Imaging C-Fos Gene Expression in Burns Using Lipid Coated Spion Nanoparticles.

Aristarchos Papagiannaros, Valeria Righi, George G Day, Laurence G Rahme, Philip K Liu, Alan J Fischman, Ronald G Tompkins, A Aria Tzika
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Abstract

MR imaging of gene transcription is important as it should enable the non-invasive detection of mRNA alterations in disease. A range of MRI methods have been proposed for in vivo molecular imaging of cells based on the use of ultra-small super-paramagnetic iron oxide (USPIO) nanoparticles and related susceptibility weighted imaging methods. Although immunohistochemistry can robustly differentiate the expression of protein variants, there is currently no direct gene assay technique that is capable of differentiating established to differentiate the induction profiles of c-Fos mRNA in vivo. To visualize the differential FosB gene expression profile in vivo after burn trauma, we developed MR probes that link the T2* contrast agent [superparamagnetic iron oxide nanoparticles (SPION)] with an oligodeoxynucleotide (ODN) sequence complementary to FosB mRNA to visualize endogenous mRNA targets via in vivo hybridization. The presence of this SPION-ODN probe in cells results in localized signal reduction in T2*-weighted MR images, in which the rate of signal reduction (R2*) reflects the regional iron concentration at different stages of amphetamine (AMPH) exposure in living mouse tissue. Our aim was to produce a superior contrast agent that can be administered using systemic as opposed to local administration and which will target and accumulate at sites of burn injury. Specifically, we developed and evaluated a PEGylated lipid coated MR probe with ultra-small super-paramagnetic iron oxide nanoparticles (USPION, a T2 susceptibility agent) coated with cationic fusogenic lipids, used for cell transfection and gene delivery and covalently linked to a phosphorothioate modified oligodeoxynucleotide (sODN) complementary to c-Fos mRNA (SPION-cFos) and used the agent to image mice with leg burns. Our study demonstrated the feasibility of monitoring burn injury using MR imaging of c-Fos transcription in vivo, in a clinically relevant mouse model of burn injury for the first time.

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利用脂质包被的螺旋纳米粒子成像烧伤C-Fos基因表达。
基因转录的MR成像是重要的,因为它应该能够非侵入性地检测疾病中的mRNA变化。基于超小超顺磁性氧化铁(USPIO)纳米颗粒和相关的磁化率加权成像方法,已经提出了一系列MRI方法用于细胞的体内分子成像。虽然免疫组织化学可以有效地区分蛋白变异的表达,但目前还没有能够区分体内c-Fos mRNA诱导谱的直接基因检测技术。为了可视化烧伤后FosB基因在体内的差异表达谱,我们开发了MR探针,将T2*造影剂[超顺磁性氧化铁纳米颗粒(SPION)]与FosB mRNA互补的寡脱氧核苷酸(ODN)序列连接起来,通过体内杂交来可视化内源性mRNA靶点。spon - odn探针在细胞中的存在导致T2*加权MR图像中的局部信号减少,其中信号减少率(R2*)反映了活鼠组织中安非他明(AMPH)暴露不同阶段的区域铁浓度。我们的目的是生产一种优异的造影剂,它可以全身施用而不是局部施用,它可以靶向烧伤部位并在烧伤部位积累。具体来说,我们开发并评估了一种聚乙二醇化脂质包被MR探针,该探针用阳离子促聚变脂质包被的超小超顺磁性氧化铁纳米颗粒(USPION,一种T2易感性剂)包裹,用于细胞转染和基因传递,共价连接到与c-Fos mRNA互补的硫代修饰寡脱氧核苷酸(sODN) (SPION-cFos),并使用该试剂对腿部烧伤的小鼠进行成像。我们的研究首次在临床相关的烧伤小鼠模型中证明了利用体内c-Fos转录的MR成像监测烧伤损伤的可行性。
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