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铁蛋白作为一种新型的光声分子成像报告基因。

Ferritin as a novel reporter gene for photoacoustic molecular imaging.

机构信息

Center for Ultrasound Molecular Imaging and Therapeutics, University of Pittsburgh and University of Pittsburgh Medical Center, Pittsburgh, Pennsylvania 15213, USA.

出版信息

Cytometry A. 2012 Oct;81(10):910-5. doi: 10.1002/cyto.a.22160. Epub 2012 Sep 4.

Abstract

Reporter genes may serve as endogenous contrast agents in the field of photoacoustic (PA) molecular imaging (PMI), enabling greater characterization of detailed cellular processes and disease progression. To demonstrate the feasibility of using ferritin as a reporter gene, human melanoma SK-24 (SK-MEL-24) cells were co-transfected with plasmid expressing human heavy chain ferritin (H-FT) and plasmid expressing enhanced green fluorescent protein (pEGFP-C1) using lipofectamine™ 2000. Nontransfected SK-MEL-24 cells served as a negative control. Fluorescent imaging of GFP confirmed transfection and transgene expression in co-transfected cells. To detect iron accumulation due to ferritin overexpression in SK-MEL-24 cells, a focused high-frequency ultrasonic transducer (60 MHz, f/1.5), synchronized to a pulsed laser (fluence < 5 mJ/cm(2)) was used to scan the PA signal at a wide range NIR wavelengths (850-950 nm). PA signal intensity from H-FT transfected SK-MEL-24 cells was about 5-9 dB higher than nontransfected SK-MEL-24 cells at 850-950 nm. Immunofluorescence and RT-PCR analysis both indicate high levels of ferritin expression in H-FT transfected SK-MEL24 cells, with little ferritin expression in nontransfected SK-MEL-24 cells. In this study, the feasibility of using ferritin as a reporter gene for PMI has been demonstrated in vitro. The use of ferritin as a reporter gene represents a novel concept for PMI using an endogenous contrast agent and may provide various opportunities for molecular imaging and basic science research.

摘要

报告基因可用作光声(PA)分子成像(PMI)领域的内源性对比剂,从而能够更详细地描述细胞过程和疾病进展。为了证明使用铁蛋白作为报告基因的可行性,用人重链铁蛋白(H-FT)表达质粒和增强型绿色荧光蛋白(pEGFP-C1)表达质粒通过 Lipofectamine™2000 共转染人黑色素瘤 SK-24(SK-MEL-24)细胞。未转染的 SK-MEL-24 细胞作为阴性对照。GFP 的荧光成像证实了共转染细胞中的转染和转基因表达。为了检测由于铁蛋白过表达在 SK-MEL-24 细胞中引起的铁积累,使用聚焦高频超声换能器(60MHz,f/1.5),与脉冲激光(<5mJ/cm 2 )同步,在宽范围近红外波长(850-950nm)下扫描 PA 信号。在 850-950nm 时,H-FT 转染的 SK-MEL-24 细胞的 PA 信号强度比未转染的 SK-MEL-24 细胞高约 5-9dB。免疫荧光和 RT-PCR 分析均表明 H-FT 转染的 SK-MEL24 细胞中铁蛋白表达水平较高,而未转染的 SK-MEL-24 细胞中铁蛋白表达水平较低。在这项研究中,已经在体外证明了使用铁蛋白作为报告基因进行 PMI 的可行性。使用铁蛋白作为报告基因代表了使用内源性对比剂进行 PMI 的新概念,可为分子成像和基础科学研究提供各种机会。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/a737/3626421/a915962697d9/nihms456188f1.jpg

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