Expression Levels of a Kinesin-13 Microtubule Depolymerase Modulates the Effectiveness of Anti-Microtubule Agents

A Desai; AM Mulder; B Gigant; DG Hedrick; GC Rogers; Gregory V. Schimizzi; J Howard; Joshua D. Currie; KN Bhalla; KW Wood; MA Jordan; MA Jordan; Mikhail V. Blagosklonny; PV Jallepalli; RD Vale; S Uppuluri; SL Rogers; Stephen L. Rogers; T Ogawa; V Mennella; VM Bolanos-Garcia

Expression Levels of a Kinesin-13 Microtubule Depolymerase Modulates the Effectiveness of Anti-Microtubule Agents

Authors: A Desai
AM Mulder
B Gigant
DG Hedrick
GC Rogers
Gregory V. Schimizzi
J Howard
Joshua D. Currie
KN Bhalla
KW Wood
MA Jordan
MA Jordan
Mikhail V. Blagosklonny
PV Jallepalli
RD Vale
S Uppuluri
SL Rogers
Stephen L. Rogers
T Ogawa
V Mennella
VM Bolanos-Garcia
Publication date: 1 January 2010
Publisher: Public Library of Science
Doi

Abstract

Chemotherapeutic drugs often target the microtubule cytoskeleton as a means to disrupt cancer cell mitosis and proliferation. Anti-microtubule drugs inhibit microtubule dynamics, thereby triggering apoptosis when dividing cells activate the mitotic checkpoint. Microtubule dynamics are regulated by microtubule-associated proteins (MAPs); however, we lack a comprehensive understanding about how anti-microtubule agents functionally interact with MAPs. In this report, we test the hypothesis that the cellular levels of microtubule depolymerases, in this case kinesin-13 s, modulate the effectiveness of the microtubule disrupting drug colchicine.We used a combination of RNA interference (RNAi), high-throughput microscopy, and time-lapse video microscopy in Drosophila S2 cells to identify a specific MAP, kinesin-like protein 10A (KLP10A), that contributes to the efficacy of the anti-microtubule drug colchicine. KLP10A is an essential microtubule depolymerase throughout the cell cycle. We find that depletion of KLP10A in S2 cells confers resistance to colchicine-induced microtubule depolymerization to a much greater extent than depletion of several other destabilizing MAPs. Using image-based assays, we determined that control cells retained 58% (+/-2%SEM) of microtubule polymer when after treatment with 2 microM colchicine for 1 hour, while cells depleted of KLP10A by RNAi retained 74% (+/-1%SEM). Likewise, overexpression of KLP10A-GFP results in increased susceptibility to microtubule depolymerization by colchicine.Our results demonstrate that the efficacy of microtubule destabilization by a pharmacological agent is dependent upon the cellular expression of a microtubule depolymerase. These findings suggest that expression levels of Kif2A, the human kinesin-13 family member, may be an attractive biomarker to assess the effectiveness of anti-microtubule chemotherapies. Knowledge of how MAP expression levels affect the action of anti-microtubule drugs may prove useful for evaluating possible modes of cancer treatment