1991
DOI: 10.1016/0092-8674(91)90618-9
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Intracompartmental sorting of essential myosin light chains: Molecular dissection and in vivo monitoring by epitope tagging

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Cited by 71 publications
(63 citation statements)
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“…The involvement of the COOH terminus of the ELC in heavy chain binding is consistent with previous observations (7,8), but participation of residues at NH 2 terminus of the ELC has not been previously demonstrated. We tested the possibility that the NH 2 -terminal residues are required for maintaining an overall conformation of the ELC rather than being in a direct association with the heavy chain.…”
Section: Resultssupporting
confidence: 80%
See 1 more Smart Citation
“…The involvement of the COOH terminus of the ELC in heavy chain binding is consistent with previous observations (7,8), but participation of residues at NH 2 terminus of the ELC has not been previously demonstrated. We tested the possibility that the NH 2 -terminal residues are required for maintaining an overall conformation of the ELC rather than being in a direct association with the heavy chain.…”
Section: Resultssupporting
confidence: 80%
“…Skeletal muscle alkali light chain A1 in which the COOH-terminal 14 residues were chemically removed did not bind the S1 heavy chain, although the conformation remained largely unchanged (7). Transfection studies also showed that a COOH-terminal truncation of the alkali light chain A1 failed to colocalize with acto-myosin structures in cultured myocytes (8).…”
mentioning
confidence: 89%
“…Chaussepied and Kasprzak (1989) have shown that the presence of different MLC isoforms in a myosin molecule confers different properties of association with actin. A study of intracompartmental sorting of MLC isoforms in rat cardiomyocytes has suggested that differences in affinity between MHC and MLC isoforms affect the sorting process (Soldati and Perriard, 1991). Work on the body wall musculature of C .…”
Section: Significance Of the Differentiation Programmentioning
confidence: 99%
“…For transient and stable transfections, we used a pCMV␤ vector (Clontech Laboratories AG, Basel, CH), in which the neomycin gene was cloned in EcoRI and in which the ␤-galactosidase gene was replaced by full-length cDNA encoding rat ␣-SMA, human ␥-and ␤-cytoplasmic actins, and chicken ␣-cardiac muscle actin. The 3Ј untranslated region (3ЈUTR) of actin isoforms was replaced by cDNA coding for the vesicular stomatitis virus G-protein (VSV-G; Soldati and Perriard, 1991), thus tagging the actins on C terminus. 3T3 fibroblasts were transfected with the use of FuGene 6 (Boehringer Mannheim AG, Mannheim, Germany) according to the manufacturer's protocol.…”
Section: Actin Constructs and Transfectionmentioning
confidence: 99%