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University of Minnesota, Morris 1981 Commencement

Author: University Relations
Publication venue: University of Minnesota Morris Digital Well
Publication date: 01/06/1981
Field of study

The University of Minnesota, Morris Commencement June 12, 1981 Campus Mall 7:30 p.m.https://digitalcommons.morris.umn.edu/commencement/1031/thumbnail.jp

University of Minnesota, Morris (UMM): Digital Well

University of Minnesota, Morris 1982 Commencement

Author: University Relations
Publication venue: University of Minnesota Morris Digital Well
Publication date: 01/06/1982
Field of study

The University of Minnesota, Morris Commencement June 11, 1982 Campus Mall 7:30 p.m.https://digitalcommons.morris.umn.edu/commencement/1030/thumbnail.jp

University of Minnesota, Morris (UMM): Digital Well

Specific β-Tubulin Isotypes Can Functionally Enhance or Diminish Epothilone B Sensitivity in Non-Small Cell Lung Cancer Cells

Author: AL Risinger
B Lin
C Dumontet
CG Milross
CP Yang
DM Bollag
EH Rubin
Frances L. Byrne
H Freedman
H Yang
J Vansteenkiste
JA McCarroll
James Garner
JH Nettles
JJ Lee
JJ Lee
Joshua A. McCarroll
K Blade
K Kamath
M Kavallaris
M Magnani
Maria Kavallaris
NM Verrills
NR Khawaja
P Giannakakou
P Giannakakou
P Seve
PA Joe
PA Phillips
Paraskevi Giannakakou
Pei Pei Gan
PP Gan
PP Gan
PP Gan
RJ Kowalski
S Mozzetti
T O'Reilly
Publication venue: Public Library of Science
Publication date: 01/01/2011
Field of study

Epothilones are a new class of microtubule stabilizing agents with promising preclinical and clinical activity. Their cellular target is β-tubulin and factors influencing intrinsic sensitivity to epothilones are not well understood. In this study, the functional significance of specific β-tubulin isotypes in intrinsic sensitivity to epothilone B was investigated using siRNA gene knockdown against βII-, βIII- or βIVb-tubulins in two independent non-small cell lung cancer (NSCLC) cell lines, NCI-H460 and Calu-6. Drug-treated clonogenic assays showed that sensitivity to epothilone B was not altered following knockdown of βII-tubulin in both NSCLC cell lines. In contrast, knockdown of βIII-tubulin significantly increased sensitivity to epothilone B. Interestingly, βIVb-tubulin knockdowns were significantly less sensitive to epothilone B, compared to mock- and control siRNA cells. Cell cycle analysis of βIII-tubulin knockdown cells showed a higher percentage of cell death with epothilone B concentrations as low as 0.5 nM. In contrast, βIVb-tubulin knockdown cells displayed a decrease in epothilone B-induced G2-M cell cycle accumulation compared to control siRNA cells. Importantly, βIII-tubulin knockdowns displayed a significant dose-dependent increase in the percentage of apoptotic cells upon treatment with epothilone B, as detected using caspase 3/7 activity and Annexin-V staining. Higher concentrations of epothilone B were required to induce apoptosis in the βIVb-tubulin knockdowns compared to control siRNA, highlighting a potential mechanism underlying decreased sensitivity to this agent. This study demonstrates that specific β-tubulin isotypes can influence sensitivity to epothilone B and may influence differential sensitivity to this promising new agent

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