| Literature DB >> 30085302 |
Zhong-Bin Wang1,2,3, Zhi-Qiang Du1,2,3, Wei Na1,2,3, Jun-Hong Jing1,2,3, Yu-Mao Li1,2,3, Li Leng1,2,3, Peng Luan1,2,3, Chun-Yan Wu1,2,3, Ke Zhang1,2,3, Yu-Xiang Wang1,2,3, Wen-Li Liu1,2,3, Hui Yuan1,2,3, Zhong-Hua Liu4, Yan-Shuang Mu4, Qing-Wen Meng5, Ning Wang1,2,3, Cai-Xia Yang1,2,3, Hui Li1,2,3.
Abstract
The generation of transgenic chickens is of both biomedical and agricultural significance, and recently chicken transgenesis technology has been greatly advanced. However, major issues still exist in the efficient production of transgenic chickens. This study was designed to optimize the production of enhanced green fluorescence protein (EGFP)-transgenic broilers, including egg windowing at the blunt end (air cell) of egg, and the direct transfection of circulating primordial germ cells by microinjection of the Tol2 plasmid-liposome complex into the early embryonic dorsal aorta. For egg windowing, we discovered that proper manipulation of the inner shell membrane at the blunt end could improve the rate of producing G0 transgenic roosters. From 27 G0 roosters, we successfully collected semen with EGFP-positive sperms from 16 and 19 roosters after direct fluorescence observation and fluorescence-activated cell sorting analyses (13 detected by both methods), respectively. After artificial insemination using the G0 rooster with the highest number of EGFP fluorescent sperm, one G1 EGFP transgenic broiler (1/81, 1.23%) was generated. Our results indicate that appropriate egg windowing and screening of potentially transgene-positive roosters can improve the production of germline-transmitted transgenic birds.Entities:
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Year: 2019 PMID: 30085302 DOI: 10.3382/ps/pey321
Source DB: PubMed Journal: Poult Sci ISSN: 0032-5791 Impact factor: 3.352