We recently developed a direct fluorescence ratio assay (Zhai, Y., and G.G. Borisy. 1994. J. Cell Sci. 107:881-890) to quantify microtubule (MT) polymer in order to determine if net MT depolymerization occurred upon anaphase onset as the spindle was disassembled. Our results showed no net decrease in polymer, indicating that the disassembly of kinetochore MTs was balanced by assembly of midbody and astral MTs. Thus, the mitosis-interphase transition occurs by a redistribution of tubulin among different classes of MTs at essentially constant polymer level. We now examine the reverse process, the interphase-mitosis transition. Specifically, we quantitated both the level of MT polymer and the dynamics of MTs during the G2/M transition using the fluorescence ratio assay and a fluorescence photoactivation approach, respectively. Prophase cells before nuclear envelope breakdown (NEB) had high levels of MT polymer (62%) similar to that previously reported for random interphase populations (68%). However, prophase cells just after NEB had significantly reduced levels (23%) which recovered as MT attachments to chromosomes were made (prometaphase, 47%; metaphase, 56%). The abrupt reorganization of MTs at NEB was corroborated by anti-tubulin immunofluorescence staining using a variety of fixation protocols. Sensitivity to nocodazole also increased at NEB. Photoactivation analyses of MT dynamics showed a similar abrupt change at NEB, basal rates of MT turnover (pre-NEB) increased post-NEB and then became slower later in mitosis. Our results indicate that the interphase-mitosis (G2/M) transition of the MT array does not occur by a simple redistribution of tubulin at constant polymer level as the mitosis-interphase (M/G1) transition. Rather, an abrupt decrease in MT polymer level and increase in MT dynamics occurs tightly correlated with NEB. A subsequent increase in MT polymer level and decrease in MT dynamics occurs correlated with chromosome attachment. These results carry implications for understanding spindle morphogenesis. They indicate that changes in MT dynamics may cause the steady-state MT polymer level in mitotic cells to be lower than in interphase. We propose that tension exerted on the kMTs may lead to their lengthening and thereby lead to an increase in the MT polymer level as chromosomes attach to the spindle.
Skip Nav Destination
Article navigation
1 October 1996
Article|
October 01 1996
Microtubule dynamics at the G2/M transition: abrupt breakdown of cytoplasmic microtubules at nuclear envelope breakdown and implications for spindle morphogenesis.
Y Zhai,
Y Zhai
Laboratory of Molecular Biology, University of Wisconsin, Madison 53706, USA.
Search for other works by this author on:
P J Kronebusch,
P J Kronebusch
Laboratory of Molecular Biology, University of Wisconsin, Madison 53706, USA.
Search for other works by this author on:
P M Simon,
P M Simon
Laboratory of Molecular Biology, University of Wisconsin, Madison 53706, USA.
Search for other works by this author on:
G G Borisy
G G Borisy
Laboratory of Molecular Biology, University of Wisconsin, Madison 53706, USA.
Search for other works by this author on:
Y Zhai
Laboratory of Molecular Biology, University of Wisconsin, Madison 53706, USA.
P J Kronebusch
Laboratory of Molecular Biology, University of Wisconsin, Madison 53706, USA.
P M Simon
Laboratory of Molecular Biology, University of Wisconsin, Madison 53706, USA.
G G Borisy
Laboratory of Molecular Biology, University of Wisconsin, Madison 53706, USA.
Online ISSN: 1540-8140
Print ISSN: 0021-9525
J Cell Biol (1996) 135 (1): 201–214.
Citation
Y Zhai, P J Kronebusch, P M Simon, G G Borisy; Microtubule dynamics at the G2/M transition: abrupt breakdown of cytoplasmic microtubules at nuclear envelope breakdown and implications for spindle morphogenesis.. J Cell Biol 1 October 1996; 135 (1): 201–214. doi: https://doi.org/10.1083/jcb.135.1.201
Download citation file:
Sign in
Don't already have an account? Register
Client Account
You could not be signed in. Please check your email address / username and password and try again.
Could not validate captcha. Please try again.
Sign in via your Institution
Sign in via your InstitutionEmail alerts
Advertisement
Advertisement