Lipofection with Lipofectamine™ 2000 in a heparin‐free growth medium results in high transfection efficiency in chicken primordial germ cells

Author:

Watanabe Tenkai1,Ochi Yuta1,Kajihara Ryota1,Ichikawa Kennosuke23,Ezaki Ryo1,Matsuzaki Mei1,Horiuchi Hiroyuki12ORCID

Affiliation:

1. Laboratory of Immunobiology Graduate School of Integrated Sciences for Life Hiroshima University Higashi‐Hiroshima Japan

2. Genome Editing Innovation Center Hiroshima University Higashi‐Hiroshima Japan

3. The Roslin Institute University of Edinburgh Edinburgh UK

Abstract

AbstractPrimordial germ cells (PGCs) that can differentiate into gametes are used to produce genome‐edited chickens. However, the transfection efficiency into PGCs is low in chickens; therefore, the yield efficiency of PGCs modified via genome editing is problematic. In this study, we improved transfection efficiency and achieved highly efficient genome editing in chicken PGCs. For transfection, we used lipofection, which is convenient for gene transfer. Chicken PGC cultures require adding heparin to support growth; however, heparin significantly reduces lipofection efficiency (p < 0.01). Heparin‐induced lipofection efficiency was restored by adding protamine. Based on these results, we optimized gene transfer into chicken PGCs. Lipofectamine 2000 and our PGC medium were the most efficient transfection reagent and medium, respectively. Finally, based on established conditions, we compared the gene knock‐out efficiencies of ovomucoid, a major egg allergen, and gene knock‐in efficiencies at the ACTB locus. These results indicate that optimized lipofection is useful for CRISPR/Cas9‐mediated knock‐out and knock‐in. Our findings may contribute to the generation of genome‐edited chickens and stimulate research in various applications involving them.

Publisher

Wiley

Subject

Molecular Medicine,Applied Microbiology and Biotechnology,General Medicine

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