TABLE I:
Current methods and challenges in cfDNA analysis
| Challenge | Solution | Comments |
|---|---|---|
|
| ||
| DNA damage | DNA repair | Need high-yield method to reverse DNA oxidation and deamination |
| cfDNA sampling stochasticity | Larger blood volumes | Concern for patient health |
| cfDNA sampling stochasticity | Urine cfDNA | Need for extracting cfDNA from large volumes; process short cfDNA |
|
| ||
| Detecting mutations with ≤1% VAF | Digital PCR | Single-plex, only known mutations |
| Detecting mutations with ≤1% VAF | Mass spectrometry | Medium-plex, only known mutations |
| Detecting mutations with ≤1% VAF | NGS with UMIs | Expensive and low conversion yield |
| Detecting mutations with ≤1% VAF | NGS with allele enrichment | Low-plex, inaccurate quantitation, and low on-target rates |
|
| ||
| High conversion yield from cfDNA | N/A | Need high-yield end-repair and ligation |
| NGS depth uniformity | Primer/probe conc. tuning | labor-intensive and imperfect uniformity |
|
| ||
| Detecting fusions in cfDNA | Very large NGS panel | Very expensive because introns are long |
| Detecting CNVs in cfDNA | NGS, ddPCR | No current solution for detection ≤5% VAF |
|
| ||
| Rapid cfDNA diagnostics | Nanopore sequencing | High error rates and expensive reads |
| Affordable cfDNA diagnostics | N/A | Current cfDNA NGS panels have list price over $4,000 |