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1
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2
In vivo molecular imaging of cancer with a quenching near-infrared fluorescent probe using conjugates of monoclonal antibodies and indocyanine green.使用单克隆抗体与吲哚菁绿的缀合物,通过淬灭型近红外荧光探针进行癌症的体内分子成像。
Cancer Res. 2009 Feb 15;69(4):1268-72. doi: 10.1158/0008-5472.CAN-08-3116. Epub 2009 Jan 27.
3
Tumor-specific detection of an optically targeted antibody combined with a quencher-conjugated neutravidin "quencher-chaser": a dual "quench and chase" strategy to improve target to nontarget ratios for molecular imaging of cancer.一种结合了淬灭剂偶联中性抗生物素蛋白的光学靶向抗体的肿瘤特异性检测方法——“淬灭-追踪”:一种双重“淬灭与追踪”策略,用于提高癌症分子成像中的靶标与非靶标比率。
Bioconjug Chem. 2009 Jan;20(1):147-54. doi: 10.1021/bc8003765.
4
Cell culture and xenograft-bearing animal studies of radiolabeled antisense DNA carrier nanoparticles with streptavidin as a linker.以链霉亲和素作为连接物的放射性标记反义DNA载体纳米颗粒的细胞培养和荷瘤动物研究。
J Nucl Med. 2007 Nov;48(11):1845-52. doi: 10.2967/jnumed.106.039339.
5
Optical antisense imaging of tumor with fluorescent DNA duplexes.利用荧光DNA双链体对肿瘤进行光学反义成像。
Bioconjug Chem. 2007 Nov-Dec;18(6):1905-11. doi: 10.1021/bc700221d. Epub 2007 Oct 17.
6
Whole-body optical imaging in animal models to assess cancer development and progression.在动物模型中进行全身光学成像以评估癌症的发生和进展。
Clin Cancer Res. 2007 Jun 15;13(12):3490-7. doi: 10.1158/1078-0432.CCR-07-0402.
7
Improved delivery in cell culture of radiolabeled antisense DNAs by duplex formation.
Mol Imaging Biol. 2006 Sep-Oct;8(5):278-83. doi: 10.1007/s11307-006-0050-7.
8
Oligonucleotide-modified gold nanoparticles for intracellular gene regulation.用于细胞内基因调控的寡核苷酸修饰金纳米颗粒。
Science. 2006 May 19;312(5776):1027-30. doi: 10.1126/science.1125559.
9
Near-infrared fluorescent deoxyglucose analogue for tumor optical imaging in cell culture and living mice.用于细胞培养和活体小鼠肿瘤光学成像的近红外荧光脱氧葡萄糖类似物
Bioconjug Chem. 2006 May-Jun;17(3):662-9. doi: 10.1021/bc050345c.
10
The influence of chemical structure of DNA and other oligomer radiopharmaceuticals on tumor delivery.
Curr Opin Mol Ther. 2006 Apr;8(2):136-43.

使用改进的荧光DNA双链体探针在体内进行光学反义肿瘤靶向。

Optical antisense tumor targeting in vivo with an improved fluorescent DNA duplex probe.

作者信息

Liang Minmin, Liu Xinrong, Cheng Dengfeng, Nakamura Kayoko, Wang Yi, Dou Shuping, Liu Guozheng, Rusckowski Mary, Hnatowich Donald J

机构信息

Department of Radiology, University of Massachusetts Medical School, Worcester, Massachusetts, USA.

出版信息

Bioconjug Chem. 2009 Jun;20(6):1223-7. doi: 10.1021/bc9000933.

DOI:10.1021/bc9000933
PMID:19489604
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC4793961/
Abstract

Fluorescent conjugated DNA oligonucleotides for antisense targeting of mRNA has the potential of improving tumor/normal tissue ratios over that achievable by nuclear antisense imaging. By conjugating the Cy5.5 emitter to the 3' equivalent end of a 25 mer phosphorothioate (PS) antisense major DNA and hybridizing with a shorter 18 mer phosphodiester (PO) complementary minor DNA (cDNA) with the Black Hole inhibitor BHQ3 on its 5' end (i.e., PS DNA25-Cy5.5/PO cDNA18-BHQ3), we previously achieved antisense optical imaging in mice as a proof of this concept. In a process of optimization, we have now evaluated the stability of a small series of duplexes with variable-length minor strands. From these results, a new study anti-mdr1 antisense duplex was selected with a 10 mer minor strand (i.e., PS DNA25-Cy5.5/PO cDNA10-BHQ3). The new study duplex shows stability in serum environments at 37 degrees C and provides a dramatically enhanced fluorescence in KB-G2 (pgp++) cells when compared with KB-31 (pgp+/-) as evidence of antisense dissociation at its mdr1 mRNA target. The duplex was also administered to KB-G2 tumor bearing mice, and when compared to the duplex used previously, the fluorescence from the tumor thigh was more obvious and the tumor-to-background fluorescence ratio was improved. In conclusion, by a process designed to optimize the duplex for optical antisense tumor targeting, the fluorescence signal was improved both in cells and in tumored mice.

摘要

用于mRNA反义靶向的荧光共轭DNA寡核苷酸有潜力提高肿瘤/正常组织比率,超过核反义成像所能达到的水平。通过将Cy5.5发射体与25聚体硫代磷酸酯(PS)反义主要DNA的3'等效末端共轭,并与较短的18聚体磷酸二酯(PO)互补次要DNA(cDNA)杂交,该次要DNA在其5'末端带有黑洞抑制剂BHQ3(即PS DNA25-Cy5.5/PO cDNA18-BHQ3),我们之前在小鼠中实现了反义光学成像,以此证明这一概念。在优化过程中,我们现在评估了一小系列具有可变长度次要链的双链体的稳定性。根据这些结果,选择了一种新的研究性抗mdr1反义双链体,其带有10聚体次要链(即PS DNA25-Cy5.5/PO cDNA10-BHQ3)。新的研究性双链体在37摄氏度的血清环境中显示出稳定性,并且与KB-31(pgp+/-)相比,在KB-G2(pgp++)细胞中提供了显著增强的荧光,作为其在mdr1 mRNA靶点处反义解离的证据。该双链体也被施用于携带KB-G2肿瘤的小鼠,与之前使用的双链体相比,来自肿瘤大腿的荧光更明显,肿瘤与背景的荧光比率得到改善。总之,通过旨在优化用于光学反义肿瘤靶向的双链体的过程,荧光信号在细胞和荷瘤小鼠中均得到改善。