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Antisense oligonucleotides selected by hybridisation to scanning arrays are effective reagents in vivo

机译:选择了反义寡核苷酸 通过与扫描阵列杂交是有效的试剂 体内

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摘要

Transcripts representing mRNAs of three Xenopus cyclins, B1, B4 and B5, were hybridised to arrays of oligonucleotides scanning the first 120 nt of the coding region to assess the ability of the immobilised oligonucleotides to form heteroduplexes with their targets. Oligonucleotides that produced high heteroduplex yield and others that showed little annealing were assayed for their effect on translation of endogenous cyclin mRNAs in Xenopus egg extracts and their ability to promote cleavage of cyclin mRNAs in oocytes by RNase H. Excellent correlation was found between antisense potency and affinity of oligonucleotides for the cyclin transcripts as measured by the array, despite the complexity of the cellular environment.
机译:将代表三个非洲爪蟾细胞周期蛋白B1,B4和B5的mRNA的转录本与扫描编码区前120 nt的寡核苷酸阵列杂交,以评估固定的寡核苷酸与其靶标形成异源双链体的能力。分析了产生高异源双链体产量的寡核苷酸和几乎没有退火的寡核苷酸对非洲爪蟾卵提取物中内源性cyclin mRNA的翻译的影响以及它们通过RNase H促进卵母细胞对cyclin mRNA裂解的能力。反义能力与尽管细胞环境复杂,但通过阵列测量寡核苷酸对细胞周期蛋白转录本的亲和力。

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