Efficiency of whole genome amplification of single circulating tumor cells enriched by CellSearch and sorted by FACS

BACKGROUND: Tumor cells in the blood of patients with metastatic carcinomas are associated with poor survival. Knowledge of the cells’ genetic make-up can help to guide targeted therapy. We evaluated the efficiency and quality of isolation and amplification of DNA from single circulating tumor cells...

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Autores principales: Swennenhuis, Joost F, Reumers, Joke, Thys, Kim, Aerssens, Jeroen, Terstappen, Leon WMM
Formato: Online Artículo Texto
Lenguaje:English
Publicado: BioMed Central 2013
Materias:
Research
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3978840/
https://www.ncbi.nlm.nih.gov/pubmed/24286536
http://dx.doi.org/10.1186/gm510
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author Swennenhuis, Joost F
Reumers, Joke
Thys, Kim
Aerssens, Jeroen
Terstappen, Leon WMM
author_facet Swennenhuis, Joost F
Reumers, Joke
Thys, Kim
Aerssens, Jeroen
Terstappen, Leon WMM
author_sort Swennenhuis, Joost F
collection PubMed
description BACKGROUND: Tumor cells in the blood of patients with metastatic carcinomas are associated with poor survival. Knowledge of the cells’ genetic make-up can help to guide targeted therapy. We evaluated the efficiency and quality of isolation and amplification of DNA from single circulating tumor cells (CTC). METHODS: The efficiency of the procedure was determined by spiking blood with SKBR-3 cells, enrichment with the CellSearch system, followed by single cell sorting by fluorescence-activated cell sorting (FACS) and whole genome amplification. A selection of single cell DNA from fixed and unfixed SKBR-3 cells was exome sequenced and the DNA quality analyzed. Single CTC from patients with lung cancer were used to demonstrate the potential of single CTC molecular characterization. RESULTS: The overall efficiency of the procedure from spiked cell to amplified DNA was approximately 20%. Losses attributed to the CellSearch system were around 20%, transfer to FACS around 25%, sorting around 5% and DNA amplification around 25%. Exome sequencing revealed that the quality of the DNA was affected by the fixation of the cells, amplification, and the low starting quantity of DNA. A single fixed cell had an average coverage at 20× depth of 30% when sequencing to an average of 40× depth, whereas a single unfixed cell had 45% coverage. GenomiPhi-amplified genomic DNA had a coverage of 72% versus a coverage of 87% of genomic DNA. Twenty-one percent of the CTC from patients with lung cancer identified by the CellSearch system could be isolated individually and amplified. CONCLUSIONS: CTC enriched by the CellSearch system were sorted by FACS, and DNA retrieved and amplified with an overall efficiency of 20%. Analysis of the sequencing data showed that this DNA could be used for variant calling, but not for quantitative measurements such as copy number detection. Close to 55% of the exome of single SKBR-3 cells were successfully sequenced to 20× depth making it possible to call 72% of the variants. The overall coverage was reduced to 30% at 20× depth, making it possible to call 56% of the variants in CellSave-fixed cells.
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spelling pubmed-39788402014-04-12 Efficiency of whole genome amplification of single circulating tumor cells enriched by CellSearch and sorted by FACS Swennenhuis, Joost F Reumers, Joke Thys, Kim Aerssens, Jeroen Terstappen, Leon WMM Genome Med Research BACKGROUND: Tumor cells in the blood of patients with metastatic carcinomas are associated with poor survival. Knowledge of the cells’ genetic make-up can help to guide targeted therapy. We evaluated the efficiency and quality of isolation and amplification of DNA from single circulating tumor cells (CTC). METHODS: The efficiency of the procedure was determined by spiking blood with SKBR-3 cells, enrichment with the CellSearch system, followed by single cell sorting by fluorescence-activated cell sorting (FACS) and whole genome amplification. A selection of single cell DNA from fixed and unfixed SKBR-3 cells was exome sequenced and the DNA quality analyzed. Single CTC from patients with lung cancer were used to demonstrate the potential of single CTC molecular characterization. RESULTS: The overall efficiency of the procedure from spiked cell to amplified DNA was approximately 20%. Losses attributed to the CellSearch system were around 20%, transfer to FACS around 25%, sorting around 5% and DNA amplification around 25%. Exome sequencing revealed that the quality of the DNA was affected by the fixation of the cells, amplification, and the low starting quantity of DNA. A single fixed cell had an average coverage at 20× depth of 30% when sequencing to an average of 40× depth, whereas a single unfixed cell had 45% coverage. GenomiPhi-amplified genomic DNA had a coverage of 72% versus a coverage of 87% of genomic DNA. Twenty-one percent of the CTC from patients with lung cancer identified by the CellSearch system could be isolated individually and amplified. CONCLUSIONS: CTC enriched by the CellSearch system were sorted by FACS, and DNA retrieved and amplified with an overall efficiency of 20%. Analysis of the sequencing data showed that this DNA could be used for variant calling, but not for quantitative measurements such as copy number detection. Close to 55% of the exome of single SKBR-3 cells were successfully sequenced to 20× depth making it possible to call 72% of the variants. The overall coverage was reduced to 30% at 20× depth, making it possible to call 56% of the variants in CellSave-fixed cells. BioMed Central 2013-11-29 /pmc/articles/PMC3978840/ /pubmed/24286536 http://dx.doi.org/10.1186/gm510 Text en Copyright © 2013 Swennenhuis et al.; licensee BioMed Central Ltd. http://creativecommons.org/licenses/by/2.0 This is an open access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/2.0), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Research
Swennenhuis, Joost F
Reumers, Joke
Thys, Kim
Aerssens, Jeroen
Terstappen, Leon WMM
Efficiency of whole genome amplification of single circulating tumor cells enriched by CellSearch and sorted by FACS
title Efficiency of whole genome amplification of single circulating tumor cells enriched by CellSearch and sorted by FACS
title_full Efficiency of whole genome amplification of single circulating tumor cells enriched by CellSearch and sorted by FACS
title_fullStr Efficiency of whole genome amplification of single circulating tumor cells enriched by CellSearch and sorted by FACS
title_full_unstemmed Efficiency of whole genome amplification of single circulating tumor cells enriched by CellSearch and sorted by FACS
title_short Efficiency of whole genome amplification of single circulating tumor cells enriched by CellSearch and sorted by FACS
title_sort efficiency of whole genome amplification of single circulating tumor cells enriched by cellsearch and sorted by facs
topic Research
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3978840/
https://www.ncbi.nlm.nih.gov/pubmed/24286536
http://dx.doi.org/10.1186/gm510
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