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Transcript
Chapter 21 Genomics Copyright © The McGraw-Hill Companies, Inc. Permission required for reproduction or display. Copyright © The McGraw-Hill Companies, Inc. Permission required for reproduction or display. Cytogenetic map: Three types of maps associated with the Genome sc (1A8) w (3B6) A B C D E FA 1 Obtained from analysis of polytene chromosomes 1 B C D 2 EF 2 A B C 3 3 Linkage map: sc w 1.5 mu The results from each type of mapping technique may be slightly different Physical map: sc D E F A B w ~ 2.4 x 106 bp Brooker, Figure 21.1 Copyright ©The McGraw-Hill Companies, Inc. Permission required for reproduction or display 4 C Fluorescence in situ hybridization Sister chromatids Treat cells with agents that make them swell and fixes them onto slide. Hybridized probe Denature chromosomal DNA. Add fluorescently labeled avidin, which binds to biotin. Denatured DNA (not in a doublehelix form) Fluorescent molecule bound to probe Add single-stranded DNA probes that have biotin incorporated into them. View with a fluorescence microscope. Figure 21.2 Copyright ©The McGraw-Hill Companies, Inc. Permission required for reproduction or display Copyright © The McGraw-Hill Companies, Inc. Permission required for reproduction or display. © : From Ried, T., Baldini, A., Rand, T.C., and Ward, D.C. "Simultaneous visualization of seven different DNA probes by in situ hybridization using combinatorial fluorescence and digital imaging microscopy. PNAS. 89: 4.1388-92. 1992. Courtesy Thomas Ried 21 - 13 EcoRI sites PRESENT on both chromosomes Copyright © The McGraw-Hill Companies, Inc. Permission required for reproduction or display. Region of two homologous chromosomes from individual 1 EcoRI 2000 bp EcoRI EcoRIEcoRI EcoRI 5000 bp 1500 bp 3000 bp EcoRI EcoRI EcoRI 2000 bp EcoRI 5000 bp 1500 bp 3000 bp 2500 bp EcoRI 2000 bp EcoRI 2000 bp 5000 bp 4500 bp EcoRI EcoRI 5000 bp EcoRI 2500 bp EcoRI 4500 bp EcoRI 2500 bp Region of two homologous chromosomes from individual 2 EcoRI EcoRI EcoRI EcoRI EcoRI sites ABSENT from both chromosomes EcoRI EcoRI 2500 bp Figure 21.4 Copyright ©The McGraw-Hill Companies, Inc. Permission required for reproduction or display 21 - 17 EcoRI site found only on one chromosome Copyright © The McGraw-Hill Companies, Inc. Permission required for reproduction or display. Region of two homologous chromosomes from individual 3 EcoRI 5000 bp 2000 bp EcoRI 2000 bp The three individuals share many DNA fragments that are identical in size. Indeed, if these segments are found in 99% of individuals in the population, they are termed monomorphic EcoRI EcoRI EcoRI 1500 bp 5000 bp 2500 bp 3000 bp EcoRI EcoRI EcoRI EcoRI EcoRI EcoRI 4500 bp 2500 bp Cut the DNA from all 3 individuals with EcoRI. Separate the DNA fragments by gel electrophoresis. 1 2 3 5000 bp 4500 bp 3000 bp Polymorphic bands are indicated at the arrows. 2500 bp 2000 bp Figure 21.4 1500 bp Copyright ©The McGraw-Hill Companies, Inc. Permission required for reproduction or display 21 - 18 Southern Blotting of RFLP Figure not in Brooker RFLPs (and other markers) can be mapped Figure not in Brooker Short Tandem Repeats (STR) TTTTC = (TTTTC)1 TTTTCTTTTCTTTTC = (TTTTC)3 TTTTCTTTTCTTTTCTTTTCTTTTCTTTTC = (TTTTC)5 Cataloging the world’s SNP variation www.hapmap.org PCR of microsatellites Set of chromosomes Add PCR primers. The PCR primers specifically recognize sequences on chromosome 2. The two STS copies in this case are different in length. Therefore, their microsatellites have different numbers of CA repeats Figure 21.5 2 2 Many cycles of PCR produce a large amount of the DNA fragment contained between the 2 primers. Gel electrophoresis Copyright © The McGraw-Hill Companies, Inc. Permission required for reproduction or display. Parents 1 2 Offspring 3 4 5 3 4 5 (a) Pedigree Fragment length bp 1 2 154 150 146 140 (b) Electrophoretic gel of PCR products for a polymorphic microsatellite found in the family in (a). Figure 20.12 Copyright ©The McGraw-Hill Companies, Inc. Permission required for reproduction or display In human genetics, computer algorithms can be used to determine linkage The likelihood of linkage between two RFLPs is determined by the lod (logarithm of the odds) score method – Computer programs analyze pooled data from a large number of pedigrees or crosses involving many RFLPs – They determine probabilities that are used to calculate the lod score Probability of a certain degree of linkage Probability of independent assortment • lod score = log10 Copyright ©The McGraw-Hill Companies, Inc. Permission required for reproduction or display Physical Mapping A B C D E F GH I J K L M NO P Q R Clone individual pieces into vectors. A B C 1 D GH F 3 J I 5 NO M K 7 P 9 Vector B C 2 D E 4 F I GH 6 K L M P 8 Q R A collection of overlapping clones, known as a contig 10 The numbers denote the order of the members of the contig Figure 21.7 Copyright ©The McGraw-Hill Companies, Inc. Permission required for reproduction or display 21 - 31 Copyright © The McGraw-Hill Companies, Inc. Permission required for reproduction or display. Region of chromosome 11 Gene A Gene B 1.5 mu Gene A 1 2 Gene B 3 4 5 6 7 • Genes A and B had been mapped previously to specific regions of chromosome 11 – Gene A was found in the insert of clone #2 – Gene B was found in the insert of clone #7 • So Genes A and B can be used as genetic markers (i.e., reference points) to align the members of the contig Figure 21.8 Copyright ©The McGraw-Hill Companies, Inc. Permission required for reproduction or display 21 - 33 Copyright © The McGraw-Hill Companies, Inc. Permission required for reproduction or display. ARS (yeast origin of replication) Each arm has a different selectable marker. Therefore, it is possible to select for yeast cells with YACs that have both arms EcoRI site CEN (yeast centromere) Chromosomal DNA EcoRI is used at low concentrations so only some sites are digested ORI (E.coli origin of replication) Selectable marker gene TEL TEL (yeast telomere) Left arm Selectable Marker gene BamHI site Cut with EcoRI and BamHI. BamHI site Cut (occasionally) with a low concentration of EcoRI to yield very large fragments. + Right arm Fragment not needed in yeast + Mix and add DNA ligase. Yeast artificial chromosome (YAC) TEL Selectable marker gene Figure 21.9 ORI CEN ARS Large piece of chromosomal DNA Note: This is not drawn to scale. The chromosomal DNA is much larger than the YAC vector. Selectable marker gene TEL 21 - 36 Copyright © The McGraw-Hill Companies, Inc. Permission required for reproduction or display. lacZ cm R HindIII BamHI SphI parC parB BAC vector repE parA oriS 21 - 37 Copyright © The McGraw-Hill Companies, Inc. Permission required for reproduction or display. Chromosome 16 95 million bp Cytogenetic map (resolution of in situ hybridization 3–5 megabases) Linkage map (resolution 3–5 cM; not all linkage markers are shown) D16S144 D16S40 D16S160 22.1 22.2 22.3 23.1 23.2 23.3 24.1 24.2 24.3 21.0 12.2 13.0 * D16S150 D16S149 11.2 D16AC6.5 12.1 11.1 D16S48 11.2 13.2 13.13 13.12 13.11 D16S159 12.3 12.2 12.1 q D16S60 D16S85 13.2 Low resolution (3–5 million bp) p * YAC N16Y1 150,000 bp * 310C4 N16Y1-29 Physical map of overlapping cosmid clones (resolution 5–10 kilobases) = (GT)n N16Y1-18 N16Y1-13 N16Y1-14 N16Y1-12 N16Y1-16 N16Y1-30 High resolution (1–100,000 bp) Cosmid contig 211 5F3 312F1 309G11 N16Y1-19 N16Y1-10 * STS N16Y1-10 Primer 3′ 5′ 3′ AGTCAAACGTTTCCGGCCTA GATCAAGGCGTTACATGA TCAGTTTGCAAAGGCCGGAT CTAGTTCCGCAATGTACT AGTCAAACGTTTCCGGCCTA 5′ 3′ Sequence-tagged site 5′ (resolution 1 base) 5′— GATCAAGGCGTTACATGA — 3′ Primer 219 bp Figure 21.11 21 - 39 Copyright © The McGraw-Hill Companies, Inc. Permission required for reproduction or display. Gene B 1 Gene B Gene A 2 3 4 5 Numbers indicate regions that are subcloned. (Starting clone) The number of steps required to reach the gene of interest depends on the distance between the start and end points Cosmid vector Subclone. Screen a library. 1 2 ....n (Second clone) Subclone. 2 Screen a library. 2 3 (Third clone) Repeat subcloning and screening until gene A is reached. n Figure 20.18 Gene A 21 - 42 Copyright © The McGraw-Hill Companies, Inc. Permission required for reproduction or display. Isolate chromosomal DNA Isolate chromosomal DNA Clone large chromosomal DNA fragments into BACs and create a contig for each chromosome. Shear DNA into small and large pieces. Clone chromosomal DNA pieces into vectors. BAC vector Vector BAC contig Chromosomal DNA For each BAC, shear into smaller pieces and clone DNA pieces into vectors. Chromosomal DNA Vector Clones from one BAC insert: Chromosomal DNA From the clones of each BAC, determine the chromosomal DNA sequence, usually at one end, by shotgun sequencing. The results below show the sequences from three chromosomal DNA clones. CCGA CCT T A CCGACCA G A C C A C C C GA T T A A T T T A A T C GC GA A T T G Based on overlapping regions, create one contiguous sequence. C C G A C C T T A C C GA C C A C C C G A T T A A T C G C GA A T T G (a) Hierarchical genome shotgun sequencing Figure 21.14 Determine the chromosomal DNA sequence, usually at both ends, by shotgun sequencing. The results below show sequences of three chromosomal DNA clones. T T A C C G G T A GGC A C C T C A C C T GT T A C GGGT C GGGT C A A A C C T A GG Based on overlapping regions, create one contiguous sequence. T T A C C GGT A G G C A C C T G T T A C G GG T C A A A C C T A G G (b) Whole-genome shotgun sequencing 21 - 46 Copyright © The McGraw-Hill Companies, Inc. Permission required for reproduction or display. Isolate genomic DNA and break into fragments. Deposit the beads into a picotiter plate. Only one bead can fit into each well. Fragment of genomic DNA Covalently attach oligonucleotide adaptors to the 5′ and 3′ ends of the DNA. Adaptors Denature the DNA into single strands and attach to beads via the adaptors. Note: Only one DNA strand is attached to a bead. Add sequencing reagents: DNA polymerase, primers, ATP sulfurylase, luciferase, apyrase, adenosine 5′ phosphosulfate, and luciferin. Sequentially flow solutions containing A, T, G, or C into the wells. In the example below, T has been added to the wells. PPi (pyrophosphate) is released when T is incorporated into the growing strand. T C Emulsify the beads so there is only one bead per droplet. The droplets also contain PCR reagents that amplify the DNA. A T T C G A Primer PPi + Adenosine 5′ phosphosulfate ATP sulfurylase ATP + luciferin Luciferase Light Light is detected by a camera in the sequencing machine. 21 - 48
