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Download 2. Identifying coding sequences (genes)
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Transcript
Chapter 7 Analyzing DNA and gene structure, variation and expression 1. Sequencing and genotyping DNA • Standard/manual DNA sequencing using dideoxynucleotide chain terminators ddATP, ddGTP, ddCTP, and ddTTP. 07_01.jpg 07_02.jpg 07_02_2.jpg • Automated DNA sequencing using fluorophores and capillary gel electrophoresis. 07_03.jpg • Simple/basic genotyping by restriction site polymorphisms (RSPs) and varaible number tandem repeats (VNTRs) - RSPs: single nucleotide polymorphism may cause a loss or gain in a restriction site generating an RSP. Used in identifying carriers for some disease causing genes. - VNTR: use of PCR or Southern blot hybridization to identify differences in the number of microsatellite tandem repeats. 07_05.jpg 07_05_2.jpg 07_06.jpg 07_07.jpg 07_08.jpg 2. Identifying coding sequences (genes) in cloned DNA (e.g. libraries) and establishing their structure • Three features distinguish coding DNA from noncoding DNA: -i- coding sequences are highly conserved -ii- presence, in coding sequences, of open reading frames (ORFs). -iii- vertebrate coding sequences are often associated with CpG islands. • Routine/traditional methods for identifying evolutionary conserved coding sequences include zooblots. Recently, homology searching of sequence databases became a useful tool. 07_09.jpg • Besides routine methods, new more specialized procedures are used to identify coding sequences: -i- Exon trapping uses an artificial RNA splicing assay. -ii- cDNA selection by heteroduplex formation using magnetic beads capture identifies expressed sequences in genomic clones. 07_10.jpg 07_10_2.jpg 07_11.jpg 07_11_2.jpg -iii- To obtain full length cDNA of any gene, a cDNA library is screened using a probe (an oligonucleotide of the gene) and a set of overlapping truncated cDNA clones are produced. Then, RACE-PCR (rapid amplification of cDNA ends) is a technique used to extend the 5’ and/or 3’ ends of a short cDNA clone to onbtain a full length cDNA. 07_12.jpg 07_12_2.jpg -iv- Mapping transcription start site could be achieved by S1 nuclease protection or primer extension. 07_13.jpg 3. Studying gene expression • Principles of expression screening – in vitro versus in vivo. RNA analysis versus tissues and individual cells. 07_14.jpg 07_15.jpg 07_16.jpg 07_17.jpg 07_18.jpg 07_19.jpg
