The development of noninvasive methods to detect and monitor tumors continues to be a bottleneck in oncology research. Circulating cell-free DNA shows great promise, but still requires improvements and additional research before it becomes standard practice.
At Cambridge Healthtech Institute’s Fifth Annual Circulating Cell-Free DNA, leading researchers from academia and industry will come together to address advances as well as existing challenges in this rapidly growing field.
This year’s event will place emphasis on early detection, next steps in monitoring treatment response, and making cfDNA standard clinical practice.
Thursday, February 15
7:00 am Registration Open and Morning Coffee
8:25 Chairperson’s Opening Remarks
Abhijit Patel, M.D., Ph.D., Associate Professor, Yale University School of Medicine
8:30 Eliminating Barriers in NGS Sample Preparation, Yet Catching the Needles-in-a-Haystack
G. Mike Makrigiorgos, Ph.D., Professor, Radiation Oncology, Dana-Farber Cancer Institute, Harvard Medical School
With the continuous reduction in sequencing costs, sample preparation for targeted re-sequencing presents a bottle-neck to efficient sequencing. We provide novel mutation enrichment-based sample preparation methods that (a) provide higher sensitivity
for detection of rare mutations, and (b) reduce the cost of both sample preparation and re-sequencing by orders of magnitude. Application in circulating DNA from clinical cancer samples will be presented.
9:00 Tracking Therapeutic Response Using an NGS-Based ctDNA Assay
Abhijit Patel, M.D., Ph.D., Associate Professor, Yale University School of Medicine
Our group has developed a simple, inexpensive, and ultrasensitive NGS-based assay that enables highly multiplexed measurement of mutant ctDNA. Data will be presented from ongoing studies to establish the clinical utility of this technology, with a focus
on monitoring of therapeutic response.
9:30 Multiplexed Enrichment of Rare Sequence Variants in Tumor and Cell-Free DNA
David Yu Zhang, Ph.D., Ted Law Jr., Assistant Professor, Bioengineering, Rice University
Rare DNA sequence variants hold important clinical and biological information, but are challenging for existing methods (e.g. PCR, NGS) to profile in an inexpensive, multiplexed, simple-to-implement, and sequence-general way. Here, we present Blocker
Displacement Amplification (BDA), a temperature-robust PCR method that selectively amplifies all sequence variants within a roughly 20nt window by 1000-fold over wildtype sequences, allowing easy detection and quantitation of hundreds of potentials
variants originally at <0.1% allele frequency.
10:00cfDNA Challenges and Solutions for Early Detection and Monitoring
Brian Haynes, Ph.D., Associate Director, Bioinformatics, Asuragen, Inc.
NGS analysis of ctDNA is highly centralized, owing to cumbersome workflows, complex assays, and a lack of high-performance kitted solutions. With the benefit of patient-like reference materials for assay familiarization and methods optimization, we developed an ultrasensitive targeted amplicon NGS workflow for profiling somatic mutations in cfDNA. We applied our NGS technology to a cohort of more than 50 cancers with matched plasma and tissue specimens and achieved accurate detection of variants down to 0.1% allele frequency.
10:15 Automated Solution for the Isolation of cfDNA from 4ml of Blood and the Stop-Primer Methode for qPCR Analysis
Christoph Mauracher, Ph.D., Managing Director, STRATEC Consumables GmbH
Circulating cell-free DNA (cfDNA) is of interest in many applications (e.g. fetal DNA in maternal plasma, or liquid biopsies). We developed an automated cfDNA extraction method for the InviGenius Plus which can be combined with our priority Stop-Primer
qPCR methode for the analysis of cancer genes.
10:30 Coffee Break in the Exhibit Hall with Poster Viewing
11:15 Real World Experience: Concordance of Genomic Alterations by Next-Generation Sequencing in Tumor Tissue versus Circulating Tumor DNA
Young Kwang Chae, M.D., MPH, MBA., Assistant Professor of Medicine, Feinberg School of Medicine, Northwestern University
The concordance of genomic alterations between two commercially available ctDNA and tissue biopsies was compared in patients with cancer using paired next-generation sequencing tissue and ctDNA biopsies. Across all genes, concordance between the two
platforms was approximately 90%. When only considering genomic alterations in either assay (e.g., excluding wild type/wild type genes), concordance was in the range of 10-20%. Concordant mutations were associated with significantly higher variant
allele frequency.
11:45 Biomarkers and Technologies for Early Detection
Michael J. Heller, Ph.D., Distinguished Scientist, OHSU Knight Cancer Early Detection Advanced Research Center (CEDAR); Professor Emeritus, Departments of Nanoengineering and Bioengineering, University of California, San Diego
Point of care (POC) devices for cancer and other molecular diagnostics still present considerable challenges. Cell-free (cf) DNA and exosomal RNA and proteins are now regarded as important biomarkers for liquid biopsy cancer diagnostics, therapy
monitoring and hold promise for early cancer detection. New electrokinetic technologies will provide powerful seamless sample to answer devices that will hopefully meet the challenges for liquid biopsy diagnostics and early detection.
12:15
pm Single Cell Analysis with the Naica System
Laura Cavé, Applications Specialist, Applications & Sales, Stilla Technologies
The Naica System uniquely allows users to image droplets and their contents, both pre- and post-amplification, as well as recover droplets for downstream analysis. We have taken advantage of these features to develop exciting new applications
for single cell analysis in mammalian cells and bacteria.
12:30 Session Break
12:40 Luncheon Presentation: Inroads into Cancer Patient Care with Droplet Digital PCR
George Karlin-Neumann, Ph.D., Director, Scientific Affairs, Digital Biology Center, Bio-Rad Laboratories
Over the past 5 years, Droplet DigitalTM PCR technology has proven to be a highly sensitive and accurate means for the detection and quantification of nucleic acid markers in 1000’s of labs worldwide. Its widespread adoption in liquid
biopsy studies and its demonstrated interlab reproducibility have propelled it into clinical use for cancer patients in cutting-edge diagnostic labs. Where biomarkers of interest are known, ddPCR provides affordable and rapid answers
to aid in clinical decision-making.
1:15 Session Break
1:55 Chairperson’s Remarks
Maximilian Diehn, M.D., Ph.D., Assistant Professor, Radiation Oncology, Stanford Cancer Institute, Institute for Stem Cell Biology & Regenerative Medicine, Stanford University
2:00 The Role of ctDNA in Immunotherapy
Razelle Kurzrock, Ph.D., M.D., Director, Center for Personalized Cancer Therapy, University of California
Blood-derived circulating tumor DNA (ctDNA) permits genomic sequencing of DNA shed from multiple sites. High ctDNA alteration numbers correlated with improved outcomes post-checkpoint inhibitors (variants of unknown significance ((VUS)
>3 versus ≤3), stable disease ≥6 months/partial/complete responses (PR/CR), 45% versus 15%; p = 0.014); median progression-free survival, 23 versus 2.3 months (p = 0.0004) (2-month landmark analysis, responders versus non-responders,
VUS>3) Therefore, hyper-mutated ctDNA predicts better outcome after immunotherapy.
2:30 Early Detection of Molecular Residual Disease in Localized Lung Cancer via Circulating Tumor DNA Profiling
Maximilian Diehn, M.D., Ph.D., Assistant Professor, Radiation Oncology, Stanford Cancer Institute, Institute
for Stem Cell Biology & Regenerative Medicine, Stanford University
Circulating tumor DNA (ctDNA) represents a promising biomarker for sensitive, specific, and dynamic detection of disease burden in cancer patients. In this presentation I will describe application of the high throughput sequencing-based
Cancer Personalized Profiling by Deep Sequencing (CAPP-Seq) method to detection of ctDNA molecular residual disease following curative-intent therapy in early stage lung cancer.
3:00 Cell Free Tumor Derived DNA in the Management of Human Tumors
Chetan Bettegowda, M.D., Ph.D., Assistant Professor, Neurosurgery and Oncology, Johns Hopkins University
School of Medicine
There are no clinically utilized biomarkers for the majority of central nervous system malignancies. Brain tumors infrequently shed tumor-derived DNA into the circulation. This talk will describe ongoing efforts to utilize cerebrospinal
fluid as a reservoir for tumor derived DNA and potential applications of such an approach.
3:30 Refreshment Break and Poster Competition Winner Announced in the Exhibit Hall
4:15 Dynamic Monitoring of Circulating Tumor DNA in Non-Hodgkin Lymphoma
Christopher Melani, M.D., Staff Clinician, Center for Cancer Research, National Cancer Institute
Next-generation sequencing-based assays detect circulating tumor DNA allowing assessment of tumor dynamics in blood. Monitoring ctDNA encoding immunoglobulin receptors detects recurrent disease prior to scans in diffuse large B-cell
lymphoma. “Liquid biopsies” of ctDNA for somatic mutations address tumor heterogeneity, clonal evolution, and mechanisms of resistance to guide precision treatment. I will describe applications of ctDNA in lymphoma
including real-time analysis of tumor dynamics, early disease detection, and precision-directed treatment.
4:45 Early Response Monitoring with Circulating Tumor DNA in Lung Cancer
Hatim Husain, M.D., Assistant Professor of Medicine, Division of Medical Oncology, Department of Medicine, University
of California, San Diego
Non-invasive drug response biomarkers for early assessment of tumor response can enable adaptive therapeutic decision-making for individualized patient treatment and proof-of-concept for target inhibition of tumor cells by investigational
drugs. Findings suggest that tyrosine kinase inhibitors induced tumor apoptosis within days of initial patient dosing. We demonstrate that early monitoring of ctDNA by non-invasive sampling provides temporal and quantitative dissection
of early early tumor response.
5:15 Panel Discussion: Monitoring Residual Disease and Therapeutic Response
Maximilian Diehn, M.D., Ph.D., Assistant Professor, Radiation Oncology, Stanford Cancer Institute, Institute for Stem Cell Biology & Regenerative Medicine, Stanford University
5:45 Reception in the Exhibit Hall with Poster Viewing
6:45 Close of Day
Friday, February 16
8:00 am Registration Open and Morning Coffee
8:25 Chairperson’s Remarks
Filip Janku, MD, Ph.D., Associate Professor, Department of Investigational Cancer Therapeutics, The University of Texas MD Anderson Cancer Center
8:30 Liquid Biopsies in Cancer: Cell-Free DNA and Beyond
Filip Janku, M.D., Ph.D., Associate Professor, Department of Investigational Cancer Therapeutics, The University of
Texas MD Anderson Cancer Center
Molecular testing of liquid biopsies provide minimally invasive approaches for molecular diagnostics in cancer. Testing of plasma-derived cell-free DNA has been approved by regulatory agencies in selected indications and is widely
accepted in clinical and translational research. Novel circulating sources of cancer DNA such as exosomal nucleic acids, nucleic acids from tumor educated platelets are being investigated.
9:00 pm Single-Color Digital PCR Provides High-Performance Detection of Cancer Mutations from Circulating DNA
Christina Wood-Bouwens, Cellular and Molecular Biology, Life Science Research Professional,
Stanford University
Single-color digital droplet PCR enables absolute quantification of mutation-bearing cell-free molecules for a fraction of the cost of next generation sequencing; Our novel assay has a molecular limit of detection down to 3 mutation
ctDNA molecules, and can used with non-amplified template. I will describe how this technology will be used to create customized mutation assays for individual cancer patients on a high-throughput scale, enabling rapid longitudinal
monitoring of ctDNA.
9:30 Novel Nanosensing Technologies for Exosome Detection and Profiling
Cesar M. Castro, M.D., Director, Cancer Program, MGH Center for Systems Biology, Hematology - Oncology, Massachusetts
General Hospital/Harvard Medical School
Exosomes have emerged as highly promising cancer biomarkers because they’re abundant in biofluids, carry proteins and RNA reflecting parental cells, and are stable in circulation. Yet, reliable and sensitive approaches for analyzing
exosomes and their molecular information are lacking. This talk will discuss novel nanotechnology sensing platforms developed to analyze exosomal proteins and RNAs directly from clinical specimens and discuss future developments
to facilitate their translation into routine clinical use.
10:00 Poster Presentation: A Comprehensive Approach to Sequence-Oriented IsomiR Annotation (CASMIR): Demonstration with IsomiR Profiling in Colorectal Neoplasia
Wilson Wu, PhD., Principal Research Technologist, Gastroenterology & Hepatology, Mayo Clinic
10:30 Coffee Break in the Exhibit Hall with Poster Viewing
11:15 Diversity of the Vesicular Secretome
Jan Lötvall, Professor, Department of Internal Medicine, Göteborg University, Chief Scientist, Codiak BioSciences
All cells release multiple types of extracellular vesicles, that can shuttle proteins, RNA and DNA between cells. The released vesicles are traditionally divided into “exosomes” and “microvesicles”, but current
data shows that cells release multiple types vesicles with different morphology and cargo, far beyond the traditional “exosomes” and “microvesicles”. This presentation will discuss the diversity of the “vesicular
secretome”, and will suggest subgroupings far beyond the traditional nomenclature.
11:45 Highly Sensitive Tumor Detection and Classification Using Methylome Analysis of Plasma DNA
Daniel De Carvalho, Ph.D., Associate Professor, Princess Margaret Cancer Centre, University
of Toronto
Methylome analysis of cfDNA is highly sensitive and suitable for detecting circulating tumor DNA (ctDNA) in early stage patients. A machine-learning derived classifier using cfDNA methylomes was able to correctly classify plasma
samples from patients with seven cancer types and healthy donors. Therefore, methylome analysis of cfDNA can be used for non-invasive early stage detection of ctDNA and robustly classify cancer types.
12:15 Exploiting the Biology of Exosomes for Diagnosis and Treatment of Cancer
Raghu Kalluri, Ph.D., Professor, Chair, The University of Texas MD Anderson Cancer Center, Department of
Cancer Biology
Exosomes are detected in the tumor microenvironment and emerging evidence suggests that they play a role in facilitating tumorigenesis by regulating angiogenesis, immunity and metastasis. Circulating exosomes could be used as liquid
biopsies and non-invasive biomarkers to potentially inform on early detection and diagnosis of cancer patients. Exosomes can be used for the treatment of cancer. This lecture will highlight some of the recent advances in the
area of exosomes biology and their utility in the diagnosis and treatment of cancer.
12:45 Close of Symposium