Presentation is loading. Please wait.

Presentation is loading. Please wait.

PHYSICAL MAPPING AND POSITIONAL CLONING. Linkage mapping – Flanking markers identified – 1cM, for example Probably ~ 1 MB or more in humans Need very.

Published byElijah McDaniel Modified over 9 years ago

Similar presentations

Presentation on theme: "PHYSICAL MAPPING AND POSITIONAL CLONING. Linkage mapping – Flanking markers identified – 1cM, for example Probably ~ 1 MB or more in humans Need very."— Presentation transcript:

1 PHYSICAL MAPPING AND POSITIONAL CLONING

2 Linkage mapping – Flanking markers identified – 1cM, for example Probably ~ 1 MB or more in humans Need very many families to get closer than this in human, or very large populations

3 What to Do Next? Identify genes in this region Then determine what is the gene of interest

4 What to do next? In 1990, clone region around markers, make physical map(s), look for genes experimentally In 2000, use better physical maps, at least in some organisms In 2010, use bioinformatic knowledge, experimental proof still necessary

5 Physical Mapping A physical map is primarily based on the locations of landmarks along a DNA molecule and units of distance are expressed in base pairs.

6 Low Resolution Physical Mapping Cytogenetic map In situ hybridization

7

8

9

10

11

12 Chromosome Sorting Flow cytometry Used in library construction Also for chromosome paints

13

14 Pulsed Field Gel Electrophoresis

15

16

17 Polymerase Chain Reaction (PCR) Ability to generate identical high copy number DNAs made possible in the 1970s by recombinant DNA technology (i.e., cloning). Cloning DNA is time consuming and expensive (>>$15/sample). Probing libraries can be like hunting for a needle in a haystack. PCR, “discovered” in 1983 by Kary Mullis, enables the amplification (or duplication) of millions of copies of any DNA sequence with known flanking sequences. Requires only simple, inexpensive ingredients and a couple hours. DNA template Primers (anneal to flanking sequences) DNA polymerase dNTPs Mg 2+ Buffer Can be performed by hand or in a machine called a thermal cycler. 1993: Nobel Prize for Chemistry

18 Fig. 9.3 Denature Anneal PCR Primers Extend PCR Primers w/Taq Repeat…

19 Somatic Cell Genetics in Mammals

20

21

22

23 Radiation Hybrid Mapping

24

25 Fluorescent Dye Dideoxy-sequencing

26 Top-down mapping

27

28

29 Bottom-up Mapping (Contig Maps, Mapping With Ordered Clones)

30

31 African-AmericanAsian-ChineseHispanic-MexicanCaucasian Whose genome did Celera sequence? Supposedly: Actually: Celera’s genome is Craig Venter’s Science v. 291, pp 1304-1351

32 Cloning Vectors Plasmid Phagemid Cosmid, fosmid YACs BACs PACs

33

34

35

36 BAC Construction Scheme T7 Insert SP6 Insert size ; 50-300Kb ( mean 110kb) BAC vector (pIndigo 536)

37 Application Of BAC library BAC library Whole genome sequencing Construction of integrated genetic and physical map Fine mapping for interest gene Chromosome walking & contig assembly Positional cloning Fluorescent in situ hybridization

38

39

40 “virtual autorad” - real-time DNA sequence output from ABI 377 1.Trace files (dye signals) are analyzed and bases called to create chromatograms. 2.Chromatograms from opposite strands are reconciled with software to create double- stranded sequence data.

41 Maximum pyrosequencing read lengths currently are 300-500 nt. Commercial applications: 454 Life Sciences Genome Sequencer FLX Generate 400 million nt in 10 hours $5-7K USD per run $1M for mammalian genome

42

43

44

45 Zoo Blot

46

47 CpG islands

48 Northern Blots

49 Real-time Quantitative PCR: Measures the abundance of DNA as it is amplified. Useful for quantitatively measuring the levels of mRNA in a sample. Uses reverse transcriptase to generate cDNA for the template. Can also be used to quantitatively estimate fraction of DNA from various organisms in a heterogenous sample (e.g, can be used to measure abundance of different microbes in soil sample). Fluorescent dye, SYBR Green, is incorporated into PCR reaction. SYBR Green fluoresces strongly when bound to DNA, but emits little fluorescence when not bound to DNA. SYBR Green fluorescence is proportional to the amount of DNA amplified, detected with a laser or other device. Experimental samples are compared to control sample with known concentration of cDNA.

50 Fig. 10.9 SYBR Green binds to double-stranded DNA and fluoresces

51 Real-time Quantitative PCR amplification plot:

52 4h8h12h1d 15’30’1h2hNA4h8h12h1d 15’30’1h2hNA P. trifoliataC. paradisi PtCBF CORc115

53 Use trapped exons to identify candidate genes from cDNAs

54 Sequence Conservation Homology searches

55 Array Technology

56

57

58

59 Gene Complementation Mutants Overexpression “Knockouts” RNAi Reporter assays

60

61

62

63

64

65

Download ppt "PHYSICAL MAPPING AND POSITIONAL CLONING. Linkage mapping – Flanking markers identified – 1cM, for example Probably ~ 1 MB or more in humans Need very."

Similar presentations

Polymerase Chain Reaction

Polymerase Chain Reaction
DNA Technology & Gene Mapping Biotechnology has led to many advances in science and medicine including the creation of DNA clones via recombinant clones,

DNA Technology & Gene Mapping Biotechnology has led to many advances in science and medicine including the creation of DNA clones via recombinant clones,
Recombinant DNA Technology

Recombinant DNA Technology
Chapter Six Nucleic Acid Hybridization: Principles & Applications 1.Preparation of nucleic acid probes: - DNA: from cell-based cloning or by PCR. Probe.

Chapter Six Nucleic Acid Hybridization: Principles & Applications 1.Preparation of nucleic acid probes: - DNA: from cell-based cloning or by PCR. Probe.
SEQUENCING-related topics 1. chain-termination sequencing 2. the polymerase chain reaction (PCR) 3. cycle sequencing 4. large scale sequencing stefanie.hartmann.

SEQUENCING-related topics 1. chain-termination sequencing 2. the polymerase chain reaction (PCR) 3. cycle sequencing 4. large scale sequencing stefanie.hartmann.
9 Genomics and Beyond Brief Chapter Outline

9 Genomics and Beyond Brief Chapter Outline
Recombinant DNA Introduction to Recombinant DNA technology

Recombinant DNA Introduction to Recombinant DNA technology
Lecture 36: Cloning and Sequencing Genes. Lecture Outline, 12/5/05 Case Study: BRCA1, continued –Cloning DNA fragments into plasmids other vectors “Libraries”

Lecture 36: Cloning and Sequencing Genes. Lecture Outline, 12/5/05 Case Study: BRCA1, continued –Cloning DNA fragments into plasmids other vectors “Libraries”
1 Library Screening, Characterization, and Amplification Screening of libraries Amplification of DNA (PCR) Analysis of DNA (Sequencing) Chemical Synthesis.

1 Library Screening, Characterization, and Amplification Screening of libraries Amplification of DNA (PCR) Analysis of DNA (Sequencing) Chemical Synthesis.
DNA Sequencing and Gene Analysis

DNA Sequencing and Gene Analysis
Lecture ONE: Foundation Course Genetics Tools of Human Molecular Genetics I.

Lecture ONE: Foundation Course Genetics Tools of Human Molecular Genetics I.
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.
1 Characterization, Amplification, Expression Screening of libraries Amplification of DNA (PCR) Analysis of DNA (Sequencing) Chemical Synthesis of DNA.

1 Characterization, Amplification, Expression Screening of libraries Amplification of DNA (PCR) Analysis of DNA (Sequencing) Chemical Synthesis of DNA.
Applied Biosystems 7900HT Fast Real-Time PCR System I. Real-time RT-PCR analysis of siRNA-induced knockdown in mammalian cells (Amit Berson, Mor Hanan.

Applied Biosystems 7900HT Fast Real-Time PCR System I. Real-time RT-PCR analysis of siRNA-induced knockdown in mammalian cells (Amit Berson, Mor Hanan.
Making, screening and analyzing cDNA clones Genomic DNA clones

Making, screening and analyzing cDNA clones Genomic DNA clones
More Molecular Genetic Technologies (Chapters 8, 9, 10) 1.Polymerase Chain Reaction (PCR) 1.Standard PCR 2.Real-time quantitative PCR 2.DNA sequencing.

More Molecular Genetic Technologies (Chapters 8, 9, 10) 1.Polymerase Chain Reaction (PCR) 1.Standard PCR 2.Real-time quantitative PCR 2.DNA sequencing.
Polymerase Chain Reaction

Polymerase Chain Reaction
Fig 11-1 Chapter 11: recombinant DNA and related techniques.

Fig 11-1 Chapter 11: recombinant DNA and related techniques.
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.
HAPLOID GENOME SIZES (DNA PER HAPLOID CELL) Size rangeExample speciesEx. Size BACTERIA1-10 Mb E. coli: 4.639 Mb FUNGI10-40 Mb S. cerevisiae 13 Mb INSECTS.

HAPLOID GENOME SIZES (DNA PER HAPLOID CELL) Size rangeExample speciesEx. Size BACTERIA1-10 Mb E. coli: Mb FUNGI10-40 Mb S. cerevisiae 13 Mb INSECTS.

Similar presentations

Ads by Google