Contribution of Plus and Minus End Pathways to Microtubule Turnover. I.A. Vorobjev, V.I. Rodionov, I.V. Maly, and G.G. Borisy J. Cell Sci., 112(Pt 14):2277-2289, 1999

Turnover is important for the maintenance and remodeling of the cytoskeleton during the processes of cell morphogenesis, mitosis and motility. Microtubule (MT) turnover is thought to occur by dynamic instability, growth and shortening at distal (plus) ends. Recent observation of MT release from the centrosome and depolymerization from proximal (minus) ends indicates the existence of a minus end pathway. To evaluate the relative contributions of plus and minus end pathways to turnover, we analyzed MT dynamics in a model system, the fish melanophore, a large non-motile cell with a regular radial array of long MTs. MT ends were tracked in digital fluorescence time lapse sequences and life histories of individual MTs were analyzed using random walk theory generalized to the case of diffusion with drift. Analysis of plus end dynamics gave an apparent diffusion coefficient of D = 7.5 µm²/min. The random walk model predicts that the half-time for turnover driven solely by plus end dynamics will depend strongly on position in the cell. Based on the experimentally determined value of D, turnover of MTs near the center of a typical melanophore of radius 70 µm was calculated to require over 5 hours, a paradoxically long time.

To examine MT behavior deep in the cytoplasm, we developed a novel, sequential subtraction mode of image analysis. This analysis revealed a subpopulation of MTs which shortened from their minus ends, presumably after constitutive release from the centrosome. Given the relative slowness of plus end dynamics to turn over the root of a long MT, the turnover of MTs near the cell center is determined primarily by the minus-end pathway. MTs released from the centrosome become replaced by newly nucleated ones. The relative contributions of plus and minus end pathways was estimated from the diffusion coefficient, D, for the plus end, the length distribution of MTs, the frequency of free minus ends, and the rate of minus-end shortening. We conclude that, in large animal cells with a centrosomally focussed array of MTs, turnover occurs by a combination of plus and minus end pathways,--the plus end dominating at the cell periphery and the minus end dominating near the cell center.

	Figure 1 (76 K) - MT dynamics during approach to the steady-state
	Figure 2 (77 K) - Life history plots of MTs during approach to the steady-state
	Figure 3 (75 K) - Random walk analysis of MT dynamics during the approach to steady-state
	Figure 4 (105 K) - MT dynamics at steady-state
	Figure 5 (119 K) - Analysis of MT dynamics at steady-state
	Figure 6 (94 K) - Sequential subtraction analysis of MT dynamics at steady-state
	Figure 7 (267 K) - Minus-end shortening revealed by sequential subtraction analysis
	Figure 8 (44 K) - Relative contribution of plus and minus end pathways to MT turnover

	Sequence 1 (911 K) - Dynamic instability of plus ends (new growth shown in red)
	Sequence 2 (1.6 M) - Microtubule dynamics in fish melanophores; Sequential subtraction analysis of MT dynamics
	Sequence 3 (1.8 M) - Sequence of subtracted frames
	Sequence 4 (915 K) - Sequence of subtracted frames, enlarged
	Sequence 5 (1.6 M) - Minus-end shortening revealed by sequential subtraction analysis