A strategy for constructing aneuploid yeast strains by transient nondisjunction of a target chromosome

BACKGROUND: Most methods for constructing aneuploid yeast strains that have gained a specific chromosome rely on spontaneous failures of cell division fidelity. In Saccharomyces cerevisiae, extra chromosomes can be obtained when errors in meiosis or mitosis lead to nondisjunction, or when nuclear br...

Descripción completa

Detalles Bibliográficos
Autores principales: Anders, Kirk R, Kudrna, Julie R, Keller, Kirstie E, Kinghorn, BreAnna, Miller, Elizabeth M, Pauw, Daniel, Peck, Anders T, Shellooe, Christopher E, Strong, Isaac JT
Formato: Texto
Lenguaje:English
Publicado: BioMed Central 2009
Materias:
Methodology Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2725114/
https://www.ncbi.nlm.nih.gov/pubmed/19594932
http://dx.doi.org/10.1186/1471-2156-10-36
_version_ 1782170484925792256
author Anders, Kirk R
Kudrna, Julie R
Keller, Kirstie E
Kinghorn, BreAnna
Miller, Elizabeth M
Pauw, Daniel
Peck, Anders T
Shellooe, Christopher E
Strong, Isaac JT
author_facet Anders, Kirk R
Kudrna, Julie R
Keller, Kirstie E
Kinghorn, BreAnna
Miller, Elizabeth M
Pauw, Daniel
Peck, Anders T
Shellooe, Christopher E
Strong, Isaac JT
author_sort Anders, Kirk R
collection PubMed
description BACKGROUND: Most methods for constructing aneuploid yeast strains that have gained a specific chromosome rely on spontaneous failures of cell division fidelity. In Saccharomyces cerevisiae, extra chromosomes can be obtained when errors in meiosis or mitosis lead to nondisjunction, or when nuclear breakdown occurs in heterokaryons. We describe a strategy for constructing N+1 disomes that does not require such spontaneous failures. The method combines two well-characterized genetic tools: a conditional centromere that transiently blocks disjunction of one specific chromosome, and a duplication marker assay that identifies disomes among daughter cells. To test the strategy, we targeted chromosomes III, IV, and VI for duplication. RESULTS: The centromere of each chromosome was replaced by a centromere that can be blocked by growth in galactose, and ura3::HIS3, a duplication marker. Transient exposure to galactose induced the appearance of colonies carrying duplicated markers for chromosomes III or IV, but not VI. Microarray-based comparative genomic hybridization (CGH) confirmed that disomic strains carrying extra chromosome III or IV were generated. Chromosome VI contains several genes that are known to be deleterious when overexpressed, including the beta-tubulin gene TUB2. To test whether a tubulin stoichiometry imbalance is necessary for the apparent lethality caused by an extra chromosome VI, we supplied the parent strain with extra copies of the alpha-tubulin gene TUB1, then induced nondisjunction. Galactose-dependent chromosome VI disomes were produced, as revealed by CGH. Some chromosome VI disomes also carried extra, unselected copies of additional chromosomes. CONCLUSION: This method causes efficient nondisjunction of a targeted chromosome and allows resulting disomic cells to be identified and maintained. We used the method to test the role of tubulin imbalance in the apparent lethality of disomic chromosome VI. Our results indicate that a tubulin imbalance is necessary for disomic VI lethality, but it may not be the only dosage-dependent effect.
format Text
id pubmed-2725114
institution National Center for Biotechnology Information
language English
publishDate 2009
publisher BioMed Central
record_format MEDLINE/PubMed
spelling pubmed-27251142009-08-12 A strategy for constructing aneuploid yeast strains by transient nondisjunction of a target chromosome Anders, Kirk R Kudrna, Julie R Keller, Kirstie E Kinghorn, BreAnna Miller, Elizabeth M Pauw, Daniel Peck, Anders T Shellooe, Christopher E Strong, Isaac JT BMC Genet Methodology Article BACKGROUND: Most methods for constructing aneuploid yeast strains that have gained a specific chromosome rely on spontaneous failures of cell division fidelity. In Saccharomyces cerevisiae, extra chromosomes can be obtained when errors in meiosis or mitosis lead to nondisjunction, or when nuclear breakdown occurs in heterokaryons. We describe a strategy for constructing N+1 disomes that does not require such spontaneous failures. The method combines two well-characterized genetic tools: a conditional centromere that transiently blocks disjunction of one specific chromosome, and a duplication marker assay that identifies disomes among daughter cells. To test the strategy, we targeted chromosomes III, IV, and VI for duplication. RESULTS: The centromere of each chromosome was replaced by a centromere that can be blocked by growth in galactose, and ura3::HIS3, a duplication marker. Transient exposure to galactose induced the appearance of colonies carrying duplicated markers for chromosomes III or IV, but not VI. Microarray-based comparative genomic hybridization (CGH) confirmed that disomic strains carrying extra chromosome III or IV were generated. Chromosome VI contains several genes that are known to be deleterious when overexpressed, including the beta-tubulin gene TUB2. To test whether a tubulin stoichiometry imbalance is necessary for the apparent lethality caused by an extra chromosome VI, we supplied the parent strain with extra copies of the alpha-tubulin gene TUB1, then induced nondisjunction. Galactose-dependent chromosome VI disomes were produced, as revealed by CGH. Some chromosome VI disomes also carried extra, unselected copies of additional chromosomes. CONCLUSION: This method causes efficient nondisjunction of a targeted chromosome and allows resulting disomic cells to be identified and maintained. We used the method to test the role of tubulin imbalance in the apparent lethality of disomic chromosome VI. Our results indicate that a tubulin imbalance is necessary for disomic VI lethality, but it may not be the only dosage-dependent effect. BioMed Central 2009-07-13 /pmc/articles/PMC2725114/ /pubmed/19594932 http://dx.doi.org/10.1186/1471-2156-10-36 Text en Copyright © 2009 Anders et al; licensee BioMed Central Ltd. http://creativecommons.org/licenses/by/2.0 This is an Open Access article distributed under the terms of the Creative Commons Attribution License ( (http://creativecommons.org/licenses/by/2.0) ), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Methodology Article
Anders, Kirk R
Kudrna, Julie R
Keller, Kirstie E
Kinghorn, BreAnna
Miller, Elizabeth M
Pauw, Daniel
Peck, Anders T
Shellooe, Christopher E
Strong, Isaac JT
A strategy for constructing aneuploid yeast strains by transient nondisjunction of a target chromosome
title A strategy for constructing aneuploid yeast strains by transient nondisjunction of a target chromosome
title_full A strategy for constructing aneuploid yeast strains by transient nondisjunction of a target chromosome
title_fullStr A strategy for constructing aneuploid yeast strains by transient nondisjunction of a target chromosome
title_full_unstemmed A strategy for constructing aneuploid yeast strains by transient nondisjunction of a target chromosome
title_short A strategy for constructing aneuploid yeast strains by transient nondisjunction of a target chromosome
title_sort strategy for constructing aneuploid yeast strains by transient nondisjunction of a target chromosome
topic Methodology Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2725114/
https://www.ncbi.nlm.nih.gov/pubmed/19594932
http://dx.doi.org/10.1186/1471-2156-10-36
work_keys_str_mv AT anderskirkr astrategyforconstructinganeuploidyeaststrainsbytransientnondisjunctionofatargetchromosome
AT kudrnajulier astrategyforconstructinganeuploidyeaststrainsbytransientnondisjunctionofatargetchromosome
AT kellerkirstiee astrategyforconstructinganeuploidyeaststrainsbytransientnondisjunctionofatargetchromosome
AT kinghornbreanna astrategyforconstructinganeuploidyeaststrainsbytransientnondisjunctionofatargetchromosome
AT millerelizabethm astrategyforconstructinganeuploidyeaststrainsbytransientnondisjunctionofatargetchromosome
AT pauwdaniel astrategyforconstructinganeuploidyeaststrainsbytransientnondisjunctionofatargetchromosome
AT peckanderst astrategyforconstructinganeuploidyeaststrainsbytransientnondisjunctionofatargetchromosome
AT shellooechristophere astrategyforconstructinganeuploidyeaststrainsbytransientnondisjunctionofatargetchromosome
AT strongisaacjt astrategyforconstructinganeuploidyeaststrainsbytransientnondisjunctionofatargetchromosome
AT anderskirkr strategyforconstructinganeuploidyeaststrainsbytransientnondisjunctionofatargetchromosome
AT kudrnajulier strategyforconstructinganeuploidyeaststrainsbytransientnondisjunctionofatargetchromosome
AT kellerkirstiee strategyforconstructinganeuploidyeaststrainsbytransientnondisjunctionofatargetchromosome
AT kinghornbreanna strategyforconstructinganeuploidyeaststrainsbytransientnondisjunctionofatargetchromosome
AT millerelizabethm strategyforconstructinganeuploidyeaststrainsbytransientnondisjunctionofatargetchromosome
AT pauwdaniel strategyforconstructinganeuploidyeaststrainsbytransientnondisjunctionofatargetchromosome
AT peckanderst strategyforconstructinganeuploidyeaststrainsbytransientnondisjunctionofatargetchromosome
AT shellooechristophere strategyforconstructinganeuploidyeaststrainsbytransientnondisjunctionofatargetchromosome
AT strongisaacjt strategyforconstructinganeuploidyeaststrainsbytransientnondisjunctionofatargetchromosome

Ejemplares similares