东北林业大学学报
東北林業大學學報
동북임업대학학보
JOURNAL OF NORTHEAST FORESTRY UNIVERSITY
2014年
11期
146-149
,共4页
李璐%李婷%李沐%吴炎%齐琳%崔东明%胡薇
李璐%李婷%李沐%吳炎%齊琳%崔東明%鬍薇
리로%리정%리목%오염%제림%최동명%호미
鹿茸细胞%miRNA-93-5p%血管内皮生长因子%转录调控%细胞增殖
鹿茸細胞%miRNA-93-5p%血管內皮生長因子%轉錄調控%細胞增殖
록용세포%miRNA-93-5p%혈관내피생장인자%전록조공%세포증식
Antler cells%miRNA-93-5p%Vascular endothelial growth factor%Transcriptional regulation%Cell prolif-eration
为了探讨miRNA-93-5p对梅花鹿血管内皮生长因子( VEGF)的转录调控作用及其与鹿茸细胞生长的关系,分离了鹿茸顶端软骨组织细胞,利用Trizol试剂法提取细胞总RNA,反转录合成cDNA。根据GenBank已发表的相关序列设计梅花鹿VEGF基因的3′端非编码区部分序列(3′UTR)特异引物并进行克隆,构建VEGF基因的3′UTR野生型及其突变体序列双荧光素酶报告基因载体并进行荧光素酶活性检测。再将人工合成的miRNA-93-5p模拟物转染鹿茸软骨细胞,MTT法检测鹿茸细胞体外增殖的变化;Western blotting分析VEGF蛋白的表达丰度。结果表明:成功获得了鹿茸组织VEGF基因的3′UTR序列,野生型序列长度为356 bp,突变体长度为336 bp。荧光素酶活性检测结果表明,转染野生型质粒组细胞荧光素酶活性降低,而转染突变体组细胞荧光素酶活性无明显变化。 MTT法和Western blotting结果显示,鹿茸细胞的体外增殖受到抑制,VEGF蛋白的表达水平下降,且呈时间依赖性。
為瞭探討miRNA-93-5p對梅花鹿血管內皮生長因子( VEGF)的轉錄調控作用及其與鹿茸細胞生長的關繫,分離瞭鹿茸頂耑軟骨組織細胞,利用Trizol試劑法提取細胞總RNA,反轉錄閤成cDNA。根據GenBank已髮錶的相關序列設計梅花鹿VEGF基因的3′耑非編碼區部分序列(3′UTR)特異引物併進行剋隆,構建VEGF基因的3′UTR野生型及其突變體序列雙熒光素酶報告基因載體併進行熒光素酶活性檢測。再將人工閤成的miRNA-93-5p模擬物轉染鹿茸軟骨細胞,MTT法檢測鹿茸細胞體外增殖的變化;Western blotting分析VEGF蛋白的錶達豐度。結果錶明:成功穫得瞭鹿茸組織VEGF基因的3′UTR序列,野生型序列長度為356 bp,突變體長度為336 bp。熒光素酶活性檢測結果錶明,轉染野生型質粒組細胞熒光素酶活性降低,而轉染突變體組細胞熒光素酶活性無明顯變化。 MTT法和Western blotting結果顯示,鹿茸細胞的體外增殖受到抑製,VEGF蛋白的錶達水平下降,且呈時間依賴性。
위료탐토miRNA-93-5p대매화록혈관내피생장인자( VEGF)적전록조공작용급기여록용세포생장적관계,분리료록용정단연골조직세포,이용Trizol시제법제취세포총RNA,반전록합성cDNA。근거GenBank이발표적상관서렬설계매화록VEGF기인적3′단비편마구부분서렬(3′UTR)특이인물병진행극륭,구건VEGF기인적3′UTR야생형급기돌변체서렬쌍형광소매보고기인재체병진행형광소매활성검측。재장인공합성적miRNA-93-5p모의물전염록용연골세포,MTT법검측록용세포체외증식적변화;Western blotting분석VEGF단백적표체봉도。결과표명:성공획득료록용조직VEGF기인적3′UTR서렬,야생형서렬장도위356 bp,돌변체장도위336 bp。형광소매활성검측결과표명,전염야생형질립조세포형광소매활성강저,이전염돌변체조세포형광소매활성무명현변화。 MTT법화Western blotting결과현시,록용세포적체외증식수도억제,VEGF단백적표체수평하강,차정시간의뢰성。
We isolated the cartilage cells from antler tip and extracted cells total RNA by Trizol reagent to explore the effect tran-scriptional regulation of miRNA-93-5p on vascular endothelial growth factor ( VEGF) and the relationship with the growth of antler cells, and synthesized cDNA by reverse transcription.With the published relative sequence in GenBank, we de-signed and cloned the specially primers of 3’ UTR of sika deer VEGF gene, constructed dual luciferase reporter gene vec-tors of VEGF gene 3’ UTR containing wild-type or mutant sequence, and detected the relative activity of luciferase.We de-tected the changes of the in vitro proliferation of cartilage cells by MTT after transfected cartilage cells using miRNA-93-5p mimics, and analyzed the expression abundance of VEGF protein by western blotting.We obtained 3’ UTR sequence of VEGF from antler tissue.The length of wild-type sequence is 356 bp and the length of mutant sequence is 336 bp.Lucifer-ase activity detection indicates that the luciferase activity of the wild-type plasmid transfected cells is reduced, whereas mu-tant cells have no obvious change of luciferase activity .By MTT assay and western blotting, antler cells are inhibited in vitro and the expression level of VEGF protein decrease along with the time increase.
