkanek (patrz artykuł Suszek i współaut. w tym zeszycie KOSMOSU). Badania prowadzone w ostatnich dwóch dekadach wykazały niezbicie, że zarówno aktyna (i szereg białek wiążących aktynę) oraz liczne miozyny (przedstawiciele rodzin I, II, V, VI, XVI i XVIII) lokalizują się w jądrze komórkowym gdzie są zaangażowane w procesy transkrypcji i naprawy DNA, transport w nukleoplazmie oraz import i eksport jądrowy, a także w utrzymywanie architektury jądra. Niniejszy artykuł opisuje dotychczasowy stan wiedzy o roli układu akto-miozynowego w jądrze komórkowym.
Actin and myosins are the proteins mainly known from their key roles in muscle contraction. However, besides typical muscle isoforms there are actins and myosins that are present in all cell and tissue types. Studies performed within the last two decades have irrefutably shown that both the cytoplasmic actin isoforms (along with numerous actin-binding proteins) as well as many myosins (representing class I, II, V, VI, XVI and XVIII) are present within the nucleus. They play important roles in nuclear processes as they are involved in transcription and DNA repair, intranuclear transport as well as nuclear import and export, and in maintenance of nuclear architecture. This article describes the current knowledge on the acto-myosin system in this biggest cellular compartment.
Źródło:: Kosmos; 2018, 67, 1; 75-93
0023-4249
Pojawia się w:: Kosmos
Dostawca treści:: Biblioteka Nauki

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Skocz do pozycji: 3.

Tytuł:: Chicken meat proteins as potential precursors of bioactive peptides
Autorzy:: Dziuba, J.
Minkiewicz, P.
Plitnik, K.
Powiązania:: https://bibliotekanauki.pl/articles/1371527.pdf
Data publikacji:: 1996
Wydawca:: Instytut Rozrodu Zwierząt i Badań Żywności Polskiej Akademii Nauk w Olsztynie
Tematy:: peptide
proteolysis
food biochemistry
tropomyosin
Gallus gallus
collagen
meat protein
chicken meat
myosin
troponin
bioactive peptide
protein
chicken
Opis:: Amino acid sequences of chicken (Gallus gallus) meat proteins: myosin, tropomyosin, troponin, collagen and connectin taken from SWISS-PROT and EMBL databases have been analysed using "PROTEIN" computer program searching for fragments identical to bioactive peptides and for bonds susceptible to the action of endopeptidases in protein chains. Chicken meat proteins contain fragments with antihypertensive (connectin), immunomodulating (myosin, tropomyosin, collagen), antithrombotic (collagen), antibacterial (collagen), embryotoxic (collagen) activity and also neuroactive (myosin, collagen, connectin) occurring in amino acid sequences with the frequency higher than that expected from the probability of appearance of given fragments in random amino acid sequences. There is a theoretical possibility of release of bioactive fragments from chicken meat proteins by endopeptidases. Such possibility especially occurs in the case of hydrolysis by proteinase K (EC 3.4.21.14). The frequency of occurrence of bioactive fragments may be applied for quantitative comparison of value of proteins as a source of bioactive peptides, although different affinity of bioactive fragments to their receptors and different susceptibility of proteins to proteolysis should be taken into consideration.
Sekwencje aminokwasowe białek mięsa kurcząt (Gallus gallus): miozyny, tropomiozyny, troponiny, kolagenu i konektyny pochodzące z baz danych SWISS-PROT i E MB L były analizowane za pomocą programu komputerowego PROTEIN wyszukującego w łańcuchach białek fragmenty identyczne z sekwencjami bioaktywnych peptydów oraz wiązania podatne na działanie endopeptydaz. Białka mięsa kurcząt zawierają fragmenty o aktywności przeciwnadciśnieniowej (konektyna) (rys. 3), immunomodulacyjnej (miozyna, tropomiozyna, kolagen), przeciwkrzepliwej (kolagen), antybakteryjnej (kolagen), embriotoksycznej (kolagen) (rys. 2) oraz neuroaktywne (miozyna, kolagen, konektyna) (rys. 2, 3) występujące w sekwencjach aminokwasowych z częstością większą, niż przewidywana na podstawie prawdopodobieństwa pojawienia się danych fragmentów w przypadkowych sekwencjach aminokwasowych (rys. 1). Istnieje teoretyczna możliwość uwalniania bioaktywnych peptydów z białek mięsa kurcząt przez endopeptydazy. Taka możliwość istnieje szczególnie w przypadku hydrolizy przez proteinazę K (EC 3.4.21.14) (rys. 2 i 3). Częstość występowania bioaktywnych fragmentów może służyć do ilościowego porównywania potencjalnej wartości białek jako źródła bioaktywnych peptydów, chociaż musi być uwzględnione także różne powinowactwo fragmentów do ich receptorów oraz różna podatność białek na proteolizę.
Źródło:: Polish Journal of Food and Nutrition Sciences; 1996, 05, 4; 85-96
1230-0322
2083-6007
Pojawia się w:: Polish Journal of Food and Nutrition Sciences
Dostawca treści:: Biblioteka Nauki

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Skocz do pozycji: 4.

Tytuł:: Is MLC phosphorylation essential for the recovery from ROCK inhibition in glioma C6 cells?
Autorzy:: Korczyński, Jarosław
Sobierajska, Katarzyna
Krzemiński, Patryk
Wasik, Anna
Wypych, Dorota
Pomorski, Paweł
Kłopocka, Wanda
Powiązania:: https://bibliotekanauki.pl/articles/1039964.pdf
Data publikacji:: 2011
Wydawca:: Polskie Towarzystwo Biochemiczne
Tematy:: RhoA
myosin II
calcium signaling
actin
MLC phosphorylation
Opis:: Inhibition of Rho-associated protein kinase (ROCK) activity in glioma C6 cells induces changes in actin cytoskeleton organization and cell morphology similar to those observed in other types of cells with inhibited RhoA/ROCK signaling pathway. We show that phosphorylation of myosin light chains (MLC) induced by P2Y2 receptor stimulation in cells with blocked ROCK correlates in time with actin cytoskeleton reorganization, F-actin redistribution and stress fibers assembly followed by recovery of normal cell morphology. Presented results indicate that myosin light-chain kinase (MLCK) is responsible for the observed phosphorylation of MLC. We also found that the changes induced by P2Y2 stimulation in actin cytoskeleton dynamics and morphology of cells with inhibited ROCK, but not in the level of phosphorylated MLC, depend on the presence of calcium in the cell environment.
Źródło:: Acta Biochimica Polonica; 2011, 58, 1; 125-130
0001-527X
Pojawia się w:: Acta Biochimica Polonica
Dostawca treści:: Biblioteka Nauki

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Skocz do pozycji: 5.

Tytuł:: Myosin molecule packing within the vertebrate skeletal muscle thick filaments. A complete bipolar model*
Autorzy:: Skubiszak, Ludmila
Kowalczyk, Leszek
Powiązania:: https://bibliotekanauki.pl/articles/1043686.pdf
Data publikacji:: 2002
Wydawca:: Polskie Towarzystwo Biochemiczne
Tematy:: thick filament
computer modelling
myosin molecule packing
vertebrate skeletal muscle
cross-bridge action
Opis:: Computer modelling related to the real dimensions of both the whole filament and the myosin molecule subfragments has revealed two alternative modes for myosin molecule packing which lead to the head disposition similar to that observed by EM on the surface of the cross-bridge zone of the relaxed vertebrate skeletal muscle thick filaments. One of the modes has been known for three decades and is usually incorporated into the so-called three-stranded model. The new mode differs from the former one in two aspects: (1) myosin heads are grouped into asymmetrical cross-bridge crowns instead of symmetrical ones; (2) not the whole myosin tail, but only a 43-nm C-terminus of each of them is straightened and near-parallel to the filament axis, the rest of the tail is twisted. Concurrent exploration of these alternative modes has revealed their influence on the filament features. The parameter values for the filament models as well as for the building units depicting the myosin molecule subfragments are verified by experimental data found in the literature. On the basis of the new mode for myosin molecule packing a complete bipolar structure of the thick filament is created.
Źródło:: Acta Biochimica Polonica; 2002, 49, 4; 829-840
0001-527X
Pojawia się w:: Acta Biochimica Polonica
Dostawca treści:: Biblioteka Nauki

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Skocz do pozycji: 6.

Tytuł:: Myosin VI is associated with secretory granules and is present in the nucleus in adrenal medulla chromaffin cells
Autorzy:: Majewski, Łukasz
Sobczak, Magdalena
Rędowicz, Maria
Powiązania:: https://bibliotekanauki.pl/articles/1040436.pdf
Data publikacji:: 2010
Wydawca:: Polskie Towarzystwo Biochemiczne
Tematy:: myosin VI
chromaffin granules
PC12 cells
Golgi apparatus
Opis:: Myosin VI (MVI) is the only known myosin walking towards minus end of actin filaments. Here, MVI, but not myosins IB or IIB, was detected in chromaffin granules isolated from bovine medulla and found to be tightly associated with the granule apical surface. MVI also localized to secretory granules within rat pheochromocytoma PC12 cells as well as to the Golgi apparatus, endoplasmic reticulum and clathrin-coated pits. Notably, it was also found in the nucleus. RT-PCR revealed that MVI splice variants with a large insert (LI), characteristic of polarized cells, were barely detectable in PC12 cells, whereas variants with a small insert (SI) were the major isoforms. The presented data indicate that MVI in adrenal medulla cells is engaged in secretory vesicle trafficking within the cytoplasm and possibly also involved in transport within the nucleus.
Źródło:: Acta Biochimica Polonica; 2010, 57, 1; 109-114
0001-527X
Pojawia się w:: Acta Biochimica Polonica
Dostawca treści:: Biblioteka Nauki

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Skocz do pozycji: 7.

Tytuł:: Myosins and pathology: genetics and biology.
Autorzy:: Rędowicz, Maria
Powiązania:: https://bibliotekanauki.pl/articles/1043680.pdf
Data publikacji:: 2002
Wydawca:: Polskie Towarzystwo Biochemiczne
Tematy:: vision
cardiomyopathy
myosin
pathology
deafness
Opis:: This article summarizes current knowledge on the genetics and possible molecular mechanisms of human pathologies resulted from mutations within the genes encoding several myosin isoforms. Mutations within the genes encoding some myosin isoforms have been found to be responsible for blindness (myosins III and VIIA), deafness (myosins I, IIA, IIIA, VI, VIIA and XV) and familial hypertrophic cardiomyopathy (β cardiac myosin heavy chain and both the regulatory and essential light chains). Myosin III localizes predominantly to photoreceptor cells and is proved to be engaged in the vision process in Drosophila. In the inner ear, myosin I is postulated to play a role as an adaptive motor in the tip links of stereocilia of hair cells, myosin IIA seems to be responsible for stabilizing the contacts between adjacent inner ear hair cells, myosin VI plays a role as an intracellular motor transporting membrane structures within the hair cells while myosin VIIA most probably participates in forming links between neighbouring stereocilia and myosin XV probably stabilizes the stereocilia structure. About 30% of patients with familial hypertrophic cardiomyopathy have mutations within the genes encoding the β cardiac myosin heavy chain and both light chains that are grouped within the regions of myosin head crucial for its functions. The alterations lead to the destabilization of sarcomeres and to a decrease of the myosin ATPase activity and its ability to move actin filaments.
Źródło:: Acta Biochimica Polonica; 2002, 49, 4; 789-804
0001-527X
Pojawia się w:: Acta Biochimica Polonica
Dostawca treści:: Biblioteka Nauki

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Skocz do pozycji: 8.

Tytuł:: Order-disorder structural transitions in synthetic filaments of fast and slow skeletal muscle myosins under relaxing and activating conditions.
Autorzy:: Podlubnaya, Zoya
Malyshev, Sergey
Nieznański, Krzysztof
Stępkowski, Dariusz
Powiązania:: https://bibliotekanauki.pl/articles/1044221.pdf
Data publikacji:: 2000
Wydawca:: Polskie Towarzystwo Biochemiczne
Tematy:: method of slow skeletal muscle myosin preparation.
Ca2+-induced structural transitions
myosin filaments
fast and slow skeletal muscle myosin
Opis:: In the previous study (Podlubnaya et al., 1999, J. Struc. Biol. 127, 1-15) Ca2+-induced reversible structural transitions in synthetic filaments of pure fast skeletal and cardiac muscle myosins were observed under rigor conditions (-Ca2+/+ Ca2+). In the present work these studies have been extended to new more order-producing conditions (presence of ATP in the absence of Ca2+) aimed at arresting the relaxed structure in synthetic filaments of both fast and slow skeletal muscle myosin. Filaments were formed from column-purified myosins (rabbit fast skeletal muscle and rabbit slow skeletal semimebranosus proprius muscle). In the presence of 0.1 mM free Ca2+, 3 mM Mg2+ and 2 mM ATP (activating conditions) these filaments had a spread structure with a random arrangement of myosin heads and subfragments 2 protruding from the filament backbone. Such a structure is indistinguishable from the filament structures observed previously for fast skeletal, cardiac (see reference cited above) and smooth (Podlubnaya et al., 1999, J. Muscle Res. Cell Motil. 20, 547-554) muscle myosins in the presence of 0.1 mM free Ca2+. In the absence of Ca2+ and in the presence of ATP (relaxing conditions) the filaments of both studied myosins revealed a compact ordered structure. The fast skeletal muscle myosin filaments exhibited an axial periodicity of about 14.5 nm and which was much more pronounced than under rigor conditions in the absence of Ca2+ (see the first reference cited). The slow skeletal muscle myosin filaments differ slightly in their appearance from those of fast muscle as they exhibit mainly an axial repeat of about 43 nm while the 14.5 nm repeat is visible only in some regions. This may be a result of a slightly different structural properties of slow skeletal muscle myosin. We conclude that, like other filaments of vertebrate myosins, slow skeletal muscle myosin filaments also undergo the Ca2+-induced structural order-disorder transitions. It is very likely that all vertebrate muscle myosins possess such a property.
Źródło:: Acta Biochimica Polonica; 2000, 47, 4; 1007-1017
0001-527X
Pojawia się w:: Acta Biochimica Polonica
Dostawca treści:: Biblioteka Nauki

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Skocz do pozycji: 9.

Tytuł:: Reconstitution of ventricular myosin with atrial light chains 1 improves its functional properties.
Autorzy:: Khalina, Yana
Bartsch, Holger
Petzhold, Daria
Haase, Hannelore
Podlubnaya, Zoya
Shpagina, Mila
Morano, Ingo
Powiązania:: https://bibliotekanauki.pl/articles/1041425.pdf
Data publikacji:: 2005
Wydawca:: Polskie Towarzystwo Biochemiczne
Tematy:: myosin light chains
cardiac myosin
dilated cardiomyopathy
myosin filaments
reconstituted myosin
actin-activated ATPase activity
Opis:: Atrial light chain 1 (ALC-1) is expressed in embryonic and hypertrophied human ventricles but not in normal adult human ventricles. We investigated the effects of recombinant human atrial light chains (hALC-1) on the structure and enzymatic activity of synthetic filaments of ventricular myosin. The endogenous ventricular myosin light chain 1 (VLC-1) was partially replaced by recombinant hALC-1 yielding hALC-1 levels of 12%, 24% and 42%. This reconstitution of ventricular myosin with hALC-1 did not change the length of synthetic myosin filaments but led to more rounded myosin heads in comparison with those of control filaments. Actin-activated ATPase activity of myosin, a parameter of functional activity of molecular motor, amounted to 79.5 nmol Pi/mg per min in control myosin filaments. Reconstitution with hALC-1 caused a profound increase of the actin-activated myosin ATPase activity in a dose dependent manner, for example, synthetic myosin filaments formed with 12%, 24% and 42% hALC-1 reconstituted myosin revealed the actin-activated ATPase activity increased by 18%, 26% and 36%, respectively, as compared to control. These results strongly suggest that in vivo expression of ALC-1 enhances ventricular myosin function, thereby contributing to cardiac compensation.
Źródło:: Acta Biochimica Polonica; 2005, 52, 2; 443-448
0001-527X
Pojawia się w:: Acta Biochimica Polonica
Dostawca treści:: Biblioteka Nauki

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Skocz do pozycji: 10.

Tytuł:: Structural determinants of cooperativity in acto-myosin interactions.
Autorzy:: Moraczewska, Joanna
Powiązania:: https://bibliotekanauki.pl/articles/1043682.pdf
Data publikacji:: 2002
Wydawca:: Polskie Towarzystwo Biochemiczne
Tematy:: cooperativity
acto-myosin regulation
tropomyosin
contraction
Opis:: Regulation of muscle contraction is a very cooperative process. The presence of tropomyosin on the thin filament is both necessary and sufficient for cooperativity to occur. Data recently obtained with various tropomyosin isoforms and mutants help us to understand better the structural requirements in the thin filament for cooperative protein interactions. Forming an end-to-end overlap between neighboring tropomyosin molecules is not necessary for the cooperativity of the thin filament activation. When direct contacts between tropomyosin molecules are disrupted, the conformational changes in the filament are most probably transmitted cooperatively through actin subunits, although the exact nature of these changes is not known. The function of tropomyosin ends, alternatively expressed in various isoforms, is to confer specific actin affinity. Tropomyosin's affinity or actin is directly related to the size of the apparent cooperative unit defined as the number of actin subunits turned into the active state by binding of one myosin head. Inner sequences of tropomyosin, particularly actin-binding periods 3 to 5, play crucial role in myosin-induced activation of the thin filament. A plausible mechanism of tropomyosin function in this process is that inner tropomyosin regions are either specifically recognized by myosin or they define the right actin conformation required for tropomyosin movement from its blocking position.
Źródło:: Acta Biochimica Polonica; 2002, 49, 4; 805-812
0001-527X
Pojawia się w:: Acta Biochimica Polonica
Dostawca treści:: Biblioteka Nauki

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Skocz do pozycji: 11.

Tytuł:: Structure, function, and regulation of myosin 1C.
Autorzy:: Barylko, Barbara
Jung, Gwanghyun
Albanesi, Joseph
Powiązania:: https://bibliotekanauki.pl/articles/1041416.pdf
Data publikacji:: 2005
Wydawca:: Polskie Towarzystwo Biochemiczne
Tematy:: myosin 1
membrane protein translocation
domain structure
Opis:: Myosin 1C, the first mammalian single-headed myosin to be purified, cloned, and sequenced, has been implicated in the translocation of plasma membrane channels and transporters. Like other forms of myosin I (of which eight exist in humans) myosin 1C consists of motor, neck, and tail domains. The neck domain binds calmodulins more tightly in the absence than in the presence of Ca^(2+). Release of calmodulins exposes binding sites for anionic lipids, particularly phosphoinositides. The tail domain, which has an isoelectic point of 10.5, interacts with anionic lipid headgroups. When both neck and tail lipid binding sites are engaged, the myosin associates essentially irreversibly with membranes. Despite this tight membrane binding, it is widely believed that myosin 1C docking proteins are necessary for targeting the enzyme to specific subcellular location. The search for these putative myosin 1C receptors is an active area of research.
Źródło:: Acta Biochimica Polonica; 2005, 52, 2; 373-380
0001-527X
Pojawia się w:: Acta Biochimica Polonica
Dostawca treści:: Biblioteka Nauki

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Skocz do pozycji: 12.

Tytuł:: The slow sarco/endoplasmic reticulum Ca2+-ATPase declines independently of slow myosin in soleus muscle of diabetic rats
Autorzy:: Rácz, Gábor
Szabó, András
Vér, Ágota
Zádor, Ernő
Powiązania:: https://bibliotekanauki.pl/articles/1040545.pdf
Data publikacji:: 2009
Wydawca:: Polskie Towarzystwo Biochemiczne
Tematy:: muscle fibers
myosin
SERCA
diabetic rat
Opis:: The sarcoplasmic reticulum Ca2+-ATPase (SERCA) isoforms are normally expressed in coordination with the corresponding myosin heavy chain (MyHC) isoforms in the fibers of skeletal muscle but this coordination is often disrupted in pathological conditions. In the streptozotocin-induced diabetes of rats (stz-rats), the soleus muscle showed peripheral neuropathy and the SERCA2a level decreased in type I (slow-oxidative) fibers compared to the control muscles, whereas the expression of the corresponding slow MyHC1 did not change. No difference was found at the mRNA and protein levels of SERCA and MyHC isoforms in the whole soleus, except that the level of the SERCA2a protein specifically declined in stz-rats compared to the controls. This shows that the coordinated expression of SERCA2a and MyHC1 is disrupted at the SERCA2a protein level in the diabetic soleus. The results are in line with previous observations that regulators of the Ca-homeostasis may adapt faster to type I diabetes than the contractile elements.
Źródło:: Acta Biochimica Polonica; 2009, 56, 3; 487-493
0001-527X
Pojawia się w:: Acta Biochimica Polonica
Dostawca treści:: Biblioteka Nauki

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Skocz do pozycji: 13.

Tytuł:: The vertebrate skeletal muscle thick filaments are not three-stranded. Reinterpretation of some experimental data*
Autorzy:: Skubiszak, Ludmila
Kowalczyk, Leszek
Powiązania:: https://bibliotekanauki.pl/articles/1043687.pdf
Data publikacji:: 2002
Wydawca:: Polskie Towarzystwo Biochemiczne
Tematy:: thick filament symmetry
mass distribution
Fourier transform
myosin molecule packing
cross-bridge movement
Opis:: Computer simulation of mass distribution within the model and Fourier transforms of images depicting mass distribution are explored for verification of two alternative modes of the myosin molecule arrangement within the vertebrate skeletal muscle thick filaments. The model well depicting the complete bipolar structure of the thick filament and revealing a true threefold-rotational symmetry is a tube covered by two helices with a pitch of 2 × 43 nm due to arrangement of the myosin tails along a helical path and grouping of all myosin heads in the crowns rotated by 240° and each containing three cross-bridges separated by 0°, 120°, and 180°. The cross-bridge crown parameters are verified by EM images as well as by optical and low-angle X-ray diffraction patterns found in the literature. The myosin tail arrangement, at which the C-terminus of about 43-nm length is near-parallel to the filament axis and the rest of the tail is quite strongly twisted around, is verified by the high-angle X-ray diffraction patterns. A consequence of the new packing is a new way of movement of the myosin cross-bridges, namely, not by bending in the hinge domains, but by unwrapping from the thick filament surface towards the thin filaments along a helical path.
Źródło:: Acta Biochimica Polonica; 2002, 49, 4; 841-853
0001-527X
Pojawia się w:: Acta Biochimica Polonica
Dostawca treści:: Biblioteka Nauki

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Skocz do pozycji: 14.

Tytuł:: Transcriptional pattern of TGF-beta1 inhibitory effect on mouse C2C12 myoblasts differentiation
Autorzy:: Wicik, Z.
Sadkowski, T.
Jank, M.
Motyl, T.
Powiązania:: https://bibliotekanauki.pl/articles/30377.pdf
Data publikacji:: 2010
Wydawca:: Polska Akademia Nauk. Czytelnia Czasopism PAN
Tematy:: transforming growth factor-beta 1
myogenesis
microarray
DNA microarray
differentiation
myoblast
mouse
mice
muscle cell
myosin heavy chain
Opis:: The aim of the present study was to define the effect of TGF-β1 on C2C12 myoblasts myogenesis. TGF-β1 together with its receptor is a negative auto-paracrine regulator of myogenesis, which influences the proliferation, differentiation, and functions of muscle cells. TGF-β1 exerts highly significant inhibitory effect on differentiation of C2C12 mouse myoblasts manifested by the impairment of cell fusion and very low expression of myosin heavy chain. The study of differentiating C2C12 mouse myoblasts treated with TGF-β1 revealed 502 genes (436 down-regulated and 66 up-regulated) with statistically different expression. TGF-β1-regulated genes were identified to be involved in 29 biological processes, 29 molecular functions groups and 59 pathways. The strongest inhibiting effect of TGF-β1 was observed in the cadherin and Wnt pathways. The key-genes that could play the role of TGF-β1 targets during myoblasts differentiation was identified such as: Max, Creb1, Ccna2, Bax, MdfI, Tef, Tubg1, Cxcl5, Rho, Calca and Lgals4.
Źródło:: Polish Journal of Veterinary Sciences; 2010, 13, 4
1505-1773
Pojawia się w:: Polish Journal of Veterinary Sciences
Dostawca treści:: Biblioteka Nauki