Presentation is loading. Please wait.

Presentation is loading. Please wait.

Sequence information can be obtained from single DNA molecules Ido Braslavsky, Benedict Hebert, Emil Kartalov Stephen R. Quake Article critique presented.

Published by Modified over 9 years ago

Similar presentations

Presentation on theme: "Sequence information can be obtained from single DNA molecules Ido Braslavsky, Benedict Hebert, Emil Kartalov Stephen R. Quake Article critique presented."— Presentation transcript:

1 Sequence information can be obtained from single DNA molecules Ido Braslavsky, Benedict Hebert, Emil Kartalov Stephen R. Quake Article critique presented by Véronique Lecault January 30 th, 2007 EECE 491c PNAS, 100(7):3960-3964 (2003)

2 EECE 491c Braslavsky et al. (2003) PNAS 100(7):3960-3964 2 The 1000$ Genome Challenge Human genome project: Current cost for mammalian genome: 2010 target: 2015 target: $3 billion $30 million $100 000 $1000 “Remember that time is money” -Benjamin Franklin, 1748

3 EECE 491c Braslavsky et al. (2003) PNAS 100(7):3960-3964 3 Routes to Genomic Sequence Source of DNA Amplification of a single DNA copy DNA amplification and/or modification Sequencing

4 EECE 491c Braslavsky et al. (2003) PNAS 100(7):3960-3964 4 What are the advantages of single molecule sequencing?  Individual fragments of DNA do not need to be amplified.  Sequencing can be in real-time (reading do not become dephased)  Low volumes required  Massive parallelization possible

5 EECE 491c Braslavsky et al. (2003) PNAS 100(7):3960-3964 5 The Experimental System

6 EECE 491c Braslavsky et al. (2003) PNAS 100(7):3960-3964 6 Results

7 EECE 491c Braslavsky et al. (2003) PNAS 100(7):3960-3964 7 Results 1.Expose primer 2.Photobleach primer 3.Flow dUTP-Cy3 + polymerase and wash out 4.Expose with green laser 5.Flow dCTP-Cy5 + polymerase and wash out 6.Expose with red laser 7.Flow dATP and dGTP + polymerase and wash out 8.Flow dCTP + polymerase and wash out 9.Expose with red laser

8 EECE 491c Braslavsky et al. (2003) PNAS 100(7):3960-3964 8 Results – Template 1 Yield : 50%

9 EECE 491c Braslavsky et al. (2003) PNAS 100(7):3960-3964 9 Results – Template 3 Yield : 10%

10 EECE 491c Braslavsky et al. (2003) PNAS 100(7):3960-3964 10 Results – Templates 1 & 2

11 EECE 491c Braslavsky et al. (2003) PNAS 100(7):3960-3964 11 Is That Enough for the Challenge? Limitations :  FRET readout length (5 nm – 15 pb)  DNA polymerase interaction with modified nucleotides  Far from de novo sequencing with 5 pb and only 2 nucleotides  Hard to assess consecutives bases

12 EECE 491c Braslavsky et al. (2003) PNAS 100(7):3960-3964 12 Critique Summary To be improvedGood Major points Minor points A signature of 5 bp with 2 nucleotides is not very impressive More work should be done to improve the yield and allow adjacent incorporations Current limitations of this technology are underestimated The time and cost of each experiment should be addressed Clever way of reducing background fluorescence Important step forward in single molecule DNA sequencing Solutions suggested to resolve some of the limitations Clear representation of FRET signaling It is not very clear to see what the correlogram correlates The paper is disappointing compared to the exciting abstract A picture without incorporation is missing for the reader

Download ppt "Sequence information can be obtained from single DNA molecules Ido Braslavsky, Benedict Hebert, Emil Kartalov Stephen R. Quake Article critique presented."

Similar presentations

RAPD Randomly Amplified Polymorphic DNA

RAPD Randomly Amplified Polymorphic DNA
Sequencing Using DNA dependant DNA polymerase Initiation & elongation commences Denature & anneal labelled primer * * dCTP dGTP dATP dTTPdCTP dATP dTTPdATP.

Sequencing Using DNA dependant DNA polymerase Initiation & elongation commences Denature & anneal labelled primer * * dCTP dGTP dATP dTTPdCTP dATP dTTPdATP.
Virus discovery-454 sequencing

Virus discovery-454 sequencing
COMPUTER EXERCISE Design of PCR and PCR-RFLP experiments This presentation shows all steps of a PCR-RFLP experiment and is a companion of the computer.

COMPUTER EXERCISE Design of PCR and PCR-RFLP experiments This presentation shows all steps of a PCR-RFLP experiment and is a companion of the computer.
Long-Term Monitoring of Bacteria Undergoing Programmed Population Control in a Microchemostat Frederick K. Balagaddé, Lingchong You, Carl L. Hansen, Frances.

Long-Term Monitoring of Bacteria Undergoing Programmed Population Control in a Microchemostat Frederick K. Balagaddé, Lingchong You, Carl L. Hansen, Frances.
RNA-Seq An alternative to microarray. Steps Grow cells or isolate tissue (brain, liver, muscle) Isolate total RNA Isolate mRNA from total RNA (poly.

RNA-Seq An alternative to microarray. Steps Grow cells or isolate tissue (brain, liver, muscle) Isolate total RNA Isolate mRNA from total RNA (poly.
PCR Basics Purpose of PCR Overview Components of PCR Reaction

PCR Basics Purpose of PCR Overview Components of PCR Reaction
PCR Basics 1.Purpose of PCR 2.Overview 3.Components of PCR Reaction 4.Variables Temperature Cycle Times and Numbers Primer Buffer Polymerase 5.Experimental.

PCR Basics 1.Purpose of PCR 2.Overview 3.Components of PCR Reaction 4.Variables Temperature Cycle Times and Numbers Primer Buffer Polymerase 5.Experimental.
RNA-Seq An alternative to microarray. Steps Grow cells or isolate tissue (brain, liver, muscle) Isolate total RNA Isolate mRNA from total RNA (poly.

RNA-Seq An alternative to microarray. Steps Grow cells or isolate tissue (brain, liver, muscle) Isolate total RNA Isolate mRNA from total RNA (poly.
PCR. PCR AMPLIFICATION PCR APPLICATIONS b MOLECULAR BIOLOGY b ENVIRONMENTAL SCIENCE b FORENSIC/MEDICAL SCIENCE b BIOTECHNOLOGY b GENETICS b GENE CLONING.

PCR. PCR AMPLIFICATION PCR APPLICATIONS b MOLECULAR BIOLOGY b ENVIRONMENTAL SCIENCE b FORENSIC/MEDICAL SCIENCE b BIOTECHNOLOGY b GENETICS b GENE CLONING.
Lab 8: PCR (Polymerase Chain Reaction)

Lab 8: PCR (Polymerase Chain Reaction)
Sanger-Coulson Dideoxynucleotide Sequencing Kwamina Bentsi-Barnes Deisy Mendoza Jennifer Aoki Lecture 10/30/00 Best printed in color for clarity.

Sanger-Coulson Dideoxynucleotide Sequencing Kwamina Bentsi-Barnes Deisy Mendoza Jennifer Aoki Lecture 10/30/00 Best printed in color for clarity.
CS 6293 Advanced Topics: Current Bioinformatics

CS 6293 Advanced Topics: Current Bioinformatics
The polymerase chain reaction (PCR) rapidly

The polymerase chain reaction (PCR) rapidly
1 100 120 University of Oklahoma Genome Center4/14/12.

University of Oklahoma Genome Center4/14/12.
Kamila Balušíková.  DNA – sequence of genes, repetitive sequence of noncoding regions  RNA  Proteins gene expression.

Kamila Balušíková.  DNA – sequence of genes, repetitive sequence of noncoding regions  RNA  Proteins gene expression.
Analyzing your clone 1) FISH 2) “Restriction mapping” 3) Southern analysis : DNA 4) Northern analysis: RNA tells size tells which tissues or conditions.

Analyzing your clone 1) FISH 2) “Restriction mapping” 3) Southern analysis : DNA 4) Northern analysis: RNA tells size tells which tissues or conditions.
From Haystacks to Needles AP Biology Fall 2010. Isolating Genes  Gene library: a collection of bacteria that house different cloned DNA fragments, one.

From Haystacks to Needles AP Biology Fall Isolating Genes  Gene library: a collection of bacteria that house different cloned DNA fragments, one.
Announcements Lab notebooks due Monday by 5 No Ch. 9 Part 2 homework

Announcements Lab notebooks due Monday by 5 No Ch. 9 Part 2 homework
A technique to make a lot of DNA from only a little!

A technique to make a lot of DNA from only a little!

Similar presentations

Ads by Google