4.7 Article

Controlling kinesin by reversible disulfide cross-linking: Identifying the motility-producing conformational change

Journal

JOURNAL OF CELL BIOLOGY
Volume 151, Issue 5, Pages 1081-1092

Publisher

ROCKEFELLER UNIV PRESS
DOI: 10.1083/jcb.151.5.1081

Keywords

kinesin; processivity; disulfide crosslinking; neck linker; one-dimensional diffusion

Categories

Funding

  1. NIAMS NIH HHS [AR42895] Funding Source: Medline
  2. NIGMS NIH HHS [R01 GM038499] Funding Source: Medline

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Conventional kinesin, a dimeric molecular motor, uses ATP-dependent conformational changes to move unidirectionally along a row of tubulin subunits on a microtubule. Two models have been advanced for the major structural change underlying kinesin motility: the first involves an unzippering/zippering of a small peptide (neck linker) from the motor catalytic core and the second proposes an unwinding/rewinding of the adjacent coiled-coil (neck coiled-coil). Here, we have tested these models using disulfide cross-linking of cysteines engineered into recombinant kinesin motors. When the neck linker motion was prevented by crosslinking, kinesin ceased unidirectional movement and only showed brief one-dimensional diffusion along microtubules. Motility fully recovered upon adding reducing agents to reverse the cross-link. When the neck linker motion was partially restrained, single kinesin motors showed biased diffusion towards the microtubule plus end but could not move effectively against a load imposed by an optical trap. Thus, partial movement of the neck linker suffices for directionality but not for normal processivity or force generation. In contrast, preventing neck coiled-coil unwinding by disulfide cross-linking had relatively little effect on motor activity, although the average run length of single kinesin molecules decreased by 30-50%. These studies indicate that conformational changes in the neck linker, not in the neck coiled-coil, drive processive movement by the kinesin motor.

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