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Quantitative measurement of allele-specific protein expression in a diploid yeast hybrid by LC-MS.


ABSTRACT: Understanding the genetic basis of gene regulatory variation is a key goal of evolutionary and medical genetics. Regulatory variation can act in an allele-specific manner (cis-acting) or it can affect both alleles of a gene (trans-acting). Differential allele-specific expression (ASE), in which the expression of one allele differs from another in a diploid, implies the presence of cis-acting regulatory variation. While microarrays and high-throughput sequencing have enabled genome-wide measurements of transcriptional ASE, methods for measurement of protein ASE (pASE) have lagged far behind. We describe a flexible, accurate, and scalable strategy for measurement of pASE by liquid chromatography-coupled mass spectrometry (LC-MS). We apply this approach to a hybrid between the yeast species Saccharomyces cerevisiae and Saccharomyces bayanus. Our results provide the first analysis of the relative contribution of cis-acting and trans-acting regulatory differences to protein expression divergence between yeast species.

SUBMITTER: Khan Z 

PROVIDER: S-EPMC3435501 | biostudies-literature | 2012

REPOSITORIES: biostudies-literature

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Quantitative measurement of allele-specific protein expression in a diploid yeast hybrid by LC-MS.

Khan Zia Z   Bloom Joshua S JS   Amini Sasan S   Singh Mona M   Perlman David H DH   Caudy Amy A AA   Kruglyak Leonid L  

Molecular systems biology 20120101


Understanding the genetic basis of gene regulatory variation is a key goal of evolutionary and medical genetics. Regulatory variation can act in an allele-specific manner (cis-acting) or it can affect both alleles of a gene (trans-acting). Differential allele-specific expression (ASE), in which the expression of one allele differs from another in a diploid, implies the presence of cis-acting regulatory variation. While microarrays and high-throughput sequencing have enabled genome-wide measureme  ...[more]

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