Recombineering, transfection, Western, IP and ChIP methods for protein tagging via gene targeting or BAC transgenesis

Research output: Contribution to journalResearch articleContributedpeer-review

Contributors

Abstract

Protein tagging offers many advantages for proteomic and regulomic research. Ideally, protein tagging is equivalent to having a high affinity antibody for every chosen protein. However, these advantages are compromised if the tagged protein is overexpressed, which is usually the case from cDNA expression vectors. Physiological expression of tagged proteins can be achieved by gene targeting to knock-in the protein tag or by BAC transgenesis. BAC transgenes usually retain the native gene architecture including all cis-regulatory elements as well as the exon-intron configurations. Consequently most BAC transgenes are authentically regulated (e.g. by transcription factors, cell cycle, miRNA) and can be alternatively spliced. Recombineering has become the method of choice for generating targeting constructs or modifying BACs. Here we present methods with detailed protocols for protein tagging by recombineering for BAC transgenesis and/or gene targeting, including the evaluation of tagged protein expression, the retrieval of associated protein complexes for mass spectrometry and the use of the tags in ChIP (chromatin immunoprecipitation).

Details

Original languageEnglish
Pages (from-to)437-452
Number of pages16
JournalMethods
Volume53
Issue number4
Publication statusPublished - Apr 2011
Peer-reviewedYes

External IDs

researchoutputwizard legacy.publication#57011
Scopus 79952708432
PubMed 21195765
ORCID /0000-0002-4754-1707/work/142248063
ORCID /0000-0001-7499-5125/work/142253611

Keywords

Keywords

  • BAC transgenesis, Chromatin immunoprecipitation, Gene targeting, Genotyping by long range PCR, Native affinity purification, Protein tagging, Recombineering, Western blotting