Effect of dacarbazine on CD44 in live melanoma cells as measured by atomic force microscopy-based nanoscopy

CD44 ligand–receptor interactions are known to be involved in regulating cell migration and tumor cell metastasis. High expression levels of CD44 correlate with a poor prognosis of melanoma patients. In order to understand not only the mechanistic basis for dacarbazine (DTIC)-based melanoma treatmen...

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Autores principales: Huang, Xun, He, Jiexiang, Zhang, Huan-tian, Sun, Kai, Yang, Jie, Wang, Huajun, Zhang, Hongxin, Guo, Zhenzhao, Zha, Zhen-gang, Zhou, Changren
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Dove Medical Press 2017
Materias:
Original Research
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5739545/
https://www.ncbi.nlm.nih.gov/pubmed/29296081
http://dx.doi.org/10.2147/IJN.S149107
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author Huang, Xun
He, Jiexiang
Zhang, Huan-tian
Sun, Kai
Yang, Jie
Wang, Huajun
Zhang, Hongxin
Guo, Zhenzhao
Zha, Zhen-gang
Zhou, Changren
author_facet Huang, Xun
He, Jiexiang
Zhang, Huan-tian
Sun, Kai
Yang, Jie
Wang, Huajun
Zhang, Hongxin
Guo, Zhenzhao
Zha, Zhen-gang
Zhou, Changren
author_sort Huang, Xun
collection PubMed
description CD44 ligand–receptor interactions are known to be involved in regulating cell migration and tumor cell metastasis. High expression levels of CD44 correlate with a poor prognosis of melanoma patients. In order to understand not only the mechanistic basis for dacarbazine (DTIC)-based melanoma treatment but also the reason for the poor prognosis of melanoma patients treated with DTIC, dynamic force spectroscopy was used to structurally map single native CD44-coupled receptors on the surface of melanoma cells. The effect of DTIC treatment was quantified by the dynamic binding strength and the ligand-binding free-energy landscape. The results demonstrated no obvious effect of DTIC on the unbinding force between CD44 ligand and its receptor, even when the CD44 nanodomains were reduced significantly. However, DTIC did perturb the kinetic and thermodynamic interactions of the CD44 ligand–receptor, with a resultant greater dissociation rate, lower affinity, lower binding free energy, and a narrower energy valley for the free-energy landscape. For cells treated with 25 and 75 μg/mL DTIC for 24 hours, the dissociation constant for CD44 increased 9- and 70-fold, respectively. The CD44 ligand binding free energy decreased from 9.94 for untreated cells to 8.65 and 7.39 kcal/mol for DTIC-treated cells, which indicated that the CD44 ligand–receptor complexes on DTIC-treated melanoma cells were less stable than on untreated cells. However, affinity remained in the micromolar range, rather than the millimolar range associated with nonaffinity ligands. Hence, the CD44 receptor could still be activated, resulting in intracellular signaling that could trigger a cellular response. These results demonstrate DTIC perturbs, but not completely inhibits, the binding of CD44 ligand to membrane receptors, suggesting a basis for the poor prognosis associated with DTIC treatment of melanoma. Overall, atomic force microscopy-based nanoscopic methods offer thermodynamic and kinetic insight into the effect of DTIC on the CD44 ligand-binding process.
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spelling pubmed-57395452018-01-02 Effect of dacarbazine on CD44 in live melanoma cells as measured by atomic force microscopy-based nanoscopy Huang, Xun He, Jiexiang Zhang, Huan-tian Sun, Kai Yang, Jie Wang, Huajun Zhang, Hongxin Guo, Zhenzhao Zha, Zhen-gang Zhou, Changren Int J Nanomedicine Original Research CD44 ligand–receptor interactions are known to be involved in regulating cell migration and tumor cell metastasis. High expression levels of CD44 correlate with a poor prognosis of melanoma patients. In order to understand not only the mechanistic basis for dacarbazine (DTIC)-based melanoma treatment but also the reason for the poor prognosis of melanoma patients treated with DTIC, dynamic force spectroscopy was used to structurally map single native CD44-coupled receptors on the surface of melanoma cells. The effect of DTIC treatment was quantified by the dynamic binding strength and the ligand-binding free-energy landscape. The results demonstrated no obvious effect of DTIC on the unbinding force between CD44 ligand and its receptor, even when the CD44 nanodomains were reduced significantly. However, DTIC did perturb the kinetic and thermodynamic interactions of the CD44 ligand–receptor, with a resultant greater dissociation rate, lower affinity, lower binding free energy, and a narrower energy valley for the free-energy landscape. For cells treated with 25 and 75 μg/mL DTIC for 24 hours, the dissociation constant for CD44 increased 9- and 70-fold, respectively. The CD44 ligand binding free energy decreased from 9.94 for untreated cells to 8.65 and 7.39 kcal/mol for DTIC-treated cells, which indicated that the CD44 ligand–receptor complexes on DTIC-treated melanoma cells were less stable than on untreated cells. However, affinity remained in the micromolar range, rather than the millimolar range associated with nonaffinity ligands. Hence, the CD44 receptor could still be activated, resulting in intracellular signaling that could trigger a cellular response. These results demonstrate DTIC perturbs, but not completely inhibits, the binding of CD44 ligand to membrane receptors, suggesting a basis for the poor prognosis associated with DTIC treatment of melanoma. Overall, atomic force microscopy-based nanoscopic methods offer thermodynamic and kinetic insight into the effect of DTIC on the CD44 ligand-binding process. Dove Medical Press 2017-12-18 /pmc/articles/PMC5739545/ /pubmed/29296081 http://dx.doi.org/10.2147/IJN.S149107 Text en © 2017 Huang et al. This work is published and licensed by Dove Medical Press Limited The full terms of this license are available at https://www.dovepress.com/terms.php and incorporate the Creative Commons Attribution – Non Commercial (unported, v3.0) License (http://creativecommons.org/licenses/by-nc/3.0/). By accessing the work you hereby accept the Terms. Non-commercial uses of the work are permitted without any further permission from Dove Medical Press Limited, provided the work is properly attributed.
spellingShingle Original Research
Huang, Xun
He, Jiexiang
Zhang, Huan-tian
Sun, Kai
Yang, Jie
Wang, Huajun
Zhang, Hongxin
Guo, Zhenzhao
Zha, Zhen-gang
Zhou, Changren
Effect of dacarbazine on CD44 in live melanoma cells as measured by atomic force microscopy-based nanoscopy
title Effect of dacarbazine on CD44 in live melanoma cells as measured by atomic force microscopy-based nanoscopy
title_full Effect of dacarbazine on CD44 in live melanoma cells as measured by atomic force microscopy-based nanoscopy
title_fullStr Effect of dacarbazine on CD44 in live melanoma cells as measured by atomic force microscopy-based nanoscopy
title_full_unstemmed Effect of dacarbazine on CD44 in live melanoma cells as measured by atomic force microscopy-based nanoscopy
title_short Effect of dacarbazine on CD44 in live melanoma cells as measured by atomic force microscopy-based nanoscopy
title_sort effect of dacarbazine on cd44 in live melanoma cells as measured by atomic force microscopy-based nanoscopy
topic Original Research
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5739545/
https://www.ncbi.nlm.nih.gov/pubmed/29296081
http://dx.doi.org/10.2147/IJN.S149107
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