Published: Vol 3, Iss 8, Apr 20, 2013 DOI: 10.21769/BioProtoc.452 Views: 12955
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Abstract
In this protocol, determination of seed paternity by microsatellite markers in Nicotiana attenuata is described. However, this does not include a protocol for the novel marker selection/identification, but rather exploits the markers generated for a closely related species N. tabacum (Bindler et al., 2007). This is a high-throughput protocol optimized and streamlined for one skilled person to process 384 (96 x 4) seeds in 5 days, from DNA isolation (from seedlings) to paternity assessment by microsatellite genotype data.
Keywords: Microsatellite genotypingMaterials and Reagents
Equipment
Procedure
a) | Follow the procedure to measure concentration of DNA in Nanodrop. |
b) | Export to excel file for reference. |
1) | Select Show result-'best configuration'. |
2) | Copy the table of assigned father ID/mother ID to each sample. |
3) | Sort parents and count offsprings sired by them in excel. Population analysis in GenAlEx |
Recipes
Acknowledgments
This work was supported by the Max Planck Gesellschaft. The protocol was adapted from the publication: Kessler et al. (2012).
References
Article Information
Copyright
© 2013 The Authors; exclusive licensee Bio-protocol LLC.
How to cite
Bhattacharya, S. and Baldwin, I. T. (2013). High-throughput Method for Determination of Seed Paternity by Microsatellite Markers. Bio-protocol 3(8): e452. DOI: 10.21769/BioProtoc.452.
Category
Molecular Biology > DNA > Genotyping
Plant Science > Plant molecular biology > DNA
Plant Science > Plant physiology > Tissue analysis
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