基础医学与临床
基礎醫學與臨床
기출의학여림상
BASIC MEDICAL SCIENCES AND CLINICS
2009年
12期
1249-1253
,共5页
蒋宁%周利群%辛殿祺%吕天敬%韩文科
蔣寧%週利群%辛殿祺%呂天敬%韓文科
장저%주리군%신전기%려천경%한문과
RNA干扰%核小体结合蛋白%慢病毒%Western blot%MTT
RNA榦擾%覈小體結閤蛋白%慢病毒%Western blot%MTT
RNA간우%핵소체결합단백%만병독%Western blot%MTT
RNA interference%nucleosomal binding protein%lentivirus%Western blot%MTT
目的 构建和鉴定NSBP1基因RNA干扰慢病毒表达载体.方法 针对NSBP1 mRNA设计了3条siRNA,并构建pGCSIL-GFP-NSBP1慢病毒质粒,测序鉴定.用pGCSIL-GFP-NSBP1、pHelper1.0和pHelper2.0质粒共转染293T细胞包装产生慢病毒,测定病毒滴度.将慢病毒转染前列腺癌DU145细胞,Western-blot检测NSBP1表达,MTT法检测细胞生长活性,用转染细胞种植裸鼠成瘤,观察抑瘤效果.结果 PCR和测序证实,成功构建LV-shNSBP1的慢病毒载体,病毒滴度达2×10~8TU/mL.转染细胞中NSBP1蛋白表达显著降低,且MTT检测细胞生长活性明显减慢,转染细胞在裸鼠体内成瘤率没有影响,但对肿瘤的生长有明显抑制作用.结论 人NSBP1基因RNA干扰慢病毒载体构建成功,且NSBP1对前列腺癌激素非依赖DU145细胞的生长具有重要作用.
目的 構建和鑒定NSBP1基因RNA榦擾慢病毒錶達載體.方法 針對NSBP1 mRNA設計瞭3條siRNA,併構建pGCSIL-GFP-NSBP1慢病毒質粒,測序鑒定.用pGCSIL-GFP-NSBP1、pHelper1.0和pHelper2.0質粒共轉染293T細胞包裝產生慢病毒,測定病毒滴度.將慢病毒轉染前列腺癌DU145細胞,Western-blot檢測NSBP1錶達,MTT法檢測細胞生長活性,用轉染細胞種植裸鼠成瘤,觀察抑瘤效果.結果 PCR和測序證實,成功構建LV-shNSBP1的慢病毒載體,病毒滴度達2×10~8TU/mL.轉染細胞中NSBP1蛋白錶達顯著降低,且MTT檢測細胞生長活性明顯減慢,轉染細胞在裸鼠體內成瘤率沒有影響,但對腫瘤的生長有明顯抑製作用.結論 人NSBP1基因RNA榦擾慢病毒載體構建成功,且NSBP1對前列腺癌激素非依賴DU145細胞的生長具有重要作用.
목적 구건화감정NSBP1기인RNA간우만병독표체재체.방법 침대NSBP1 mRNA설계료3조siRNA,병구건pGCSIL-GFP-NSBP1만병독질립,측서감정.용pGCSIL-GFP-NSBP1、pHelper1.0화pHelper2.0질립공전염293T세포포장산생만병독,측정병독적도.장만병독전염전렬선암DU145세포,Western-blot검측NSBP1표체,MTT법검측세포생장활성,용전염세포충식라서성류,관찰억류효과.결과 PCR화측서증실,성공구건LV-shNSBP1적만병독재체,병독적도체2×10~8TU/mL.전염세포중NSBP1단백표체현저강저,차MTT검측세포생장활성명현감만,전염세포재라서체내성류솔몰유영향,단대종류적생장유명현억제작용.결론 인NSBP1기인RNA간우만병독재체구건성공,차NSBP1대전렬선암격소비의뢰DU145세포적생장구유중요작용.
Objective To construct and identify the efficacy of a lentiviral vector harboring RNAi sequence targe-ting NSBP1 gene. Methods Three siRNA targeting the NSBP1 mRNA were designed, the pGCSIL-GFP-NSBP1 lentivirus vectors were constructed and confirmed by DNA sequencing. A total of 293T cells were co-transfected with pGCSIL-GFP-NSBP1, pHelper1.0 and pHelper2.0 for the virus stocks produced, the titer of the virus was test-ed. After lentivirus transfecting into DU145 ceils, Western-blot and MTT methods were used to determine the ex-pression and biological activity of NSBP1 gene, the cells were transplanted into nude mice, then inhibitive effect was observed. Results PCR analysis and DNA sequencing demonstrated that the RNAi sequence targeting the hu-man NSBP1 gene was successfully inserted into the lentiviral vector. The titer of the recombinant]entiviral vector was 2 × 10~8TU/mL. NSBP1 protein expression level in transfected cells was significantly decreased and growth rate of cells transfected with lentivirus was decreased by MTT assay, the downregulation of NSBP1 reduced growth rate of transplantated tumor, whereas tumorgenicity was not influenced. Conclusion The construction of the]entiviral vector of NSBP1 has been successfully prepared and NSBP1 plays an important regulatory role in androgen-inde-pendent prostate cancer cell proliferation.
