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Map-based cloning of interesting genes In a model organism 1. Generate mutants by mutagenesis of seeds Use a genetic background with lots of known polymorphisms compared to other genotypes. Availability of polymorphic markers for mapping. 2. Select mutants with phenotypes of interest eg. Hairless or Glabra 3. Clean up mutant genotype by backcross to wild type all F1 will be heterozygous, mutant phenotype will be either dominant or recessive. 4. Allelism tests with mutants that look similar 5. Select F2’s that are homozygous for the mutation again. These can be used to map the location of the mutation. GLABRA1 (GL1) • Involved in trichome initiation – Transcription factor – Expressed in leaf primordia early trichome initiation • gl1 mutants result in near complete loss of trichome initiation Wild type gl1 mutant Scanning EM picture of Arabidopsis top leaf surface with trichomes Mapping Cross Parents: Col-0 gl1/gl1 X La-er GL1/GL1 genotypes F1 is self fertilized – all chromosomes recombine in meiosis F2 plants – recombined chromosomes segregate How to do this with an organism that cannot fertilize itself, like a mouse? Mapping an Arabidopsis gene Analyze segregation data in an F2 population. Both chromosomes have had the opportunity to become recombined in the F1 parent To avoid confusion, we focus on one locus of interest. We chose individuals that are homozygous for one allele at that locus, eg. a clear phenotype. Closely linked markers will also be homozygous in the chosen individuals. As markers are farther away on the chromosome, more of the individuals will have two different alleles for the marker genes. Interval mapping: Identify markers linked to the gene of interest that define an interval on a chromosome. Markers that define major regions of the Arabidopsis chromosomes Marker 1 from a previous year. The first lane is the glabra mutant (Columbia), the second lane is a mixture of DNA from lane 1 and lane 3 The third lane is Landsberg The rest are DNA from F2 plants If marker is unlinked to GL1, we expect ¼ L/L, ½ L/C, ¼ C/C F2s are selected as homozygous recessive gl1/gl1 by phenotype eg. Scored for 5 markers marker 1 2 3 4 5 1, 2 are not linked to GL1 13: 25: 12 C/C:C/L:L/L Map distance is calculated as #recombinant alleles/total X 100 cM 50% of alleles are C and 50% are L. Therefore the map distance from GL1 to 1 is 50 cm. Marker 3 is linked to GL1. 46 C/C: 4 C/L: 0 L/L The map distance from GL1 to 3 is 4/100 X 100 cM or 4 cM. We established that gl1 is on Chromosome 3. What do we do next? We can only find a locus by identification of recombination events on either side. Identify 2 markers on Chromosome 3 that must be on either side of gl1 www.arabidopsis.org Tools Mapviewer Chr 3 Markers Zoom to 200X Clones Markers 3, 4 and 5 are linked to GL1 on chromosome 3 We need to find another marker on the opposite side of marker 3 to define the interval that contains GL1. 5 gl1? 3 gl1? 4 There is a recombination event between marker 3 and gl1 Is gl1 closer to the centromere or the telomere? Marker 5 is centromeric Marker 4 is telomeric Plants 3, 4, 5 and 10 are useful to identify flanking markers Plants 3, 4 and 5 have recombination points within the interval that defines the location of GL1 They will be useful for further mapping Plant 4 Plant 3 is C/L at 3 L/L at 4 and C/C at 5 Plant 4 is C/C at 3 C/C at 4 and C/Lat 5 Plant 5 is C/L at 3 C/L at 4 and C/C at 5 Col-0 La-er Plant 5 Plant 3 5 5 5 5 5 5 gl1 gl1 gl1 gl1 gl1 gl1 3 3 3 3 3 3 4 4 4 4 4 4 Identify more plants with recombination in the interval We will screen more F2 plants to identify those with a recombination on either side of our chosen interval to narrow in on the location of the GL1 gene. We will analyze the alleles of new markers located between marker 3 and marker 5. We will only analyze DNA from plants heterozygous at either marker 3 or marker 5. From comparison of genome sequence to a recombination map made by Lister and Dean, we learned that Arabidopsis has approximately 250 kb per map unit. That represents about 100 genes. For convenience, we aim for map resolution of 0.1 map units, which should represent 25-100 kb and hopefully 10-20 genes. 50-100 kb is the normal insert size for BAC clones. In order to get to map resolution of 0.1 map units we screen at least 1000 F2 plants (2000 chromosomes) How to decide the number of F2’s to examine? Recombination frequency is calculated: Number of recombinants/number of chromosomes, 1 recombinant chromosome/2000 chromosomes = 0.05 map units. We can only find a locus by identification of recombination events on either side. Therefore, with 2000 chromosomes we should find one marker 0.05 cM to the right of GL1 and another marker 0.05 cm to the left. An interval of 0.1 map units between the two closest markers is the best we measure. If we want better resolution, we need more markers (which we have) and more potential recombinant chromosomes from F2 plants. Once we have defined 2 markers flanking our interval that are physically close enough, we start sequence analysis for point mutations. MDF20 MYN21 BAC T22A15 100 kb insert BAC sequence gives us a list of genes. ~20 in Arabidopsis. GenBank annotation gives us a list of predicted genes for each BAC from our ordered library. Potential functions of the predicted genes are defined by homology to other proteins. Candidate genes can be chosen by predicted function and expression pattern. Go to TAIR for GL1 marker on AGI map click clone, then look at gene annotation Candidate genes can be PCR amplified from the mutant and the sequence can be compared to wild type. When a mutation is identified, we call that a candidate gene. Transform mutant plant with the wild type candidate gene for complementation. Alternatively, the entire BAC can be broken into subclones. Each subclone can be used to transform the mutant plant. If the BAC is made with wild type DNA, subclones with the correct gene in them will complement the mutation. Grant et al 1995 Science 269;843-846. Final confirmation • Sequence mutant and wild type – multiple mutant alleles needed to be convincing • Complement mutation by making a transgenic with the wild type copy of the candidate gene. Finding a gene based on phenotype • 1. 100’s of DNA markers mapped onto each chromosome – high density linkage map. • 2. identify markers linked to trait of interest by recombination analysis • 3. Narrow region down to a manageable length of DNA – for cloning and sequence comparison • 4. Compare mutant and wild type sequences to find differences that could cause mutant phenotype • 5. Prove that mutation is responsible for phenotype.