农业科学与技术:英文版
農業科學與技術:英文版
농업과학여기술:영문판
Agricultural Science & Technology
2012年
4期
893-896
,共4页
阮楠%张明军%鞠辉明%白立景%赵为民
阮楠%張明軍%鞠輝明%白立景%趙為民
원남%장명군%국휘명%백립경%조위민
南苍术%正交设计%激素%基质
南蒼術%正交設計%激素%基質
남창술%정교설계%격소%기질
Porcine growth hormone gene promoter%Gene expression%Regulation
[目的]克隆猪生长激素启动子,确定其启动子核心序列和主要的顺式作用元件。[方法]根据NCBI上公布的序列设计引物,PCR扩增了猪生长激素5’端-1821~+61bp的序列,并通过移步缺失的方法,获得9段长短不一的启动子序列,将其分别构建到双荧光素酶表达载体pGL3-basic上。通过重组质粒瞬时转染大鼠垂体瘤细胞(GH3)、猪髋动脉血管内皮细胞(PIEC)和猪肾细胞(PK15)和转染后细胞荧光素酶活性的测定,检测这些5’末端缺失质粒在垂体及非垂体细胞中的相对转录活性。[结果]成功扩增了猪GH基因5’上游启动区1882bp的片段并构建了9个pGL3-mGHpromoter报告基因载体;双荧光素酶报告基因检测系统证实插入报告基因载体中的启动子具有非常强的细胞特异性。[结论]猪生长激素特异性在垂体细胞中表达,其最小启动子位于-110bp以内,启动子区-218—110bp和-429-218bp间存在正向调控元件。
[目的]剋隆豬生長激素啟動子,確定其啟動子覈心序列和主要的順式作用元件。[方法]根據NCBI上公佈的序列設計引物,PCR擴增瞭豬生長激素5’耑-1821~+61bp的序列,併通過移步缺失的方法,穫得9段長短不一的啟動子序列,將其分彆構建到雙熒光素酶錶達載體pGL3-basic上。通過重組質粒瞬時轉染大鼠垂體瘤細胞(GH3)、豬髖動脈血管內皮細胞(PIEC)和豬腎細胞(PK15)和轉染後細胞熒光素酶活性的測定,檢測這些5’末耑缺失質粒在垂體及非垂體細胞中的相對轉錄活性。[結果]成功擴增瞭豬GH基因5’上遊啟動區1882bp的片段併構建瞭9箇pGL3-mGHpromoter報告基因載體;雙熒光素酶報告基因檢測繫統證實插入報告基因載體中的啟動子具有非常彊的細胞特異性。[結論]豬生長激素特異性在垂體細胞中錶達,其最小啟動子位于-110bp以內,啟動子區-218—110bp和-429-218bp間存在正嚮調控元件。
[목적]극륭저생장격소계동자,학정기계동자핵심서렬화주요적순식작용원건。[방법]근거NCBI상공포적서렬설계인물,PCR확증료저생장격소5’단-1821~+61bp적서렬,병통과이보결실적방법,획득9단장단불일적계동자서렬,장기분별구건도쌍형광소매표체재체pGL3-basic상。통과중조질립순시전염대서수체류세포(GH3)、저관동맥혈관내피세포(PIEC)화저신세포(PK15)화전염후세포형광소매활성적측정,검측저사5’말단결실질립재수체급비수체세포중적상대전록활성。[결과]성공확증료저GH기인5’상유계동구1882bp적편단병구건료9개pGL3-mGHpromoter보고기인재체;쌍형광소매보고기인검측계통증실삽입보고기인재체중적계동자구유비상강적세포특이성。[결론]저생장격소특이성재수체세포중표체,기최소계동자위우-110bp이내,계동자구-218—110bp화-429-218bp간존재정향조공원건。
[Objective] This study aimed to clone the porcine growth hormone gene promoter and determine the core promoter sequences and the cis-acting elements. [Method] Sequence of the 5'flanking region of porcine growth hormone gene was searched out and downloaded from the NCBI website. According to the targeted se- quence, primers were designed and synthesized for the PCR amplification. The 1 882 bp (-1 821 bp-+61 bp) fragment was amplified by PCR. Nine promoter frag- ments with different lengths were obtained by genome-walking deletion method and then cloned into luciferase reporter vectors. Relative transcriptional activities of these 5' terminal-deleted plasmids in pituitary and non-pituitary cells were determined by transient transfection of the rat pituitary adenoma cell (GH3), porcine lilac endotheli- um cell (PIEC) and porcrne Kidney-15 (PK15) with the constructed dual-luciferase vectors. [Result] Result of DNA sequencing showed that the 1 882 bp fragment of GH 5' promoter was successfully cloned. Nine luciferase reporter gene plasmids were constructed. DuaI-Luciferase reporter assay indicated that the promoter inserted into reporter gene vector had very strong cell specificity. [Conclusion] Porcine growth hormone gene specifically expresses in pituitary cells. The minimal promoter of the porcine growth hormone gene is mapped at the region -110 bp-+61 bp. Promoter regions 218 bp--110 bp and -429 bp--218 bp contain positive regulatory elements.