Literature DB >> 18612840

Identifying and genotyping transgene integration loci.

Zhong Liang1, Amy Marie Breman, Brenda R Grimes, Elliot D Rosen.   

Abstract

The random germline integration of genetically engineered transgenes has been a powerful technique to study the role of particular genes in variety of biological processes. Although the identification of the transgene insertion site is often not essential for functional analysis of the transgene, identifying the site can have practical benefit. Enabling one to distinguish between animals that are homozygous or hemizygous for the transgene locus could facilitate breeding strategies to produce animals with a large number of genetic markers. Furthermore, founder lines generated with the same transgene construct may exhibit different phenotypes and levels of transgene expression depending on the site of integration. The goal of this report was to develop a rapid protocol for the identification and verification of transgene insertion sites. To identify host genomic sequences at the coagulation Factor X transgene integration site, DNA from a tail snip of the transgenic mouse was digested with NcoI and circularized using T4 DNA ligase. Using appropriately positioned PCR primers annealing to a transgene fragment distal to a terminal transgene restriction site (NcoI), one could amplify a fragment containing the transgene terminal region and extending into the flanking genomic sequence at the insertion site. DNA sequence determination of the amplicon permitted identification of the insertion site using a BLASTN search. FISH analysis of a metaphase spread of primary fibroblasts derived from the transgenic mouse was consistent with the identification of insertion site near the end of mouse chromosome 14. Identification of transgene insertion sites will facilitate genotyping strategies useful for the construction of mice with multiple engineered genetic markers and to distinguish among different founder lines generated by the same transgene. Furthermore, identification of the insertion site is necessary to analyze unexpected phenotypes that might be caused by insertional inactivation of an endogenous gene.

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Year:  2008        PMID: 18612840     DOI: 10.1007/s11248-008-9190-7

Source DB:  PubMed          Journal:  Transgenic Res        ISSN: 0962-8819            Impact factor:   2.788


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3.  Blood coagulation factor X deficiency causes partial embryonic lethality and fatal neonatal bleeding in mice.

Authors:  M Dewerchin; Z Liang; L Moons; P Carmeliet; F J Castellino; D Collen; E D Rosen
Journal:  Thromb Haemost       Date:  2000-02       Impact factor: 5.249

4.  Genetic applications of an inverse polymerase chain reaction.

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Authors:  Angelina J Lay; Zhong Liang; Elliot D Rosen; Francis J Castellino
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6.  BLAST: improvements for better sequence analysis.

Authors:  Jian Ye; Scott McGinnis; Thomas L Madden
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  6 in total
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Review 3.  Lost in transgenesis: a user's guide for genetically manipulating the mouse in cardiac research.

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4.  Efficient mapping of transgene integration sites and local structural changes in Cre transgenic mice using targeted locus amplification.

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7.  Combining M-FISH and Quantum Dot technology for fast chromosomal assignment of transgenic insertions.

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8.  Mapping Transgene Insertion Sites Reveals Complex Interactions Between Mouse Transgenes and Neighboring Endogenous Genes.

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10.  Mapping transgene insertion sites reveals the α-Cre transgene expression in both developing retina and olfactory neurons.

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Journal:  Commun Biol       Date:  2022-05-03
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