BUCKLING OF A SINGLE MICROTUBULE BY OPTICAL TRAPPING FORCES - DIRECT MEASUREMENT OF MICROTUBULE RIGIDITY

被引:232
作者
KURACHI, M
HOSHI, M
TASHIRO, H
机构
[1] Laboratory of Photo-Biology, Photodynamics Research Center, Institute of Physical and Chemical Research (Riken, Miyagi
[2] Department of Basic Science, Faculty of Science and Technology, Ishinomaki Sensyu University, Ishinomaki, Miyagi
来源
CELL MOTILITY AND THE CYTOSKELETON | 1995年 / 30卷 / 03期
关键词
MICROTUBULES; FLEXURAL RIGIDITY; OPTICAL TRAPPING; MICROTUBULE-ASSOCIATED PROTEINS; TAXOL;
D O I
10.1002/cm.970300306
中图分类号
Q2 [细胞生物学];
学科分类号
071009 ; 090102 ;
摘要
As major determinants of cell shape and polarity, microtubules are required to have suitable rigidity. However, our knowledge of the mechanical properties of microtubules is far from satisfactory. We report here a new method of measuring the flexural rigidity of a single microtubule by direct buckling using the optical trapping technique. Microtubule buckling was induced by applying a small longitudinal compressing force through an optically trapped microsphere that was firmly attached to the microtubule. Three ways of estimating the flexural rigidity of a continuous slender rod, one from the observed critical load of buckling and two from deflected lengths and angles of bending, yielded values which agreed well when applied to the analysis of buckling microtubules. Unexpectedly, we found that the rigidity was not constant as expected but was dependent on microtubule length. This length dependency explains the discrepancies among reported Values of microtubule flexural rigidity measured by different methods. Comparing microtubules of identical lengths, microtubules assembled with brain-derived associated proteins (4 x 10(-23) Nm(2) at around 10 mu m in length) were four times more rigid than those assembled from purified tubulin and stabilized with taxol(1 X 10(-23) Nm(2)). (C) 1995 Wiley-Liss, Inc.
引用
收藏
页码:221 / 228
页数:8
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