Fully automated counting of DNA damage foci in tumor cell culture: A matter of cell separation

S Köcher; J Volquardsen; A Perugachi Heinsohn; C Petersen; D Roggenbuck; K Rothkamm; W Y Mansour

doi:10.1016/j.dnarep.2021.103100

Fully automated counting of DNA damage foci in tumor cell culture: A matter of cell separation

Standard

Fully automated counting of DNA damage foci in tumor cell culture: A matter of cell separation. / Köcher, S; Volquardsen, J; Perugachi Heinsohn, A; Petersen, C; Roggenbuck, D; Rothkamm, K ; Mansour, W Y.

In: DNA REPAIR, Vol. 102, 103100, 06.2021.

Research output: SCORING: Contribution to journal › SCORING: Journal article › Research › peer-review

Harvard

Köcher, S, Volquardsen, J, Perugachi Heinsohn, A, Petersen, C, Roggenbuck, D, Rothkamm, K & Mansour, WY 2021, 'Fully automated counting of DNA damage foci in tumor cell culture: A matter of cell separation', DNA REPAIR, vol. 102, 103100. https://doi.org/10.1016/j.dnarep.2021.103100

APA

Köcher, S., Volquardsen, J., Perugachi Heinsohn, A., Petersen, C., Roggenbuck, D., Rothkamm, K., & Mansour, W. Y. (2021). Fully automated counting of DNA damage foci in tumor cell culture: A matter of cell separation. DNA REPAIR, 102, [103100]. https://doi.org/10.1016/j.dnarep.2021.103100

Vancouver

Köcher S, Volquardsen J, Perugachi Heinsohn A, Petersen C, Roggenbuck D, Rothkamm K et al. Fully automated counting of DNA damage foci in tumor cell culture: A matter of cell separation. DNA REPAIR. 2021 Jun;102. 103100. https://doi.org/10.1016/j.dnarep.2021.103100

Bibtex

@article{f5e41830178448a8a2e0c72d2dc7fab2,

title = "Fully automated counting of DNA damage foci in tumor cell culture: A matter of cell separation",

abstract = "Analysis and quantification of residual, unrepaired DNA double-strand breaks by detecting damage-associated γH2AX or 53BP1 foci is a promising approach to evaluate radiosensitivity or radiosensitization in tumor cells. Manual foci quantification by eye is well-established but unsatisfactory due to inconsistent foci numbers between different observers, lack of information about foci size and intensity and the time-consuming scoring process. Therefore, automated foci counting is an important goal. Several software solutions for automated foci counting in separately acquired fluorescence microscopy images have been established. The AKLIDES NUK technology by Medipan combines automated microscopy and image processing/ counting, enabling affordable high throughput foci analysis as a routine application. Using this machine, automated foci counting is well established for lymphocytes but has not yet been reported for adherent tumor cells with their irregularly shaped nuclei and heterogeneous foci textures. Here we aimed to use the AKLIDES NUK system for adherent tumor cells growing in clusters. We identified cell separation as a critical step to ensure fast and reliable automated nuclei detection. We validated our protocol for the fully automated quantification of (i) the IR-dose dependent increase and (ii) the ATM as well as PARP inhibitor-induced radiosensitization. Collectively, with this protocol the AKLIDES NUK system facilitates cost effective, fast and high throughput quantitative fluorescence microscopic analysis of DNA damage induced foci such as γH2AX and 53BP1 in adherent tumor cells.",

author = "S K{\"o}cher and J Volquardsen and {Perugachi Heinsohn}, A and C Petersen and D Roggenbuck and K Rothkamm and Mansour, {W Y}",

note = "Copyright {\textcopyright} 2021. Published by Elsevier B.V.",

year = "2021",

month = jun,

doi = "10.1016/j.dnarep.2021.103100",

language = "English",

volume = "102",

journal = "DNA REPAIR",

issn = "1568-7864",

publisher = "Elsevier",

}

RIS

TY - JOUR

T1 - Fully automated counting of DNA damage foci in tumor cell culture: A matter of cell separation

AU - Köcher, S

AU - Volquardsen, J

AU - Perugachi Heinsohn, A

AU - Petersen, C

AU - Roggenbuck, D

AU - Rothkamm, K

AU - Mansour, W Y

PY - 2021/6

Y1 - 2021/6

N2 - Analysis and quantification of residual, unrepaired DNA double-strand breaks by detecting damage-associated γH2AX or 53BP1 foci is a promising approach to evaluate radiosensitivity or radiosensitization in tumor cells. Manual foci quantification by eye is well-established but unsatisfactory due to inconsistent foci numbers between different observers, lack of information about foci size and intensity and the time-consuming scoring process. Therefore, automated foci counting is an important goal. Several software solutions for automated foci counting in separately acquired fluorescence microscopy images have been established. The AKLIDES NUK technology by Medipan combines automated microscopy and image processing/ counting, enabling affordable high throughput foci analysis as a routine application. Using this machine, automated foci counting is well established for lymphocytes but has not yet been reported for adherent tumor cells with their irregularly shaped nuclei and heterogeneous foci textures. Here we aimed to use the AKLIDES NUK system for adherent tumor cells growing in clusters. We identified cell separation as a critical step to ensure fast and reliable automated nuclei detection. We validated our protocol for the fully automated quantification of (i) the IR-dose dependent increase and (ii) the ATM as well as PARP inhibitor-induced radiosensitization. Collectively, with this protocol the AKLIDES NUK system facilitates cost effective, fast and high throughput quantitative fluorescence microscopic analysis of DNA damage induced foci such as γH2AX and 53BP1 in adherent tumor cells.

AB - Analysis and quantification of residual, unrepaired DNA double-strand breaks by detecting damage-associated γH2AX or 53BP1 foci is a promising approach to evaluate radiosensitivity or radiosensitization in tumor cells. Manual foci quantification by eye is well-established but unsatisfactory due to inconsistent foci numbers between different observers, lack of information about foci size and intensity and the time-consuming scoring process. Therefore, automated foci counting is an important goal. Several software solutions for automated foci counting in separately acquired fluorescence microscopy images have been established. The AKLIDES NUK technology by Medipan combines automated microscopy and image processing/ counting, enabling affordable high throughput foci analysis as a routine application. Using this machine, automated foci counting is well established for lymphocytes but has not yet been reported for adherent tumor cells with their irregularly shaped nuclei and heterogeneous foci textures. Here we aimed to use the AKLIDES NUK system for adherent tumor cells growing in clusters. We identified cell separation as a critical step to ensure fast and reliable automated nuclei detection. We validated our protocol for the fully automated quantification of (i) the IR-dose dependent increase and (ii) the ATM as well as PARP inhibitor-induced radiosensitization. Collectively, with this protocol the AKLIDES NUK system facilitates cost effective, fast and high throughput quantitative fluorescence microscopic analysis of DNA damage induced foci such as γH2AX and 53BP1 in adherent tumor cells.

U2 - 10.1016/j.dnarep.2021.103100

DO - 10.1016/j.dnarep.2021.103100

M3 - SCORING: Journal article

C2 - 33812230

VL - 102

JO - DNA REPAIR

JF - DNA REPAIR

SN - 1568-7864

M1 - 103100

ER -