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DNA标记金纳米颗粒的飞秒激光脉冲激发:建立用于生物应用的定量局部纳米温度计。

Femtosecond Laser Pulse Excitation of DNA-Labeled Gold Nanoparticles: Establishing a Quantitative Local Nanothermometer for Biological Applications.

作者信息

Hastman David A, Melinger Joseph S, Aragonés Guillermo Lasarte, Cunningham Paul D, Chiriboga Matthew, Salvato Zachary J, Salvato Thomas M, Brown Carl W, Mathur Divita, Medintz Igor L, Oh Eunkeu, Díaz Sebastián A

机构信息

Fischell Department of Bioengineering, University of Maryland, College Park, Maryland 20742, United States.

出版信息

ACS Nano. 2020 Jul 28;14(7):8570-8583. doi: 10.1021/acsnano.0c02899. Epub 2020 Jul 17.

DOI:10.1021/acsnano.0c02899
PMID:32677822
Abstract

Femtosecond (fs) laser pulsed excitation of plasmonic nanoparticle (NP)-biomolecule conjugates is a promising method to locally heat biological materials. Studies have demonstrated that fs pulses of light can modulate the activity of DNA or proteins when attached to plasmonic NPs; however, the precision over subsequent biological function remains largely undetermined. Specifically, the temperature the localized biomolecules "experience" remains unknown. We used 55 nm gold nanoparticles (AuNPs) displaying double-stranded (ds) DNA to examine how, for dsDNA with different melting temperatures, the laser pulse energy fluence and bulk solution temperature affect the rate of local DNA denaturation. A universal "template" single-stranded DNA was attached to the AuNP surface, and three dye-labeled probe strands, distinct in length and melting temperature, were hybridized to it creating three individual dsDNA-AuNP bioconjugates. The dye-labeled probe strands were used to quantify the rate and amount of DNA release after a given number of light pulses, which was then correlated to the dsDNA denaturation temperature, resulting in a quantitative nanothermometer. The localized DNA denaturation rate could be modulated by more than threefold over the biologically relevant range of 8-53 °C by varying pulse energy fluence, DNA melting temperature, and surrounding bath temperature. With a modified dissociation equation tailored for this system, a "sensed" temperature parameter was extracted and compared to simulated AuNP temperature profiles. Determining actual biological responses in such systems can allow researchers to design precision nanoscale photothermal heating sources.

摘要

飞秒(fs)激光脉冲激发等离子体纳米颗粒(NP)-生物分子共轭物是一种局部加热生物材料的有前景的方法。研究表明,当附着在等离子体NP上时,飞秒光脉冲可以调节DNA或蛋白质的活性;然而,对后续生物功能的精确控制在很大程度上仍未确定。具体而言,局部生物分子“经历”的温度仍然未知。我们使用展示双链(ds)DNA的55纳米金纳米颗粒(AuNP)来研究,对于具有不同解链温度的dsDNA,激光脉冲能量通量和本体溶液温度如何影响局部DNA变性速率。一条通用的“模板”单链DNA附着在AuNP表面,三条长度和解链温度不同的染料标记探针链与之杂交,形成三种不同的dsDNA-AuNP生物共轭物。染料标记的探针链用于量化给定数量光脉冲后DNA释放的速率和量,然后将其与dsDNA变性温度相关联,从而得到一个定量纳米温度计。通过改变脉冲能量通量、DNA解链温度和周围浴温,在8-53°C的生物学相关范围内,局部DNA变性速率可被调节超过三倍。通过为该系统量身定制的修正解离方程,提取了一个“感知”温度参数,并与模拟的AuNP温度分布进行了比较。确定此类系统中的实际生物反应可以使研究人员设计出精确的纳米级光热加热源。

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