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Thermo Fisher Scientific • 5791 Van Allen Way • Carlsbad, CA 92008 • www.thermofisher.com
INTRODUCTION
Study of genetic Information from cell-free (cf) DNA provide valuable
opportunities in cancer research and potentially impact future oncology. As an
example, liquid biopsy provide a non-invasive and cost effective solution for
future compared to traditional biopsy tests. Here we report the application of
research based Ion Torrent™ next-generation sequencing (NGS) Oncomine™
cfDNA assays and associated workflow, which is developed to detect somatic
variants at low frequency of 0.1% in cfDNA from plasma.
MATERIALS AND METHODS
Plasma preparation:
Blood samples were collected into EDTA tubes following manufacturer’s
instructions. Plasma was obtained by centrifugation at 1600 x g for 10 min at
4˚C, followed by another spin at 6,000 x g for 30 min at 4˚C to remove any
residual blood cells.
cfDNA/FFPE DNA isolation:
cfDNA was isolated from ~4 mL of plasma using MagMAX™ Cell-Free DNA
Isolation Kit following alternative protocol in User Guide appendix B.
RecoverAll™ Multi-Sample RNA/DNA Isolation Workflow was used to isolate
DNA from FFPE samples following standard protocol.
Library preparation:
Targeted libraries were prepared using the Oncomine™ Lung (or Breast) cfDNA
Assay reagents and user guide instructions for both cfDNA and FFPE DNA.
Sequencing:
The Ion 520™ and Ion 530™ Kit-Chef were used for template preparation on the
Ion Chef™, followed by sequencing on Ion S5™XL system using the Ion 530™
Chip. Lung cfDNA libraries were sequenced as an 8-plex while breast cfDNA
libraries were run as a 12-plex.
Data analysis:
Data analysis was performed in Torrent Suite using the variant Caller plugin.
Yanchun Li, Kris Lea, Priyanka K. Kshatriya, Gu, Jian, Ballesteros-Villagrana, Jeff Schageman, Varun Bagai, Dima Brinza, Richard Chien, Kelli S. Bramlett. 2130 Woodward St. Austin, TX 78744 Thermo Fisher Scientific.
Ion Torrent™ Next Generation Sequencing-Oncomine™ Lung cfDNA assay detected 0.1% low frequency somatic variants in Cell-Free DNA
RESULTS
Figure 1. Workflow for cfDNA analysis using cfDNA Lung Assay. The Oncomine™ cfDNA
assay is a content-optimized solution for NGS cfDNA liquid biopsy research. It includes both
library prep and analysis solutions that enable limit of detection down to 0.1% allelic frequency
(with 20 ng input) for SNV and INDEL hotspots with the flexibility of using as little as 1ng input
DNA. A blood sample to report workflow can be completed in 2 days.
Figure 2. Tagging Technology for rare mutation detection
cfDNA with tumor variant Wild type cfDNA molecule
1. Labeling of DNA molecules
2. PCR amplification and sequencing
Table 1. Detection sensitivity and specificity using Horizon™ cfDNA Reference Standards
with Oncomine™ Lung cfDNA Assay. The Multiplex I cfDNA DNA Reference Standards
(HD780,Horizon™) contains 8 engineered single nucleotide variants (SNVs/SNPs) at a range of
low allelic frequencies (5%, 1%, and 0.1%). Sensitivity and specificity were calculated based on 8
true positive and 149 true negative hotspots covered in Oncomine™ Lung cfDNA Assay. Results
from either duplicates or quadruple experiments.
Horizon Input Sensitivity Specificity
0.0% 20ng
100.0% 100.0%
100.0% 100.0%
0.1% 50ng
91.7% 100.0%
83.3% 100.0%
100.0% 100.0%
91.7% 100.0%
1.0% 10ng
100.0% 100.0%
100.0% 100.0%
5.0% 5ng
100.0% 100.0%
100.0% 100.0%
Gene Variant
Oncomine™
cfDNA Lung
assay
Oncomine™
cfDNA Breast
assay
Digital PCR
KRAS p.G12D
0.20% 0.20% 0.27%
0.17% 0.14% 0.24%
PIK3CA p.E545K
0.15% 0.14% 0.02%
0.11% 0.06% 0.19%
EGFR p.E746_A750delELREA
0.12% *N/A 0.10%
0.11% *N/A 0.12%
EGFR p.L858R
0.07% 0.14% 0.05%
0.06% 0.06% 0.83%
Table 2. Cross Validation of 0.1% Detection sensitivity by Oncomine™ Lung and Breast
cfDNA Assay with digital PCR assay. Data shown is from the Horizon 0.1% control material
when used as input for the Oncomine™ lung and breast cfDNA assays and dPCR assays for the
indicated variants. Allelic frequency of variants was measured using the targeted NGS library
method in the indicated columns. Allelic frequency was validated with digital PCR as an
orthogonal method to measure low frequency variants. Measurements were made in duplicate.
*N/A indicates variants in the Horizon 0.1% control material that are not in the Oncomine™ Breast
cfDNA targeted hotspot file.
Sample Variant
cfDNA input
20ng 10ng 5ng 2ng 1ng 0.5 ng 0.25ng
S1
EGFR
p.L747_E749delLRE
9.4% NA NA 10.4% 14.7% 16.5% 7.9%
S2
KRAS p.G12D 0.2% 0.3% 0.1% 0.2% ** NA NA
MET p.T1010I 47.4% 49.8% 45.5% 47.6% 51.2% NA NA
Table 3. Detection of variants in cfDNA extracted from banked research NSCLC plasma
samples with Oncomine™ Lung cfDNA Assay. Research sample S1 contains a fairly high
frequency variant detected in cfDNA as 9.42% using recommended input of 20ng in the
Oncomine™ Lung cfDNA assay. The variant could still be detected when input was decreased to
0.25 ng of cfDNA. In research sample S2, a variant was identified using 20ng of cfDNA at low
allelic frequency of 0.22%. This variant was successfully detected using input amounts down to 2
ng. A germline variant present in sample S2 was consistently detected at levels ~50% in all input
titration libraries. NA: not tested; **: not detected.
CONCLUSIONS
• Oncomine™ cfDNA Assays provide an easy, quick, and reliable solution for
research in detecting low frequency somatic variant in blood plasma and
tissue
• Oncomine™ cfDNA Assays target specific actionable hotspot regions of genes
for indicated cancer type to create a targeted amplicon library for sequencing
with the Ion Torrent Sequencing System; Oncomine™ Lung cfDNA Assay
(Cat Lot: A31149) is currently available; Oncomine™ Breast and Colon cfDNA
assays coming soon
• The Ion Torrent™ NGS technology and tailored TSS analytical pipeline allows
this assay to detect variants as low as 0.1% limit of detection (LOD);
measured allelic frequencies confirmed by orthogonal measurement
system—dPCR
• The total process time (from plasma/FFPE specimen to result reporting)
could be as short as 32 hours with a total hand on time of ~4 hours;
supporting a lab workflow where you can receive blood samples early on day
1 and have variant calls before you go home on day 2
Sample Variant FFPE Plasma
S1 EGFR p.L858R 71.42% 2.66%
S2 TP53 p.R158L 51.89% 4.32%
S3
METp.T1010I 43.87% 51.75%
KRAS p.G12C 34.62% 0.28%
S4 ND ND ND
S5
EGFR p.L858R 58.44% 7.74%
MET p.T1010I 41.93% 48.74%
TP53 p.Y220C 35.54% 1.93%
S6 TP53 p.R158L 10.19% 1.27%
S7 TP53 p.M237I 0.49% 0.13%
S8 KRAS p.G12A 5.56% 3.02%
S9 MET p.T1010I 68.93% 50.51%
S10
KRAS p.G12V 20.01% 1.70%
KRAS p.G12C 20.03% 1.70%
S11 KRAS p.G12D 25.29% 12%
S12 KRAS p.G12C 19.91% **
S13 KRAS p.G13D 29.90% **
S14 TP53 p.R248L 21.82% 0.34%
S15 TP53 p.R337L 46.84% 0.18%
S16
KRAS p.G12D 3.98% 0.22%
MET p.T1010I 50.42% 47.44%
S17 TP53 p.R273C 4.64% **
S18 KRAS p.G12S 1.25% 6.56%
S19
TP53 p.Y234C 17.16% **
TP53 p.T125T 25.76% **
S20
KRAS p.G13C 2.65% 0.30%
MET p.T1010I 2.21% **
Table 4. Observed frequencies of variants detected from matched FFPE and Plasma
samples. Late stage NSCLC research samples were purchased from BioChain. Sample sets
included solid tumor sample embedded in FFPE and 2–4 mls plasma from blood collected in
EDTA tubes. Bold numbers indicate allelic frequencies as determined using the Oncomine™ Lung
cfDNA assay for the indicated somatic variants. Non-bold frequencies show germline variants
that were also detected in the targeted libraries. For these 6 independent research samples,
there was very high concordance between variants detected in FFPE and cfDNA from matched
plasma from the same research subjects. As expected, higher variant frequencies were observed
in the FFPE solid tumor samples with significantly lower frequencies measured in the matched
cfDNA samples. ND: no detection(negative case); **: not detected.
For Research Use Only. Not for use in diagnostic procedures.
© 2016 Thermo Fisher Scientific Inc. All rights reserved. All trademarks are the
property of Thermo Fisher Scientific and its subsidiaries unless otherwise
specified. Horizon is a trademark of Horizon Discovery Group, Inc.
Samples Sensitivity Specificity PPV
0.1%MM 90% 98.4% 94.1%
0.5% >99.9% 98.3% 94.3%
Table 5. Detection Sensitivity and Specificity. The Oncomine™ Lung cfDNA Assay
performance was evaluated using engineered controls (AcroMetrix™ Oncology Hotspot Control)
in background GM24385 genomic DNA diluted to 0.1% or 0.5% allelic frequencies. The control
and background DNA was fragmented to mimic the size of cfDNA. Mean sensitivity and
specificity values were obtained across the expected true positives and true negatives at
oncology hotspot positions.

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Thermo Fisher Scientific's OncomineTM Lung cfDNA assay detects 0.1% low frequency somatic variants in cell-free DNA

  • 1. Thermo Fisher Scientific • 5791 Van Allen Way • Carlsbad, CA 92008 • www.thermofisher.com INTRODUCTION Study of genetic Information from cell-free (cf) DNA provide valuable opportunities in cancer research and potentially impact future oncology. As an example, liquid biopsy provide a non-invasive and cost effective solution for future compared to traditional biopsy tests. Here we report the application of research based Ion Torrent™ next-generation sequencing (NGS) Oncomine™ cfDNA assays and associated workflow, which is developed to detect somatic variants at low frequency of 0.1% in cfDNA from plasma. MATERIALS AND METHODS Plasma preparation: Blood samples were collected into EDTA tubes following manufacturer’s instructions. Plasma was obtained by centrifugation at 1600 x g for 10 min at 4˚C, followed by another spin at 6,000 x g for 30 min at 4˚C to remove any residual blood cells. cfDNA/FFPE DNA isolation: cfDNA was isolated from ~4 mL of plasma using MagMAX™ Cell-Free DNA Isolation Kit following alternative protocol in User Guide appendix B. RecoverAll™ Multi-Sample RNA/DNA Isolation Workflow was used to isolate DNA from FFPE samples following standard protocol. Library preparation: Targeted libraries were prepared using the Oncomine™ Lung (or Breast) cfDNA Assay reagents and user guide instructions for both cfDNA and FFPE DNA. Sequencing: The Ion 520™ and Ion 530™ Kit-Chef were used for template preparation on the Ion Chef™, followed by sequencing on Ion S5™XL system using the Ion 530™ Chip. Lung cfDNA libraries were sequenced as an 8-plex while breast cfDNA libraries were run as a 12-plex. Data analysis: Data analysis was performed in Torrent Suite using the variant Caller plugin. Yanchun Li, Kris Lea, Priyanka K. Kshatriya, Gu, Jian, Ballesteros-Villagrana, Jeff Schageman, Varun Bagai, Dima Brinza, Richard Chien, Kelli S. Bramlett. 2130 Woodward St. Austin, TX 78744 Thermo Fisher Scientific. Ion Torrent™ Next Generation Sequencing-Oncomine™ Lung cfDNA assay detected 0.1% low frequency somatic variants in Cell-Free DNA RESULTS Figure 1. Workflow for cfDNA analysis using cfDNA Lung Assay. The Oncomine™ cfDNA assay is a content-optimized solution for NGS cfDNA liquid biopsy research. It includes both library prep and analysis solutions that enable limit of detection down to 0.1% allelic frequency (with 20 ng input) for SNV and INDEL hotspots with the flexibility of using as little as 1ng input DNA. A blood sample to report workflow can be completed in 2 days. Figure 2. Tagging Technology for rare mutation detection cfDNA with tumor variant Wild type cfDNA molecule 1. Labeling of DNA molecules 2. PCR amplification and sequencing Table 1. Detection sensitivity and specificity using Horizon™ cfDNA Reference Standards with Oncomine™ Lung cfDNA Assay. The Multiplex I cfDNA DNA Reference Standards (HD780,Horizon™) contains 8 engineered single nucleotide variants (SNVs/SNPs) at a range of low allelic frequencies (5%, 1%, and 0.1%). Sensitivity and specificity were calculated based on 8 true positive and 149 true negative hotspots covered in Oncomine™ Lung cfDNA Assay. Results from either duplicates or quadruple experiments. Horizon Input Sensitivity Specificity 0.0% 20ng 100.0% 100.0% 100.0% 100.0% 0.1% 50ng 91.7% 100.0% 83.3% 100.0% 100.0% 100.0% 91.7% 100.0% 1.0% 10ng 100.0% 100.0% 100.0% 100.0% 5.0% 5ng 100.0% 100.0% 100.0% 100.0% Gene Variant Oncomine™ cfDNA Lung assay Oncomine™ cfDNA Breast assay Digital PCR KRAS p.G12D 0.20% 0.20% 0.27% 0.17% 0.14% 0.24% PIK3CA p.E545K 0.15% 0.14% 0.02% 0.11% 0.06% 0.19% EGFR p.E746_A750delELREA 0.12% *N/A 0.10% 0.11% *N/A 0.12% EGFR p.L858R 0.07% 0.14% 0.05% 0.06% 0.06% 0.83% Table 2. Cross Validation of 0.1% Detection sensitivity by Oncomine™ Lung and Breast cfDNA Assay with digital PCR assay. Data shown is from the Horizon 0.1% control material when used as input for the Oncomine™ lung and breast cfDNA assays and dPCR assays for the indicated variants. Allelic frequency of variants was measured using the targeted NGS library method in the indicated columns. Allelic frequency was validated with digital PCR as an orthogonal method to measure low frequency variants. Measurements were made in duplicate. *N/A indicates variants in the Horizon 0.1% control material that are not in the Oncomine™ Breast cfDNA targeted hotspot file. Sample Variant cfDNA input 20ng 10ng 5ng 2ng 1ng 0.5 ng 0.25ng S1 EGFR p.L747_E749delLRE 9.4% NA NA 10.4% 14.7% 16.5% 7.9% S2 KRAS p.G12D 0.2% 0.3% 0.1% 0.2% ** NA NA MET p.T1010I 47.4% 49.8% 45.5% 47.6% 51.2% NA NA Table 3. Detection of variants in cfDNA extracted from banked research NSCLC plasma samples with Oncomine™ Lung cfDNA Assay. Research sample S1 contains a fairly high frequency variant detected in cfDNA as 9.42% using recommended input of 20ng in the Oncomine™ Lung cfDNA assay. The variant could still be detected when input was decreased to 0.25 ng of cfDNA. In research sample S2, a variant was identified using 20ng of cfDNA at low allelic frequency of 0.22%. This variant was successfully detected using input amounts down to 2 ng. A germline variant present in sample S2 was consistently detected at levels ~50% in all input titration libraries. NA: not tested; **: not detected. CONCLUSIONS • Oncomine™ cfDNA Assays provide an easy, quick, and reliable solution for research in detecting low frequency somatic variant in blood plasma and tissue • Oncomine™ cfDNA Assays target specific actionable hotspot regions of genes for indicated cancer type to create a targeted amplicon library for sequencing with the Ion Torrent Sequencing System; Oncomine™ Lung cfDNA Assay (Cat Lot: A31149) is currently available; Oncomine™ Breast and Colon cfDNA assays coming soon • The Ion Torrent™ NGS technology and tailored TSS analytical pipeline allows this assay to detect variants as low as 0.1% limit of detection (LOD); measured allelic frequencies confirmed by orthogonal measurement system—dPCR • The total process time (from plasma/FFPE specimen to result reporting) could be as short as 32 hours with a total hand on time of ~4 hours; supporting a lab workflow where you can receive blood samples early on day 1 and have variant calls before you go home on day 2 Sample Variant FFPE Plasma S1 EGFR p.L858R 71.42% 2.66% S2 TP53 p.R158L 51.89% 4.32% S3 METp.T1010I 43.87% 51.75% KRAS p.G12C 34.62% 0.28% S4 ND ND ND S5 EGFR p.L858R 58.44% 7.74% MET p.T1010I 41.93% 48.74% TP53 p.Y220C 35.54% 1.93% S6 TP53 p.R158L 10.19% 1.27% S7 TP53 p.M237I 0.49% 0.13% S8 KRAS p.G12A 5.56% 3.02% S9 MET p.T1010I 68.93% 50.51% S10 KRAS p.G12V 20.01% 1.70% KRAS p.G12C 20.03% 1.70% S11 KRAS p.G12D 25.29% 12% S12 KRAS p.G12C 19.91% ** S13 KRAS p.G13D 29.90% ** S14 TP53 p.R248L 21.82% 0.34% S15 TP53 p.R337L 46.84% 0.18% S16 KRAS p.G12D 3.98% 0.22% MET p.T1010I 50.42% 47.44% S17 TP53 p.R273C 4.64% ** S18 KRAS p.G12S 1.25% 6.56% S19 TP53 p.Y234C 17.16% ** TP53 p.T125T 25.76% ** S20 KRAS p.G13C 2.65% 0.30% MET p.T1010I 2.21% ** Table 4. Observed frequencies of variants detected from matched FFPE and Plasma samples. Late stage NSCLC research samples were purchased from BioChain. Sample sets included solid tumor sample embedded in FFPE and 2–4 mls plasma from blood collected in EDTA tubes. Bold numbers indicate allelic frequencies as determined using the Oncomine™ Lung cfDNA assay for the indicated somatic variants. Non-bold frequencies show germline variants that were also detected in the targeted libraries. For these 6 independent research samples, there was very high concordance between variants detected in FFPE and cfDNA from matched plasma from the same research subjects. As expected, higher variant frequencies were observed in the FFPE solid tumor samples with significantly lower frequencies measured in the matched cfDNA samples. ND: no detection(negative case); **: not detected. For Research Use Only. Not for use in diagnostic procedures. © 2016 Thermo Fisher Scientific Inc. All rights reserved. All trademarks are the property of Thermo Fisher Scientific and its subsidiaries unless otherwise specified. Horizon is a trademark of Horizon Discovery Group, Inc. Samples Sensitivity Specificity PPV 0.1%MM 90% 98.4% 94.1% 0.5% >99.9% 98.3% 94.3% Table 5. Detection Sensitivity and Specificity. The Oncomine™ Lung cfDNA Assay performance was evaluated using engineered controls (AcroMetrix™ Oncology Hotspot Control) in background GM24385 genomic DNA diluted to 0.1% or 0.5% allelic frequencies. The control and background DNA was fragmented to mimic the size of cfDNA. Mean sensitivity and specificity values were obtained across the expected true positives and true negatives at oncology hotspot positions.