体外转录合成小干扰Rna干扰PC3细胞膜联蛋白II基因的研究。

Ya-Wei Yuan, Ai-Min Sun, Ying Lui, Long-Hua Chen, A G Banerjee
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引用次数: 0

摘要

目的:应用小干扰RNA (siRNA)沉默前列腺癌细胞PC3中膜联蛋白II基因的表达。方法:设计4个29个核苷酸的DNA模板寡核苷酸序列进行体外转录,其中1对序列与膜联蛋白II基因互补。另一对为阴性对照。每个寡核苷酸3'端的8个核苷酸与T7启动子引物互补。用T7 RNA聚合酶对正义和反义siRNA模板进行转录,并将转录的RNA进行杂交,生成dsRNA。将siRNA转染前列腺癌细胞PC3。为了检测siRNA的效率,采用共聚焦显微镜、Northern blotting和Western blotting检测膜联蛋白II蛋白及其mRNA的表达。3H胸腺嘧啶用于测定DNA合成。结果:膜联蛋白II基因特异性siRNA序列能够抑制膜联蛋白II蛋白及其mRNA的表达。转染siRNA的细胞DNA合成明显减少。结论:T7 RNA聚合酶合成siRNA的方案是可行的。膜联蛋白II可能参与DNA合成。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Rna interference of annexin II gene in PC3 cells by using small interference RNA synthesized with in vitro transcription.

Objective: To silence annexin II gene expression by using small interference RNA (siRNA) in prostate cancer cell line PC3.

Methods: For in vitro transcription, four sequences of 29-nucleotide DNA template oligonucleotides were designed, and one pair of the sequences were complementary to annexin II gene. The other pair was negative control. The 8 nucleotides at the 3' end of each oligonucleotide were complementary to the T7 Promoter Primer. The sense and antisense siRNA templates were transcribed by T7 RNA polymerase and the resulting RNA transcripts were hybridized to create dsRNA. The siRNA was transfected into prostate cancer cell PC3. For assaying the efficiency of siRNA, confocal microscopy, Northern blotting, and Western blotting were employed to examine the expression of annexin II protein and its mRNA. 3H thymidine was used to measure DNA synthesis.

Results: The siRNA sequence specific to annexin II gene was capable of inhibiting the expression of annexin II protein and its mRNA. And cellular DNA synthesis was significantly reduced in siRNA transfected cells.

Conclusions: The protocol for the synthesis of siRNA by T7 RNA polymerase is feasible. Annexin II might be involved in DNA synthesis.

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