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用于光动力疗法的金纳米结构叶绿素e6的合成与表征。

Synthesis and characterization of gold nanostructured Chorin e6 for Photodynamic Therapy.

作者信息

Vieira L, Castilho M L, Ferreira I, Ferreira-Strixino J, Hewitt K C, Raniero L

机构信息

Laboratório de Nanossensores, Universidade do Vale do Paraíba, Av. Shishima Hifumi, 2911, São José dos Campos, São Paulo, 12244-000, Brazil.

Department of Physics and Atmospheric Science, Dalhousie University, 6310 Coburg Road, Halifax, Nova Scotia, B3H 4R2, Canada.

出版信息

Photodiagnosis Photodyn Ther. 2017 Jun;18:6-11. doi: 10.1016/j.pdpdt.2016.12.012. Epub 2017 Jan 10.

Abstract

Photodynamic therapy is an alternative treatment for cancer based on cellular uptake of a photosensitizer, illuminated with an appropriate wavelength in the presence of oxygen. A cascade of reactions generates reactive oxygen species leading to cell death. Using carbodiimide chemistry, chlorin e6 (Ce6) was covalently bonded to thiourea, and (via the sulphur end group) to gold nanoparticles (AuNPs), forming the Ce6-AuNP complex. Ce6 absorbs in the range 650-680nm, where the coefficient of biological tissue absorption is low (part of the therapeutic window), which is ideal for biological application. Transmission Electron Microscopy, UV-vis spectroscopy, Fourier transform Infrared Spectroscopy and Zeta potential measurements were completed to characterize the Ce6-AuNP complex. The bare AuNPs have an average diameter of 18±4nm. A line of human breast carcinoma cells (MDA-MB-468) was used to determine whether Ce6 functionalization to AuNPs potentiate its activity. Trypan blue assays were used to assess cell viability. In the absence of light, Ce6 either alone or bounded to AuNPs was not cytotoxic. When irradiated at 660nm, the cytotoxicity of Ce6-AuNP was higher than Ce6 alone for MDA-MB-468 cells using 4h incubation. AuNPs without Ce6 showed no cytotoxic.

摘要

光动力疗法是一种癌症替代治疗方法,其基于细胞摄取光敏剂,并在有氧存在的情况下用适当波长的光照射。一系列反应会产生活性氧,导致细胞死亡。利用碳二亚胺化学方法,将二氢卟吩e6(Ce6)共价连接到硫脲上,并(通过硫端基)连接到金纳米颗粒(AuNP)上,形成Ce6-AuNP复合物。Ce6在650-680nm范围内吸收,在此生物组织吸收系数较低(治疗窗口的一部分),这对于生物应用来说是理想的。完成了透射电子显微镜、紫外可见光谱、傅里叶变换红外光谱和zeta电位测量,以表征Ce6-AuNP复合物。裸露的AuNP平均直径为18±4nm。使用人乳腺癌细胞系(MDA-MB-468)来确定Ce6对AuNP的功能化是否增强其活性。使用台盼蓝试验评估细胞活力。在无光的情况下,单独的Ce6或与AuNP结合的Ce6均无细胞毒性。当在660nm照射时,对于MDA-MB-468细胞,使用4小时孵育,Ce6-AuNP的细胞毒性高于单独的Ce6。没有Ce6的AuNP没有显示出细胞毒性。

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