Integration of [12]aneN3 and Acenaphtho[1,2-b]quinoxaline as non-viral gene vectors with two-photon property for enhanced DNA/siRNA delivery and bioimaging

Jin-Yu Liu; Xu-Ying Liu; Rui Liu; Fang Tang; Jing-Bo Yang; Quan Tang; Zhong-Lin Lu; Hai-Jun Qiao; Lan He

doi:10.1016/j.bioorg.2021.104983

Integration of [12]aneN3 and Acenaphtho[1,2-b]quinoxaline as non-viral gene vectors with two-photon property for enhanced DNA/siRNA delivery and bioimaging

Bioorg Chem. 2021 Aug:113:104983. doi: 10.1016/j.bioorg.2021.104983. Epub 2021 May 11.

Authors

Jin-Yu Liu¹, Xu-Ying Liu¹, Rui Liu¹, Fang Tang¹, Jing-Bo Yang¹, Quan Tang¹, Zhong-Lin Lu², Hai-Jun Qiao³, Lan He⁴

Affiliations

¹ Key Laboratory of Radiopharmaceutics, Ministry of Education, College of Chemistry, Beijing Normal University, Beijing 100875, China.
² Key Laboratory of Radiopharmaceutics, Ministry of Education, College of Chemistry, Beijing Normal University, Beijing 100875, China. Electronic address: luzl@bnu.edu.cn.
³ College of Science, Gansu Agricultural University, Lanzhou 730070, China. Electronic address: qiaohj1999@126.com.
⁴ China National Institute for Food and Drug Control, Institute of Chemical Drug Control, TianTanXiLi 2, Beijing 100050, China. Electronic address: helan1961@aliyun.com.

PMID: 34029935
DOI: 10.1016/j.bioorg.2021.104983

Abstract

Two-photon fluorescent Acenaphtho[1,2-b]quinoxaline (ANQ) and the hydrophilic di-(triazole-[12]aneN₃) moieties were combined through an alkyl chain (ANQ-A-M) or a β-hairpin motif with two aromatic γ-amino acid residues (ANQ-H-M) to explore their capabilities for in vitro and in vivo gene delivery and tracing. ANQ-A-M and ANQ-H-M showed the same maximum absorption at 420 nm, and their fluorescent intensities around 650 nm were varied in different solvents and became poor in the protic solvents. Gel electrophoresis assays indicated that both compounds completely retarded the migration of pDNA at 20 μM in the presence of DOPE. However, the DNA condensation with ANQ-H-M was not reversible, and the particle size of the corresponding complexes were larger indicated from the SEM and DLS measurements. In vitro transfections indicated ANQ-A-M/DOPE achieved Luciferase and GFP expressions were to be 7.9- and 5.7-fold of those by Lipo2000 in A549 cells respectively. However, ANQ-H-M showed very poor transfection efficiency in Luciferase expression. With the help of single/two-photon fluorescence imaging it clearly demonstrated that the successful transfection of ANQ-A-M was attributed to its cellular uptake, apparent lysosomal escape, and reversible release of DNA; and the poor transfection of ANQ-H-M was resulted from the aggregation of the DNA complexes which prevented them from the cellular uptake, and also the strong binding ability which is not easy to release DNA. ANQ-A-M/DOPE also exhibited robust gene silencing (83% knockdown of Luciferase) and GFP expression (2.47-fold higher) efficiency compared with Lipo2000 in A549 and zebrafish, respectively. The work demonstrated that the linkage structure between fluorescent and di(triazole-[12]aneN₃) played the important role for their gene delivery performance, and that ANQ-A-M represents a vector with the strong transfection efficiency in vitro and in vivo as well as the efficient real time bioimaging properties, which is potential for the development in biomedical research.

Keywords: Biological tracking; Gene transfection; Non-viral gene vector; Two photon property; [12]aneN(3).

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Aniline Compounds / chemical synthesis
Aniline Compounds / chemistry*
DNA / genetics*
Fluorescent Dyes / chemical synthesis
Fluorescent Dyes / chemistry*
Gene Transfer Techniques*
Genetic Vectors / chemical synthesis
Genetic Vectors / chemistry
Optical Imaging*
Photons*
Quinoxalines / chemical synthesis
Quinoxalines / chemistry*
RNA, Small Interfering / genetics*

Substances

Aniline Compounds
Fluorescent Dyes
Quinoxalines
RNA, Small Interfering
DNA