Presentation is loading. Please wait.

Presentation is loading. Please wait.

Modified Allele Dosage (MAD) Genotyping by Hi-Res Melting  of Whole Amplicons Jason T. McKinney Scientist Human Genetics Applications.

Published byEustacia Elfreda Patrick Modified over 8 years ago

Similar presentations

Presentation on theme: "Modified Allele Dosage (MAD) Genotyping by Hi-Res Melting  of Whole Amplicons Jason T. McKinney Scientist Human Genetics Applications."— Presentation transcript:

1 Modified Allele Dosage (MAD) Genotyping by Hi-Res Melting  of Whole Amplicons Jason T. McKinney Scientist Human Genetics Applications

2 Modified what? … Who’s MAD? M odified A llele D osage = Pre-PCR DNA mixingM odified A llele D osage = Pre-PCR DNA mixing “MAD”? Well, … PHENCODE=ENCODE+GenPhen, HuGENet,LSDB’s, …“MAD”? Well, … PHENCODE=ENCODE+GenPhen, HuGENet,LSDB’s, … –Seems as though “MAD” is a MUST Genotype by Hi-Res Melting (HRM) of whole ampliconsGenotype by Hi-Res Melting (HRM) of whole amplicons Detection of heteroduplexesDetection of heteroduplexes –“Core” application of Hi-Res Melting Force heteroduplex formation in homozygous samples by mixing DNA pre-PCRForce heteroduplex formation in homozygous samples by mixing DNA pre-PCR –Typically done 1:1 volume:volume

3 Stealing from Peter? Must not compromise ability to distinguish “true” heterozygous samplesMust not compromise ability to distinguish “true” heterozygous samples Homozygous “heteroduplexes” =Homozygous “heteroduplexes” = –“intermediate” quantity of heteroduplex molecules relative to “true” heterozygous samples and wild type samples

4 Ideally …

5 Optimal Ratio of DNA mixing Palais RA, Liew MA, Wittwer CT. Quantitative heteroduplex analysis for SNP genotyping. Analytical Biochemistry. 2005. In Press.

6 Optimal ratio, … in English please? 1X WT DNA + 6X Unknown DNA yields the following heteroduplex ratio’s:1X WT DNA + 6X Unknown DNA yields the following heteroduplex ratio’s: Given HRM detection of ~5-10% variant DNA, these ratio’s should be easily discriminatedGiven HRM detection of ~5-10% variant DNA, these ratio’s should be easily discriminated

7 Benefits Genotype sans probe (labeled or unlabeled)Genotype sans probe (labeled or unlabeled) –Cost and technical benefit No asymmetric amplificationNo asymmetric amplification –Technical benefit Use “scanning” primers to genotypeUse “scanning” primers to genotype  Potential to observe variants other than the SNP of interest  Potential to observe variants other than the SNP of interest –Relative to a probe-based genotyping method

8 System Requirements Sequence characterized reference sample (wildtype or variant)Sequence characterized reference sample (wildtype or variant) Accurately quantified DNA samplesAccurately quantified DNA samples dsDNA “saturation” dye (LCGreen Plus)dsDNA “saturation” dye (LCGreen Plus) High-resolution instrumentation for melting curve analysis (HR-1, LightScanner)High-resolution instrumentation for melting curve analysis (HR-1, LightScanner) Well characterized region around SNP is beneficialWell characterized region around SNP is beneficial

9 Validation of MAD genotyping Risk burden of HDL haplotypes – 6 genes regulating HDL cholesterol metabolismRisk burden of HDL haplotypes – 6 genes regulating HDL cholesterol metabolism 1.Primer design a.Area around SNP’s interrogated in  100 chromosomes b.Primers designed to avoid observed variants 2.PCR quality a.Primer concentration across annealing temperature gradient b.Definitive criteria for Hi-Res Melting success

10 Methods Quantify DNA samples (~10ng/  l)Quantify DNA samples (~10ng/  l) Add reference DNA (wildtype) to master mix at 1 / 7 total DNAAdd reference DNA (wildtype) to master mix at 1 / 7 total DNA Add unknown DNA at 6 / 7 totalAdd unknown DNA at 6 / 7 total Amplification – 96 well thermal blockAmplification – 96 well thermal block HRM on LightScannerHRM on LightScanner Automated calling of genotypesAutomated calling of genotypes

11 Recipe for a reaction

12 Genes SNP’s  Cholesterol ester transfer protein (CETP) Hepatic lipase (LIPC) Hepatic lipase (LIPC) Scavenger receptor protein, beta 1 (SCARB1) Scavenger receptor protein, beta 1 (SCARB1)  IVS7+4 C>T; c1264 A>G; IVS15-30 A>G; c1482+1954 A>C A-763G; C-514T; C- 480T; G-250A A-763G; C-514T; C- 480T; G-250A c1050 C>T c1050 C>T

13 Show me the Data!

14 CETP IVS7 +4 C>T

15 CETP c1264 A>G

16 CETP IVS15 –30 A>G

17 CETP c1482+1954 A>C

18 LIPC A-763G

19 LIPC G-250A

20 SCARB1 c1050 C>T

21 LIPC C-514T, C-480T

22 Summary of Data SNP’s observedSNP’s observed –C>T (4), A>G (3), A>C (1), G>A (1) Fragment size range - 98-261 bpFragment size range - 98-261 bp –Strong correlation between fragment size and WT – Het difference (r=0.93) –No correlation between WT – Mut difference and fragment size (r=0.12) 50-60% GC50-60% GC 100% genotype concordance100% genotype concordance –TaqMan (350) –Sequencing (68)

Download ppt "Modified Allele Dosage (MAD) Genotyping by Hi-Res Melting  of Whole Amplicons Jason T. McKinney Scientist Human Genetics Applications."

Similar presentations

Lecture 2 Strachan and Read Chapter 13

Lecture 2 Strachan and Read Chapter 13
Validation of BRCA2 mutation scanning using the LightScanner system for high resolution melt analysis Lewis Darnell Nottingham Regional Molecular Genetics.

Validation of BRCA2 mutation scanning using the LightScanner system for high resolution melt analysis Lewis Darnell Nottingham Regional Molecular Genetics.
Development of a BRCA2 screening service – Introduction of high resolution MELT analysis A Grade Trainee Project Nick Camm Yorkshire Regional Genetics.

Development of a BRCA2 screening service – Introduction of high resolution MELT analysis A Grade Trainee Project Nick Camm Yorkshire Regional Genetics.
Mutation Scanning and Genotyping by High- Resolution DNA Melting Analysis Carl Wittwer, MD, PhD Professor of Pathology University of Utah.

Mutation Scanning and Genotyping by High- Resolution DNA Melting Analysis Carl Wittwer, MD, PhD Professor of Pathology University of Utah.
DNA was extracted from whole blood using 3 extraction instruments: Radius (Protedyne, Windsor, CT) and MagNA Pure (Roche Applied Science, Indianapolis,

DNA was extracted from whole blood using 3 extraction instruments: Radius (Protedyne, Windsor, CT) and MagNA Pure (Roche Applied Science, Indianapolis,
Assessment of a high-throughput DNA melting analysis assay for rapid screening of gene variants in the ornithine transcarbamylase gene K. Sumner*, L. Hubley*,

Assessment of a high-throughput DNA melting analysis assay for rapid screening of gene variants in the ornithine transcarbamylase gene K. Sumner*, L. Hubley*,
Fundamental in Real Time PCR

Fundamental in Real Time PCR
Tools for Molecular Biology Amplification. The PCR reaction is a way to quickly drive the exponential amplification of a small piece of DNA. PCR is a.

Tools for Molecular Biology Amplification. The PCR reaction is a way to quickly drive the exponential amplification of a small piece of DNA. PCR is a.
RNA Lab (Isolation, quantification and qPCR analysis) MCB7300.

RNA Lab (Isolation, quantification and qPCR analysis) MCB7300.
Figure 1. Melting curve of SNP marker D1 of probe and PCR amplicon on LightScanner. SNA D1 is CA or CA deletion. It is very clear to see the genotype by.

Figure 1. Melting curve of SNP marker D1 of probe and PCR amplicon on LightScanner. SNA D1 is CA or CA deletion. It is very clear to see the genotype by.
SNP Genotyping Without Probes by High Resolution Melting of Small Amplicons Robert Pryor 1, Michael Liew 2 Robert Palais 3, and Carl Wittwer 1, 2 1 Dept.

SNP Genotyping Without Probes by High Resolution Melting of Small Amplicons Robert Pryor 1, Michael Liew 2 Robert Palais 3, and Carl Wittwer 1, 2 1 Dept.
SNP Discovery in the Human Genome C244/144 November 21, 2005.

SNP Discovery in the Human Genome C244/144 November 21, 2005.
High Resolution Melting

High Resolution Melting
What Can You Do With qPCR?

What Can You Do With qPCR?
Lecture 10: DNA Quantitation.  Purpose of DNA quantitation  Quantitation Methods  Interchelating dyes  Slot blot  qPCR ▪ Taqman (Life Technologies.

Lecture 10: DNA Quantitation.  Purpose of DNA quantitation  Quantitation Methods  Interchelating dyes  Slot blot  qPCR ▪ Taqman (Life Technologies.
SNP’s: Which Method is Best for Your Study?

SNP’s: Which Method is Best for Your Study?
Real Time PCR = Quantitative PCR.

Real Time PCR = Quantitative PCR.
Real-Time PCR (Quantitative PCR)

Real-Time PCR (Quantitative PCR)
Variants of PCR Lecture 4

Variants of PCR Lecture 4
COBAS AmpliPrep/Cobas TaqMan HIV-1 Test

COBAS AmpliPrep/Cobas TaqMan HIV-1 Test

Similar presentations

Ads by Google