High Resolution Melting

High Resolution Melting What is it ? How does it work ? Jason McKinney Scientist

Scanning for sequence variants • “Scanning” = SNP discovery, rare alleles • “Genotyping” = discriminate between known alleles, common mutation • Scanning based on detection of “HETERODUPLEXES”

What is a “Heteroduplex” ?

Scanning (continued) • Based on detection of heteroduplexes • Different from fully base paired molecules • Mobility (SSCP, DGGE, CGGE) • Thermal stability (dHPLC) • Sequencing (gold standard)

Effective methods, however, … • Time consuming • Labor intensive • Technical skills • Equipment / Start up cost • … can we build a better “mouse trap” ?

Fluorescent Melting Curve analysis? • Identify heteroduplexes based on the change in fluorescent signal as a sample is thermally denatured (melted) • Dye that “glows” when bound to dsDNA • Wait a second, … haven’t people tried this already ? • Well, … yes, … it didn’t work very well.

What is a Melting Curve?

Melting with Sybr Green Lipsky, et al., Clin Chem 2001

WHY it did not work • 2 Primary Reasons • (1) Chemistry • Fluorescent dyes inhibit PCR at “SATURATING” concentrations • (2) Instrumentation • Slow data acquisition rates, optically inferior instrument, inadequate temperature control

HR-1 and LCGreen Instrument and Chemistry solutions

What is a “Saturating” dye ?

Melting with LCGreen

HR-1 Data acquisition (>100 pts/degree @ 0.30C/sec, fast) Temperature control (+/- 0.050C) Custom optics (matched to LCGreen, dedicated) LightCycler <10 data points/degree @ 0.10C/sec +/- 1-20C Generic optics, meant to be able to detect a range of fluorophores, focal distance and/or angle may change between samples HR-1 vs. LightCycler

HR-1 LightCycler Melting curves: HR-1 vs. LC

Summary • Scanning for heteroduplexes • New twist on an old game • Melting curve, sequence of events • HR-1, LCGreen, … solves 2 issues • Saturating dye • Data acquisition • Scanning is NOT Genotyping

High Resolution Melting