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Oral gene delivery: Strategies to improve stability of pDNA towards intestinal digestion.

机译:口服基因传递:改善pDNA对肠道消化的稳定性的策略。

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PURPOSE: Gastrointestinal (GI) nucleases are responsible for a rapid presystemic degradation of orally administered transgenes. Within the current study, the activity of these degrading enzymes as well as the effect of various nuclease inhibitors on the degradation process were evaluated in order to assess their potential as auxiliary agents in oral gene delivery. METHODS: Digestion assays of pDNA with DNaseI and in GI juices were performed in absence and presence of inhibitors. Consequently, a chitosan conjugate with covalently bound ethylendiaminetetraacetic acid disodium salt dihydrat (EDTA) was synthesized and its nuclease inhibitory properties were evaluated. RESULTS: Small intestinal juice was shown to possess a nuclease activity per millilitre corresponding to 0.02 Kunitz units of DNaseI. Inhibition studies revealed that inhibitory activity followed the ranking: EDTA > sodium dodecyl sulfate (SDS) > aurintricarboxylic acid (ATA) > poly (acrylic acid) > cysteine. The chitosan-EDTA conjugate offered good nuclease inhibiting properties. CONCLUSION: This study determined the nuclease activity of native porcine small intestinal juice as well as enterocytes homogenate. Moreover, several promising strategies to overcome this enzymatic barrier were identified.
机译:目的:胃肠道(GI)核酸酶负责口服施用的转基因的快速系统前降解。在当前的研究中,评估了这些降解酶的活性以及各种核酸酶抑制剂对降解过程的影响,以评估其作为口服基因递送辅助剂的潜力。方法:在不存在和存在抑制剂的情况下,用DNaseI和GI汁消化pDNA。因此,合成了具有共价结合的乙二胺四乙酸二钠盐二水合物(EDTA)的壳聚糖共轭物,并评估了其核酸酶抑制性能。结果:显示小肠汁每毫升具有核酸酶活性,相当于DNaseI的0.02 Kunitz单位。抑制研究表明抑制活性遵循以下等级:EDTA>十二烷基硫酸钠(SDS)>金三羧酸(ATA)>聚丙烯酸>半胱氨酸。壳聚糖-EDTA共轭物提供了良好的核酸酶抑制性能。结论:本研究确定了天然猪小肠汁以及肠细胞匀浆的核酸酶活性。此外,确定了克服该酶障碍的几种有希望的策略。

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