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restriction mapping (Physical mapping).pdf

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This PDF document provides a comprehensive overview of restriction mapping, a foundational technique in molecular biology that allows researchers to decipher the intricate genetic architecture of DNA molecules. Focusing on the utilization of restriction enzymes, this guide elucidates the principles, methods, and applications of restriction mapping, serving as a valuable resource for researchers, students, and enthusiasts in the field. This PDF document aims to demystify the intricacies of restriction mapping, offering both beginners and seasoned researchers an in-depth understanding of the first physical mapping technique and its continued relevance in the era of advanced genomic technologies.

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Physical mapping
Steps to map the GEnome Markers to generate highly saturated map Physical map Sequencing for the whole genome
Steps to map the GEnome Markers to generate highly saturated map Physical map Sequencing for the whole genome
Why we need to make physical mapping?
Why we need physical mapping? A map generated by genetic techniques is rarely sufficient for directing the sequencing phase of a genome project The resolution of a genetic map depends on the number of c.o. that have been scored
Why we need physical mapping? The resolution of a genetic map depends on the number of c.o. that have been scored: • it is not possible in eukaryotes to obtain large number of progeny, so relatively few meiosis can be studied. • The resolving power of linkage analysis is restricted (markers that are several tens of kb apart may appear at the same position).
Why we need physical mapping? A map generated by genetic techniques is rarely sufficient for directing the sequencing phase of a genome project The resolution of a genetic map depends on the number of c.o. that have been scored Genetic maps have limited accuracy
Why we need physical mapping? Genetic maps have limited accuracy: • Genetic maps assume that c.o. occur at random along chromosomes. • The presence of recombination hotspots means that c.o. are more likely to occur at some points rather than at others.
Why we need physical mapping? A map generated by genetic techniques is rarely sufficient for directing the sequencing phase of a genome project The resolution of a genetic map depends on the number of c.o. that have been scored Genetic maps have limited accuracy
For most eukaryotes, a genetic map must be checked and supplemented by physical mapping techniques before large-scale DNA sequencing begins
Genetic maps • Abstract maps that place the relative location of genes or markers on chromosomes based on recombination frequency. • Distances between markers is measured in centimorgan. • Different markers could be used to generate genetic maps: 1. Morphological 2. Biochemical 3. molecular. Physical maps • Use landmarks within DNA sequences ranging from restriction sites to the actual DNA sequence. • Distances between “landmarks” are measured in base-pairs ( bp). • Knowledge of DNA sequence is not necessary • Three main techniques for generating physical maps : 1. Restriction mapping 2. FISH 3. STS mapping .
Most important physical mapping techniques Restriction mapping. Fluorescent in situ hybridization (FISH). Sequence tagged sites (STS) mapping.
Most important physical mapping techniques Restriction mapping. Fluorescent in situ hybridization (FISH). Sequence tagged sites (STS) mapping.
Restriction mapping • The first physical maps • Locates the relative positions on a DNA molecule of the recognition sequences for restriction endonucleases • Based on distances between restriction sites • Overlap between smaller segments can be used to assemble them into a contig (Continuous segment of the genome).
The scale of restriction mapping is limited by the sizes of the restriction fragments • As the number of cut sites increases • the numbers of single, double and partial restriction products increases. • Restriction mapping is more applicable to small rather than large molecules • Computer analysis can be used but problems still eventually arise.
If DNA molecule >50 kb • possible to construct an unambiguous restriction map for a selection of enzymes with 6 bp recognition sequences (this could cover a few viral and organelle genomes). • a detailed restriction map can then be built up from the cloned fragments(>50) as a preliminary to sequencing the cloned region <50 • there is a possibility of using restriction analysis for mapping genomes larger than 50kb by choosing enzymes expected to have infrequent cut sites "rare cutters" in the target DNA molecule.
Rare cutters fall into 2 categories Enzymes with 7 or 8 nucleotide recognition sequences • Sap I (5'- GCTCTTC-3’) • cuts every 4^7 = 16 384 bp • Sgf I (5' - GCGA TCGC-3') cuts every 4^8 = 65 536 bp. Enzymes whose recognition sequences contain motifs that are rare in the target DNA • SmaI (5'-CCCGGG-3‘) • Bss HII(5'-GCGCGC-3')
To separate large DNA fragments, it is necessary to replace linear electric field with a more complex field In an electrophoretic gel, the resolution decreases as the molecules get longer. Thus, molecules > 50 kb in length run as a single slowly migrating band in a standard agarose gel
Pulsed Field Gel Electrophoresis (PFGE) • PFGE resolves DNA molecules of 100 - 1 000 kb • changing the direction of the electric field in a way that causes large DNA fragments to re- align more slowly with the new field direction than do smaller molecules
Basic types of PFGE systems Field inversion PFGE (FIGE) • Using a standard gel box apparatus • Works by periodically reversing the direction of the electric field Contour clamped Homologous electric field (CHEF) • Using hexagonal box • Works by multiple electric fields
Standard biochemical extraction procedures
Standard biochemical extraction procedures
PFGE DNA samples are prepared using immobilized cells in agar blocks • very large DNA fragments are randomly sheared by physical forces • soaked in lysis buffer containing detergent and proteinase K. This method gently purifies the cellular DNA without subjecting it to the shearing forces produced by pipetting. • Following cell lysis, a protease inhibitor is soaked into the agar block to inactivate the proteinase K and the DNA is then digested with RE prior to placing the agar block into the well of the PFGE gel. • Once electrophoresis is initiated, the DNA fragments migrate out of the agar block and directly into the gel

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restriction mapping (Physical mapping).pdf

  • 2. Steps to map the GEnome Markers to generate highly saturated map Physical map Sequencing for the whole genome
  • 3. Steps to map the GEnome Markers to generate highly saturated map Physical map Sequencing for the whole genome
  • 4. Why we need to make physical mapping?
  • 5. Why we need physical mapping? A map generated by genetic techniques is rarely sufficient for directing the sequencing phase of a genome project The resolution of a genetic map depends on the number of c.o. that have been scored
  • 6. Why we need physical mapping? The resolution of a genetic map depends on the number of c.o. that have been scored: • it is not possible in eukaryotes to obtain large number of progeny, so relatively few meiosis can be studied. • The resolving power of linkage analysis is restricted (markers that are several tens of kb apart may appear at the same position).
  • 7. Why we need physical mapping? A map generated by genetic techniques is rarely sufficient for directing the sequencing phase of a genome project The resolution of a genetic map depends on the number of c.o. that have been scored Genetic maps have limited accuracy
  • 8. Why we need physical mapping? Genetic maps have limited accuracy: • Genetic maps assume that c.o. occur at random along chromosomes. • The presence of recombination hotspots means that c.o. are more likely to occur at some points rather than at others.
  • 9. Why we need physical mapping? A map generated by genetic techniques is rarely sufficient for directing the sequencing phase of a genome project The resolution of a genetic map depends on the number of c.o. that have been scored Genetic maps have limited accuracy
  • 10. For most eukaryotes, a genetic map must be checked and supplemented by physical mapping techniques before large-scale DNA sequencing begins
  • 11. Genetic maps • Abstract maps that place the relative location of genes or markers on chromosomes based on recombination frequency. • Distances between markers is measured in centimorgan. • Different markers could be used to generate genetic maps: 1. Morphological 2. Biochemical 3. molecular. Physical maps • Use landmarks within DNA sequences ranging from restriction sites to the actual DNA sequence. • Distances between “landmarks” are measured in base-pairs ( bp). • Knowledge of DNA sequence is not necessary • Three main techniques for generating physical maps : 1. Restriction mapping 2. FISH 3. STS mapping .
  • 12. Most important physical mapping techniques Restriction mapping. Fluorescent in situ hybridization (FISH). Sequence tagged sites (STS) mapping.
  • 13. Most important physical mapping techniques Restriction mapping. Fluorescent in situ hybridization (FISH). Sequence tagged sites (STS) mapping.
  • 14. Restriction mapping • The first physical maps • Locates the relative positions on a DNA molecule of the recognition sequences for restriction endonucleases • Based on distances between restriction sites • Overlap between smaller segments can be used to assemble them into a contig (Continuous segment of the genome).
  • 15.
  • 16. The scale of restriction mapping is limited by the sizes of the restriction fragments • As the number of cut sites increases • the numbers of single, double and partial restriction products increases. • Restriction mapping is more applicable to small rather than large molecules • Computer analysis can be used but problems still eventually arise.
  • 17. If DNA molecule >50 kb • possible to construct an unambiguous restriction map for a selection of enzymes with 6 bp recognition sequences (this could cover a few viral and organelle genomes). • a detailed restriction map can then be built up from the cloned fragments(>50) as a preliminary to sequencing the cloned region <50 • there is a possibility of using restriction analysis for mapping genomes larger than 50kb by choosing enzymes expected to have infrequent cut sites "rare cutters" in the target DNA molecule.
  • 18. Rare cutters fall into 2 categories Enzymes with 7 or 8 nucleotide recognition sequences • Sap I (5'- GCTCTTC-3’) • cuts every 4^7 = 16 384 bp • Sgf I (5' - GCGA TCGC-3') cuts every 4^8 = 65 536 bp. Enzymes whose recognition sequences contain motifs that are rare in the target DNA • SmaI (5'-CCCGGG-3‘) • Bss HII(5'-GCGCGC-3')
  • 19. To separate large DNA fragments, it is necessary to replace linear electric field with a more complex field In an electrophoretic gel, the resolution decreases as the molecules get longer. Thus, molecules > 50 kb in length run as a single slowly migrating band in a standard agarose gel
  • 20. Pulsed Field Gel Electrophoresis (PFGE) • PFGE resolves DNA molecules of 100 - 1 000 kb • changing the direction of the electric field in a way that causes large DNA fragments to re- align more slowly with the new field direction than do smaller molecules
  • 21. Basic types of PFGE systems Field inversion PFGE (FIGE) • Using a standard gel box apparatus • Works by periodically reversing the direction of the electric field Contour clamped Homologous electric field (CHEF) • Using hexagonal box • Works by multiple electric fields
  • 24. PFGE DNA samples are prepared using immobilized cells in agar blocks • very large DNA fragments are randomly sheared by physical forces • soaked in lysis buffer containing detergent and proteinase K. This method gently purifies the cellular DNA without subjecting it to the shearing forces produced by pipetting. • Following cell lysis, a protease inhibitor is soaked into the agar block to inactivate the proteinase K and the DNA is then digested with RE prior to placing the agar block into the well of the PFGE gel. • Once electrophoresis is initiated, the DNA fragments migrate out of the agar block and directly into the gel