Initial appearance of myomesin in differentiating muscle cells

Matthias Ernst; Hans Eppenberger; Thomas Doetschman

doi:10.1016/0045-6039(83)90042-8

Initial appearance of myomesin in differentiating muscle cells

Matthias Ernst, Hans Eppenberger, Thomas Doetschman

Cellular and Molecular Medicine

Research output: Contribution to journal › Article › peer-review

Abstract

The time between the appearance of the striated-muscle-specific M-line protein myomesin and the previous mitosis was measured in individual chick breast muscle cells. The shortest time interval (16 h) was measured with time-lapse cinematography followed by indirect immunofluorescence on 84 cells during the first two days of culture. During these experiments diffuse, cell border and cross-striated fluorescent patterns were observed in both bipolar and non-bipolar cells. A quantitative comparison of the spatial distribution of myomesin to cell morphology and time of culture revealed considerable variation among individual cells. These results indicate that the mechanisms regulating these factors during terminal differentiation are separable and not strictly coordinated.

Original language	English (US)
Pages (from-to)	319-323
Number of pages	5
Journal	Cell Differentiation
Volume	13
Issue number	4
DOIs	https://doi.org/10.1016/0045-6039(83)90042-8
State	Published - Dec 1983

Keywords

M-line
myogenesis
myomesin
time-lapse cinematography

ASJC Scopus subject areas

Developmental Biology

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10.1016/0045-6039(83)90042-8

Cite this

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title = "Initial appearance of myomesin in differentiating muscle cells",

abstract = "The time between the appearance of the striated-muscle-specific M-line protein myomesin and the previous mitosis was measured in individual chick breast muscle cells. The shortest time interval (16 h) was measured with time-lapse cinematography followed by indirect immunofluorescence on 84 cells during the first two days of culture. During these experiments diffuse, cell border and cross-striated fluorescent patterns were observed in both bipolar and non-bipolar cells. A quantitative comparison of the spatial distribution of myomesin to cell morphology and time of culture revealed considerable variation among individual cells. These results indicate that the mechanisms regulating these factors during terminal differentiation are separable and not strictly coordinated.",

keywords = "M-line, myogenesis, myomesin, time-lapse cinematography",

author = "Matthias Ernst and Hans Eppenberger and Thomas Doetschman",

note = "Funding Information: Swiss Federal Instituteo f TechnologyZ, tirichand was supportedb y grant no. 3.707-0.80f rom the Swiss National ScienceF oundationa nd by a grant from the Muscular DystrophyA ssociationI,n c.",

year = "1983",

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doi = "10.1016/0045-6039(83)90042-8",

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T1 - Initial appearance of myomesin in differentiating muscle cells

AU - Ernst, Matthias

AU - Eppenberger, Hans

AU - Doetschman, Thomas

N1 - Funding Information: Swiss Federal Instituteo f TechnologyZ, tirichand was supportedb y grant no. 3.707-0.80f rom the Swiss National ScienceF oundationa nd by a grant from the Muscular DystrophyA ssociationI,n c.

PY - 1983/12

Y1 - 1983/12

N2 - The time between the appearance of the striated-muscle-specific M-line protein myomesin and the previous mitosis was measured in individual chick breast muscle cells. The shortest time interval (16 h) was measured with time-lapse cinematography followed by indirect immunofluorescence on 84 cells during the first two days of culture. During these experiments diffuse, cell border and cross-striated fluorescent patterns were observed in both bipolar and non-bipolar cells. A quantitative comparison of the spatial distribution of myomesin to cell morphology and time of culture revealed considerable variation among individual cells. These results indicate that the mechanisms regulating these factors during terminal differentiation are separable and not strictly coordinated.

AB - The time between the appearance of the striated-muscle-specific M-line protein myomesin and the previous mitosis was measured in individual chick breast muscle cells. The shortest time interval (16 h) was measured with time-lapse cinematography followed by indirect immunofluorescence on 84 cells during the first two days of culture. During these experiments diffuse, cell border and cross-striated fluorescent patterns were observed in both bipolar and non-bipolar cells. A quantitative comparison of the spatial distribution of myomesin to cell morphology and time of culture revealed considerable variation among individual cells. These results indicate that the mechanisms regulating these factors during terminal differentiation are separable and not strictly coordinated.

KW - M-line

KW - myogenesis

KW - myomesin

KW - time-lapse cinematography

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SP - 319

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JO - Cell Differentiation

JF - Cell Differentiation

IS - 4

ER -

Initial appearance of myomesin in differentiating muscle cells

Abstract

Keywords

ASJC Scopus subject areas

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