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In Situ Synthesis of Peptide Nucleic Acids in PorousSilicon for Drug Delivery and Biosensing

机译:多孔中肽核酸的原位合成用于药物递送和生物传感的硅

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摘要

Peptide nucleic acids (PNA) are a unique class of synthetic molecules that have a peptide backbone and can hybridize with nucleic acids. Here, a versatile method has been developed for the automated, in situ synthesis of PNA from a porous silicon (PSi) substrate for applications in gene therapy and biosensing. Nondestructive optical measurements were performed to monitor single base additions of PNA initiated from (3-aminopropyl)triethoxysilane attached to the surface of PSi films, and mass spectrometry was conducted to verify synthesis of the desired sequence. Comparison of in situ synthesis to postsynthesis surface conjugation of the full PNA molecules showed that surface mediated, in situ PNA synthesis increased loading 8-fold. For therapeutic proof-of-concept, controlled PNA release from PSi films was characterized in phosphate buffered saline, and PSi nanoparticles fabricated from PSi films containing in situ grown PNA complementary to micro-RNA (miR) 122 generated significant anti-miR activity in a Huh7 psiCHECK-miR122 cell line. The applicability of this platform for biosensing was also demonstrated using opticalmeasurements that indicated selective hybridization of complementaryDNA target molecules to PNA synthesized in situ on PSi films. Thesecollective data confirm that we have established a novel PNA–PSiplatform with broad utility in drug delivery and biosensing.
机译:肽核酸(PNA)是一类独特的合成分子,具有肽主链并可以与核酸杂交。在这里,已经开发了一种通用方法,用于从多孔硅(PSi)基板自动原位合成PNA,用于基因治疗和生物传感。进行非破坏性光学测量以监测由附着于PSi膜表面的(3-氨基丙基)三乙氧基硅烷引发的PNA的单碱添加,并进行质谱分析以验证所需序列的合成。完整PNA分子的原位合成与合成后的表面共轭比较表明,表面介导的原位PNA合成增加了8倍的负载量。为了进行治疗性概念验证,在磷酸盐缓冲液中对PSi膜中PNA的受控释放进行了表征,由PSi膜制成的PSi纳米颗粒含有与微RNA(miR)122互补的原位生长的PNA,可在磷酸氢钙中产生显着的抗miR活性。 Huh7 psiCHECK-miR122细胞系。还使用光学技术证明了该平台在生物传感方面的适用性指示互补杂交的选择性测量在PSi膜上原位合成PNA的DNA靶分子。这些集体数据证实我们已经建立了新颖的PNA-PSi该平台在药物输送和生物传感方面具有广泛的用途。

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