Published: Vol 4, Iss 20, Oct 20, 2014 DOI: 10.21769/BioProtoc.1272 Views: 11822
Reviewed by: Kanika GeraEmilia Krypotou Anonymous reviewer(s)
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Abstract
There are several methods to measure the capacity of yeast cell to respond to environmental impacts on their genome by mutating it. One frequently used method involves the detection of forward mutations in the CAN1 gene. The CAN1 gene encodes for an arginine permease that is responsible for the uptake of arginine and it can also transport the toxic analog of arginine, canavanine (Whelan et al., 1979). When CAN1 cells are grown on a media containing canavanine but lacking arginine, the cells die because of the uptake of the toxic canavanine. However, if a mutation in the CAN1 gene inactivates the permease, that cell survives and forms a colony on the plate.
The following protocol describes the measurement of UV-induced mutagenesis at the CAN1 locus.
Materials and Reagents
Equipment
Procedure
Representative data
Recipes
Yeast nitrogen base [w/o amino acids and w (NH4)2SO4] | 400 g |
Adenine | 1.8 g |
Arginine | 1.2 g |
Histidine | 1.2 g |
Isoleucine | 1.8 g |
Leucine | 1.8 g |
Lysine | 1.8 g |
Methionine | 1.2 g |
Phenylalanine | 3.0 g |
Tryptophan | 1.2 g |
Tyrosine | 1.8 g |
Uracil | 1.2 g |
Valine | 9.0 g |
Acknowledgments
We used this protocol in our work (Daraba et al., 2014). Funding support: Wellcome Trust, 070247/Z/03/A.
References
Article Information
Copyright
© 2014 The Authors; exclusive licensee Bio-protocol LLC.
How to cite
Unk, I. and Daraba, A. (2014). Measuring UV-induced Mutagenesis at the CAN1 Locus in Saccharomyces cerevisiae. Bio-protocol 4(20): e1272. DOI: 10.21769/BioProtoc.1272.
Category
Microbiology > Microbial genetics > Mutagenesis
Microbiology > Microbial genetics > DNA
Molecular Biology > DNA > Mutagenesis
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