TRESK基因重组腺病毒载体转染大鼠背根神经节神经元的效果
TRESK기인중조선병독재체전염대서배근신경절신경원적효과
Transfection of rat dorsal root ganglion neurons with TRESK gene recombinant adenovirus vector
  • 万方数据
    中华麻醉学杂志 중화마취학잡지
    CHINESE JOURNAL OF ANESTHESIOLOGY
    2011年 9期 1059-1061 ,共3页

    周俊%姚尚龙%杨承祥%仲吉英%王汉兵%林文静%高润兴

    주준%요상룡%양승상%중길영%왕한병%림문정%고윤흥

    神经节,脊%神经元%钾通道%转染%腺病毒科 神經節,脊%神經元%鉀通道%轉染%腺病毒科
    신경절,척%신경원%갑통도%전염%선병독과
    Ganglia,spinal%Neurons%Potassium channels%Transfection%Adenoviridae
    目的 评价TRESK基因重组腺病毒载体(pAD/CMV/V5- DEST-TRESK)转染大鼠背根神经节(DRG)神经元的效果.方法 原代培养大鼠DRG神经元,调整细胞密度为6× 104个/ml.采用随机数字表法,将细胞随机分为3组,每组6孔,每孔1ml细胞悬液,TRESK基因重组腺病毒载体组(T组)每孔加入3×107 TU的pAD/C MV/V5-DEST- TRESK;腺病毒对照组(A组)每孔加入3× 107TU的阴性对照腺病毒( pAD/CMV/V5- DEST);对照组(C组)不加入腺病毒.于72 h后采用RT-PCR法检测TRESKmRNA表达,Western blot法检测TRESK表达.结果 与C组和A组比较,T组DRG神经元IRESK及其mRNA表达上调(P<0.05),C组和A组上述指标差异无统计学意义(P>0.05).结论 pAD/CMV/V5-DEST-TRESK可有效转染大鼠DRG神经元,上调其TRESK表达.
    목적 평개TRESK기인중조선병독재체(pAD/CMV/V5- DEST-TRESK)전염대서배근신경절(DRG)신경원적효과.방법 원대배양대서DRG신경원,조정세포밀도위6× 104개/ml.채용수궤수자표법,장세포수궤분위3조,매조6공,매공1ml세포현액,TRESK기인중조선병독재체조(T조)매공가입3×107 TU적pAD/C MV/V5-DEST- TRESK;선병독대조조(A조)매공가입3× 107TU적음성대조선병독( pAD/CMV/V5- DEST);대조조(C조)불가입선병독.우72 h후채용RT-PCR법검측TRESKmRNA표체,Western blot법검측TRESK표체.결과 여C조화A조비교,T조DRG신경원IRESK급기mRNA표체상조(P<0.05),C조화A조상술지표차이무통계학의의(P>0.05).결론 pAD/CMV/V5-DEST-TRESK가유효전염대서DRG신경원,상조기TRESK표체.
    Objective To transfect rat dorsal root ganglion (DRG) neurons with TRESK gene recombinant adenovirus vector.Methods Primary cultured DRG neurons were enzymatically isolated from newborn SD rats of both sexes and cultured in DMEM liquid culture medium.The density of the cells in suspension was 6 × 104/ml.The cells were randomly assigned to one of 3 groups ( n =6 wells each):group TRESK gene recombinant adenovirus vector (group T) ; group adenovirus (group A) and group control (group C).In group T TRESK gene recombinant adenovirus vector (pAD/CMV/V5-DEST-TRESK) 3 × 107 TU was added to each well.In group A simple adenovirus 3 × 107 TU was added to each well and in group C no adenovirus was added.After 72 h incubation the expression of TRESK mRNA and protein was detected by RT-PCR and Western blot respectively.Results The expression of TRESK mRNA and protein was significantly up-regulated in group T as compared with groups C and A.Conclusion The rat DRG neurons can be effectively transfected with TRESK gene recombinant adenovirus vector.
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