Incorporation and turnover of labeled exogenous tubulin in the mitotic spindles of Chaetopterus oocytes and HeLa cells

Incorporation and turnover of labeled exogenous tubulin in the mitotic spindles of Chaetopterus oocytes and HeLa cells

The incorporation of tubulin into mitotic spindles in situ was studied by incubating permeabilized mitotic cells in solutions containing [3H]GTP‐labeled or dichlorotriazinylamino fluorescein (DTAF)‐labeled tubulin. Metaphase HeLa cells or spindle‐containing “minicells” from Chaetopterus oocytes were...

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Veröffentlicht in:Cell motility and the cytoskeleton 1986, Vol.6 (2), p.114-121
Hauptverfasser: Goode, Dennis, Sarma, Vidya
Format: Artikel
Sprache:eng
Schlagworte:
Animals
Annelida - ultrastructure
assembly polarity
Cell Membrane Permeability
Chaetopterus
Detergents
Fluoresceins
Fluorescent Dyes
Guanosine Diphosphate - metabolism
Guanosine Triphosphate - metabolism
HeLa cells
HeLa Cells - ultrastructure
Humans
Kinetics
Microscopy, Electron
microtubules
Microtubules - metabolism
mitosis
Oocytes - ultrastructure
Polyethylene Glycols
Spindle Apparatus - metabolism
Tubulin - metabolism
tubulin incorporation
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Zusammenfassung:The incorporation of tubulin into mitotic spindles in situ was studied by incubating permeabilized mitotic cells in solutions containing [3H]GTP‐labeled or dichlorotriazinylamino fluorescein (DTAF)‐labeled tubulin. Metaphase HeLa cells or spindle‐containing “minicells” from Chaetopterus oocytes were lysed in a microtubule‐assembly buffer plus 0.5% Nonidet P‐40, 1 mg/ml 120,000g supernatant mammalian brain tubulin, and [3H]GTP. After different periods of incubation, mitotic spindles were isolated in 2 M‐glycerol‐containing assembly buffer and separated from unbound counts by centrifugation through a 4 M‐glycerol cushion; 3H counts per mg protein increase linearly for 8–12 min and then reach a plateau or steady state in both Chaetopterus oocytes and HeLa cells. Addition of 4 mM CaCl2 blocks or reverses incorporation. Little or no [3H]GTP is incorporated if exogenous tubulin or lysed cells are omitted from the assembly mixture. To measure the loss rate of [3H]GTP‐tubulin from mitotic spindles, cells were incubated in tubulin plus [3H]GTP for 30 min, and a 20‐fold excess of cold GTP (2 mM) was added. Samples were removed after incubation for different periods, and spindles were isolated as described above and counted for 3H content. [3H]GTP is lost from spindles at a rate of about 16%/min until a new steady state is reached in about 8 min. These results are consistent with an incorporation and turnover of [3H]GTP‐tubulin in spindle microtubules of these lysed‐cell models. The location of this newly incorporated tubulin in the spindle was investigated by incorporating fluorescent DTAF‐tubulin into mitotic spindles of these lysed cell types. A short pulse (2–5 min) appears to label microtubules (MTs) near metaphase chromosomes and longer exposures label the entire spindle. The rates of incorporation and turnover that we see by [3H]GTP and fluorescent tubulin incorporation in situ are faster than those observed with brain MTs at steady state in vitro but are in the range of the rates of spindle fiber formation in prophase, and spindle MT reassembly after cooling.
ISSN:0886-1544
1097-0169
DOI:10.1002/cm.970060208