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Synthesis and biological activity of phosphonoacetate- and thiophosphonoacetate-modified 2'-0-methyl oligoribonucleotides

机译:膦酰基乙酸酯和硫代膦酰基乙酸酯修饰的2'-0-甲基寡核糖核苷酸的合成及生物活性

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摘要

Chimeric 2'-O-methyl oligoribonucleotides (2'-OMe ORNs) containing intemucleotide linkages which were modified with phosphonoacetate (PACE) or thiophosphonoacetate (thioPACE) were prepared by solid-phase synthesis. The modified 2'-OMe ORNs contained a central phosphate or phosphorothioate sequence with up to 4 PACE or thioPACE modifications, respectively, at either end of the ORN in a "gapmer" motif. Both PACE and thioPACE 2'-OMe ORNs formed stable duplexes with complementary RNA. The majority of these duplexes had higher thermal melting temperatures than an unmodified RNA:RNA duplex. The modified 2'-OMe ORNs were effective passenger strands with complementary, unmodified siRNAs, for inducing siRNA activity in a dual luciferase assay in the presence of a lipid transfecting agent. As single strands, thioPACE 2'-OMe ORNs were efficiently taken up by HeLa cells in the absence of a lipid transfecting agent. Furthermore, thioPACE modifications greatly improved the potency of a 2'-OMe phosphorothioate ORN as an inhibitor of micro RNA-122 in Huh7 cells, without lipid transfection.
机译:通过固相合成制备了包含被核苷酸膦酸酯(PACE)或硫代膦酰基乙酸酯(thioPACE)修饰的核苷酸间键的嵌合2'-O-甲基寡核糖核苷酸(2'-OMe ORN)。修饰的2'-OMe ORN在“ gapmer”基序的ORN的任一端分别含有中央磷酸酯或硫代磷酸酯序列,具有最多4个PACE或thioPACE修饰。 PACE和thioPACE 2'-OMe ORN均与互补RNA形成稳定的双链体。这些双链体中的大多数比未修饰的RNA:RNA双链体具有更高的热解链温度。修饰的2'-OMe ORN是具有互补的,未修饰的siRNA的有效过客链,用于在脂质转染剂存在下的双重荧光素酶测定中诱导siRNA活性。作为单链,在没有脂质转染剂的情况下,HeLa细胞可有效吸收thioPACE 2'-OMe ORN。此外,thioPACE修饰极大地提高了2'-OMe硫代磷酸酯ORN作为Huh7细胞中微小RNA-122抑制剂的能力,而无需脂质转染。

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  • 来源
    《Organic & biomolecular chemistry》 |2012年第4期|p.746-754|共9页
  • 作者单位

    Department of Chemistry & Biochemistry, University of Colorado at Boulder, 215 UCB, Boulder, CO 80309-0215,USA;

    Medical Research Council, Laboratory of Molecular Biology, Hills Road,Cambridge, CB2 0QH, UK;

    Department of Chemistry & Biochemistry, University of Colorado at Boulder, 215 UCB, Boulder, CO 80309-0215,USA;

    Medical Research Council, Laboratory of Molecular Biology, Hills Road,Cambridge, CB2 0QH, UK;

    Department of Chemistry & Biochemistry, University of Colorado at Boulder, 215 UCB, Boulder, CO 80309-0215,USA;

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