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肽核酸及肽核酸-肽缀合物的细胞内摄取与基因表达抑制

Intracellular uptake and inhibition of gene expression by PNAs and PNA-peptide conjugates.

作者信息

Kaihatsu Kunihiro, Huffman Kenneth E, Corey David R

机构信息

Department of Pharmacology, University of Texas Southwestern Medical Center, 5323 Harry Hines Boulevard, Dallas, Texas 75390-9041, USA.

出版信息

Biochemistry. 2004 Nov 16;43(45):14340-7. doi: 10.1021/bi048519l.

Abstract

Peptide nucleic acids (PNAs) offer a distinct option for silencing gene expression in mammalian cells. However, the full value of PNAs has not been realized, and the rules governing the recognition of cellular targets by PNAs remain obscure. Here we examine the uptake of PNAs and PNA-peptide conjugates by immortal and primary human cells and compare peptide-mediated and DNA/lipid-mediated delivery strategies. We find that both peptide-mediated and lipid-mediated delivery strategies promote entry of PNA and PNA-peptide conjugates into cells. Confocal microscopy reveals a punctate distribution of PNA and PNA-peptide conjugates regardless of the delivery strategy used. Peptide D(AAKK)(4) and a peptide containing a nuclear localization sequence (NLS) promote the spontaneous delivery of antisense PNAs into cultured cells. The PNA-D(AAKK)(4) conjugate inhibits expression of human caveolin 1 (hCav-1) in both HeLa and primary endothelial cells. DNA/lipid-mediated delivery requires less PNA, while peptide-mediated delivery is simpler and is less toxic to primary cells. The ability of PNA-peptide conjugates to enter primary and immortal human cells and inhibit gene expression supports the use of PNAs as antisense agents for investigating the roles of proteins in cells. Both DNA/lipid-mediated and peptide-mediated delivery strategies are efficient, but the compartmentalized localization of PNAs suggests that improving the cellular distribution may lead to increased efficacy.

摘要

肽核酸(PNA)为沉默哺乳动物细胞中的基因表达提供了一种独特的选择。然而,PNA的全部价值尚未得到充分认识,PNA识别细胞靶点的规则仍不清楚。在这里,我们研究了永生化和原代人类细胞对PNA和PNA-肽缀合物的摄取,并比较了肽介导和DNA/脂质介导的递送策略。我们发现,肽介导和脂质介导的递送策略都能促进PNA和PNA-肽缀合物进入细胞。共聚焦显微镜显示,无论使用何种递送策略,PNA和PNA-肽缀合物均呈点状分布。肽D(AAKK)(4)和一种含有核定位序列(NLS)的肽促进反义PNA自发递送至培养细胞中。PNA-D(AAKK)(4)缀合物在HeLa细胞和原代内皮细胞中均能抑制人小窝蛋白1(hCav-1)的表达。DNA/脂质介导的递送所需的PNA较少,而肽介导的递送更简单,对原代细胞的毒性更小。PNA-肽缀合物进入原代和永生化人类细胞并抑制基因表达的能力支持将PNA用作反义试剂来研究蛋白质在细胞中的作用。DNA/脂质介导和肽介导的递送策略均有效,但PNA的区室化定位表明改善细胞分布可能会提高疗效。

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