Rapid DNA extraction and PCR-sexing of mouse embryos

P J McClive; A H Sinclair

doi:10.1002/mrd.1081

Rapid DNA extraction and PCR-sexing of mouse embryos

Mol Reprod Dev. 2001 Oct;60(2):225-6. doi: 10.1002/mrd.1081.

Authors

P J McClive¹, A H Sinclair

Affiliation

¹ Department of Paediatrics, University of Melbourne and Murdoch Children's Research Institute, Royal Children's Hospital, Melbourne, Parkville, Australia. mcclivep@cryptic.rch.unimelb.edu.au

PMID: 11553922
DOI: 10.1002/mrd.1081

Abstract

We have devised a PCR-based sexing method that is quick, simple, and highly reproducible. DNA is first extracted from embryonic mouse yolk sac via a 15 min, two-step incubation procedure utilizing PCR-compatible proteinase K buffer. Without any further manipulation the lysate is subjected to 30 cycles of PCR, optimized to run in less than 1 hr. The reaction includes multiplexed primer pairs for Sry and Myog (myogenin) that generate a male specific band of 441 bp and an internal control band of 245 bp, respectively. This robust method is used routinely in our laboratory and gives rapid genotyping results with 98% reliability and 100% accuracy.

MeSH terms

Animals
DNA / isolation & purification*
DNA / metabolism
DNA-Binding Proteins / genetics
Embryo, Mammalian / physiology*
Female
Male
Mice
Myogenin / genetics
Nuclear Proteins*
Polymerase Chain Reaction / methods*
Sex Determination Processes*
Sex-Determining Region Y Protein
Time Factors
Transcription Factors*

Substances

DNA-Binding Proteins
Myog protein, mouse
Myogenin
Nuclear Proteins
Sex-Determining Region Y Protein
Sry protein, mouse
Transcription Factors
DNA