Transfection and expression of exogenous gene in laying hens oviduct in vitro and in vivo

doi:10.1631/jzus.2005.B0137

Journal of Zhejiang University-SCIENCE B (Biomedicine & Biotechnology)

2005, Vol. 6

Issue (2): 137-141 DOI: 10.1631/jzus.2005.B0137

Biology & Biotechnology

Transfection and expression of exogenous gene in laying hens oviduct in vitro and in vivo

GAO Bo, SUN Huai-chang, SONG Cheng-yi, WANG Zhi-yue, CHEN Qin, SONG Hong-qin

School of Veterinary Medicine, Yangzhou University, Yangzhou 225009, China; School of Animal Science and Technology, Yangzhou University, Yangzhou 225009, China

Download:

PDF (0 KB)
Export: BibTeX | EndNote (RIS)

Abstract To examine whether or not the regulatory sequence of chicken ovalbumin gene can drive transgene expression specifically in hen oviduct, the authors constructed an oviduct-specific expression vector (pOV), containing 3.0 kilobases (kb) of the 5′-flanking sequence and 3.0 kb of the 3′-flanking sequence of the chicken ovalbumin gene. Jellyfish green fluorescence protein (EGFP) reporter gene and bacterial LacZ reporter gene were respectively inserted into the downstream of the 5′-regulatory region. The recombinants were named as pOVEGFP and pOVLacZ. Two transfer systems, in vitro and in vivo, were used to verify the function of the vector. In vitro, the plasmid DNA pOVEGFP and pEGFP-N1 were transfected respectively by the polyethyleneimine procedure into the primary chicken oviduct epithelium (PCOE) and fibroblasts cells isolated from laying hens. In vivo, the recombinant vector pOVLacZ was injected into egg-laying hens via wing vein and the tissues were collected for RT-PCR analysis. The results showed that expression of pEGFP-N1 was achieved at low level in oviduct epithelial cells and at high level in fibroblasts, but that the recombinant vector was not expressed in both cells. RT-PCR analysis showed that the LacZ gene was transcribed in the oviduct, but not in the heart, liver, kidney and spleen of the injected hens. Accordingly, the b-galactosidase activity was only detected in the oviduct magnum (116.7 mU/ml) and eggs (16.47 mU/ml). These results indicated that the cloned regulation regions of chicken ovalbumin gene could drive exogenous gene expression specifically in the oviducts of hens. In vivo gene injection via wing vein may serve as a rapid production system of recombinant proteins in chicken eggs. In addition, the cultured primary oviduct cells from laying hens were not efficient temporary expression systems for analyzing the function of regulating elements of ovalbumin gene.

Key words： Chicken ovalbumin gene regulatory regions Oviduct-specific expression vector Oviduct epithelium In vivo expression

Received: 02 February 2004

CLC:

Q952

	Service
	E-mail this article
	Add to my bookshelf
	Add to citation manager
	E-mail Alert
	RSS
	Articles by authors
	GAO Bo
	SUN Huai-chang
	SONG Cheng-yi
	WANG Zhi-yue
	CHEN Qin
	SONG Hong-qin

Cite this article:

GAO Bo, SUN Huai-chang, SONG Cheng-yi, WANG Zhi-yue, CHEN Qin, SONG Hong-qin. Transfection and expression of exogenous gene in laying hens oviduct in vitro and in vivo. Journal of Zhejiang University-SCIENCE B (Biomedicine & Biotechnology), 2005, 6(2): 137-141.

URL:

http://www.zjujournals.com/xueshu/zjus-b/10.1631/jzus.2005.B0137 OR http://www.zjujournals.com/xueshu/zjus-b/Y2005/V6/I2/137

[1]	YU Hai-ning, SHEN Sheng-rong, XIONG Yao-kang. Cytotoxicity of epigallocatechin-3-gallate to LNCaP cells in the presence of Cu2+[J]. Journal of Zhejiang University-SCIENCE B (Biomedicine & Biotechnology), 2005, 6( 2): 9-.

Viewed

Full text

Abstract

Cited

Shared

Discussed