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使用人类H-ras原癌基因进行位点特异性DNA损伤处理的哺乳动物检测法。

Mammalian assay for site-specific DNA damage processing using the human H-ras proto-oncogene.

作者信息

Arcangeli L, Williams K J

机构信息

Biomedical Program, University of Alaska at Anchorage 99508, USA.

出版信息

Nucleic Acids Res. 1995 Jun 25;23(12):2269-76. doi: 10.1093/nar/23.12.2269.

Abstract

The human genomic H-ras proto-oncogene was inserted into an Epstein-Barr virus (EBV) vector (p220.2) that replicates synchronously with the cell cycle. Unique restriction enzyme sites, 30 bp apart, were created on either side of codon 12 to enable the construction of gapped heteroduplex (GHD) DNA. Depending upon experimental protocol, the gap could be located either on the coding (non-transcribed) strand or the non-coding (transcribed) strand. GHD DNA was created using a 1.8 kb segment of H-ras DNA containing exon 1, into which a synthetic 30 nucleotide oligomer containing a strand- and site-specific mismatched nucleotide was annealed. The 1.8 kb segment of H-ras DNA containing a codon 12; middle G:T, A:C or T:C mismatch has been religated with high efficiency into the EBV vector and transfected into NIH 3T3 cells using a mild liposome-mediated protocol. Subsequent hygromycin resistant NIH 3T3 colonies have been PCR amplified and sequenced. In this study, codon 12; middle nucleotide mismatch correction rates to wild-type G:C during replication in NIH 3T3 cells were 96.4% of G:T mismatches, 87.5% of A:C mismatches and 67% of T:C mismatches.

摘要

将人类基因组H-ras原癌基因插入到一种与细胞周期同步复制的爱泼斯坦-巴尔病毒(EBV)载体(p220.2)中。在密码子12两侧创建了相距30 bp的独特限制性酶切位点,以构建缺口异源双链(GHD)DNA。根据实验方案,缺口可位于编码(非转录)链或非编码(转录)链上。使用包含外显子1的1.8 kb H-ras DNA片段创建GHD DNA,将一个含有链和位点特异性错配核苷酸的30核苷酸合成寡聚物退火到该片段中。含有密码子12中G:T、A:C或T:C错配的1.8 kb H-ras DNA片段已高效重新连接到EBV载体中,并使用温和的脂质体介导方案转染到NIH 3T3细胞中。随后对潮霉素抗性NIH 3T3菌落进行PCR扩增和测序。在本研究中,NIH 3T3细胞复制过程中密码子12中间核苷酸错配校正为野生型G:C的比例分别为:G:T错配的96.4%、A:C错配的87.5%和T:C错配的67%。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/afdc/307017/8dbe33528b7d/nar00012-0202-a.jpg

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