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Characterization of a Taxol‐resistant Human Small‐cell Lung Cancer Cell Line
Taxol is a novel anticancer agent with activity against a broad range of tumors. It has a unique ability to stabilize polymerized tubulin into microtubule bundles within the cell. We have established a taxol‐resistant human small‐cell lung cancer cell line (H69/Txl) by exposing H69 cells to stepwise...
Autores principales: | , , , , , , , , |
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Formato: | Online Artículo Texto |
Lenguaje: | English |
Publicado: |
Blackwell Publishing Ltd
1994
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Materias: | |
Acceso en línea: | https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5919448/ https://www.ncbi.nlm.nih.gov/pubmed/7514586 http://dx.doi.org/10.1111/j.1349-7006.1994.tb02096.x |
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author | Ohta, Sei Nishio, Kazuto Kubota, Naohiro Ohmori, Tohru Funayama, Yasunori Ohira, Tatsuo Nakajima, Hiroaki Adachi, Mitsuru Saijo, Nagahiro |
author_facet | Ohta, Sei Nishio, Kazuto Kubota, Naohiro Ohmori, Tohru Funayama, Yasunori Ohira, Tatsuo Nakajima, Hiroaki Adachi, Mitsuru Saijo, Nagahiro |
author_sort | Ohta, Sei |
collection | PubMed |
description | Taxol is a novel anticancer agent with activity against a broad range of tumors. It has a unique ability to stabilize polymerized tubulin into microtubule bundles within the cell. We have established a taxol‐resistant human small‐cell lung cancer cell line (H69/Txl) by exposing H69 cells to stepwise increases in taxol concentration. The resistance of H69/Txl cells to taxol was 4.7‐fold that of the original H69 cells: the IC(50) values for H69 and H69/Txl were 113.7 ± 56.54 nM and 538.7 ± 214.7 nM by the tetrazolium dye assay, respectively. Removal of the drug from the medium resulted in a 38% decrease in the growth rate of H69/Txl as compared with that in the presence of 30 nM taxol, suggesting that the growth of H69/Txl was partially dependent on taxol. H69/Txl showed higher sensitivity to vinca alkaloids such as vindesine, vincristine and vinblastine than the parental H69. There was no significant difference in intracellular [(3)H]taxol content between H69 and H69/Txl cells. No MDR‐1 mRNA was detected in H69/Txl by the reverse transcription polymerase chain reaction. There was no significant difference of total and polymerized tubulin content between H69 and H69/Txl cells. Altered mobility of one of the α‐tubulin isoforms in H69/Txl was revealed by using isoelectric focusing and Western blotting with anti‐α‐tubulin antibody. In H69, two α‐tubulin isoforms were observed, whereas three were evident in H69/Txl, two of them comigrating with the isoforms of H69 and the other being more acidic. We observed the increased acetylation of α‐tubulin in H69/Txl cells as compared with that in H69 cells. The acetylation of α‐tubulin may be responsible for the taxol resistance and/or taxol‐dependent growth of H69/Txl. |
format | Online Article Text |
id | pubmed-5919448 |
institution | National Center for Biotechnology Information |
language | English |
publishDate | 1994 |
publisher | Blackwell Publishing Ltd |
record_format | MEDLINE/PubMed |
spelling | pubmed-59194482018-05-11 Characterization of a Taxol‐resistant Human Small‐cell Lung Cancer Cell Line Ohta, Sei Nishio, Kazuto Kubota, Naohiro Ohmori, Tohru Funayama, Yasunori Ohira, Tatsuo Nakajima, Hiroaki Adachi, Mitsuru Saijo, Nagahiro Jpn J Cancer Res Article Taxol is a novel anticancer agent with activity against a broad range of tumors. It has a unique ability to stabilize polymerized tubulin into microtubule bundles within the cell. We have established a taxol‐resistant human small‐cell lung cancer cell line (H69/Txl) by exposing H69 cells to stepwise increases in taxol concentration. The resistance of H69/Txl cells to taxol was 4.7‐fold that of the original H69 cells: the IC(50) values for H69 and H69/Txl were 113.7 ± 56.54 nM and 538.7 ± 214.7 nM by the tetrazolium dye assay, respectively. Removal of the drug from the medium resulted in a 38% decrease in the growth rate of H69/Txl as compared with that in the presence of 30 nM taxol, suggesting that the growth of H69/Txl was partially dependent on taxol. H69/Txl showed higher sensitivity to vinca alkaloids such as vindesine, vincristine and vinblastine than the parental H69. There was no significant difference in intracellular [(3)H]taxol content between H69 and H69/Txl cells. No MDR‐1 mRNA was detected in H69/Txl by the reverse transcription polymerase chain reaction. There was no significant difference of total and polymerized tubulin content between H69 and H69/Txl cells. Altered mobility of one of the α‐tubulin isoforms in H69/Txl was revealed by using isoelectric focusing and Western blotting with anti‐α‐tubulin antibody. In H69, two α‐tubulin isoforms were observed, whereas three were evident in H69/Txl, two of them comigrating with the isoforms of H69 and the other being more acidic. We observed the increased acetylation of α‐tubulin in H69/Txl cells as compared with that in H69 cells. The acetylation of α‐tubulin may be responsible for the taxol resistance and/or taxol‐dependent growth of H69/Txl. Blackwell Publishing Ltd 1994-03 /pmc/articles/PMC5919448/ /pubmed/7514586 http://dx.doi.org/10.1111/j.1349-7006.1994.tb02096.x Text en |
spellingShingle | Article Ohta, Sei Nishio, Kazuto Kubota, Naohiro Ohmori, Tohru Funayama, Yasunori Ohira, Tatsuo Nakajima, Hiroaki Adachi, Mitsuru Saijo, Nagahiro Characterization of a Taxol‐resistant Human Small‐cell Lung Cancer Cell Line |
title | Characterization of a Taxol‐resistant Human Small‐cell Lung Cancer Cell Line |
title_full | Characterization of a Taxol‐resistant Human Small‐cell Lung Cancer Cell Line |
title_fullStr | Characterization of a Taxol‐resistant Human Small‐cell Lung Cancer Cell Line |
title_full_unstemmed | Characterization of a Taxol‐resistant Human Small‐cell Lung Cancer Cell Line |
title_short | Characterization of a Taxol‐resistant Human Small‐cell Lung Cancer Cell Line |
title_sort | characterization of a taxol‐resistant human small‐cell lung cancer cell line |
topic | Article |
url | https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5919448/ https://www.ncbi.nlm.nih.gov/pubmed/7514586 http://dx.doi.org/10.1111/j.1349-7006.1994.tb02096.x |
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