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A new technique to identify hybrid myotubes in vitro without culture fixation.

作者信息

Labrecque C, Huard J, Dansereau G, Robitaille L, Tremblay J P

机构信息

Department of Anatomy, Laval University, Quebec, Canada.

出版信息

J Histochem Cytochem. 1991 Jan;39(1):139-43. doi: 10.1177/39.1.1701185.

Abstract

Fluorescent latex microspheres (FLMs) were used to label myoblasts and to permit the observation of hybrid myotubes before culture fixation. This type of labeling did not affect survival, development, or fusion of these cells. The FLMs were retained for several weeks. Labeled mouse myoblasts were co-cultured with unlabeled rat myoblasts to verify whether the marker was released and spread from labeled to unlabeled cells. The nuclear stain Hoechst 33258 was used to distinguish the myoblasts from both species and permitted the demonstration that there was virtually no re-uptake. Hybrid myotubes were also obtained by co-culturing mouse myoblasts containing rhodamine FLMs and rat myoblasts containing green FLMs. These mixed cultures were observed repeatedly with a fluorescent microscope without any cytotoxic effect. Several myotubes were observed before fixation of the cultures to contain both types of fluorescent labels. Subsequent fixation and staining with Hoechst dye confirmed that these myotubes were hybrids.

摘要

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引用本文的文献

1
Stable hybrid myotubes: a new model for studying re-expression of enzymatic activities in vitro.
Ital J Neurol Sci. 1993 Jan;14(1):35-43. doi: 10.1007/BF02339040.

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